Efficient Production of Steviol Glycosides in Recombinant Hosts
Recombinant microorganisms are disclosed that produce steviol glycosides and have altered expression of one or more endogenous transporter or transcription factor genes, or that overexpress one or more heterologous transporters, leading to increased excretion of steviol glycosides of interest.
This application claims the benefit of U.S. Provisional Application No. 61/763,290, filed Feb. 11, 2013, and U.S. Provisional Application No. 61/763,308, filed Feb. 11, 2013, the disclosures of each of which are incorporated by reference.
TECHNICAL FIELDThis disclosure relates to the recombinant production of steviol glycosides and isolation methods thereof. In particular, this disclosure relates to the production of steviol glycosides such as rebaudioside A (RebA), rebaudioside B (RebB), rebaudioside D (RebD), rebaudioside E (RebE) and rebaudioside M (RebM) by recombinant hosts such as recombinant microorganisms. This disclosure also relates to modifications to transport systems in the recombinant host to increase production, excretion or both of such steviol glycosides.
BACKGROUNDSweeteners are well known as ingredients used most commonly in the food, beverage, or confectionary industries. The sweetener can either be incorporated into a final food product during production or for stand-alone use, when appropriately diluted, as a tabletop sweetener or an at-home replacement for sugars in baking. Sweeteners include natural sweeteners such as sucrose, high fructose corn syrup, molasses, maple syrup, and honey and artificial sweeteners such as aspartame, saccharine and sucralose. Stevia extract is a natural sweetener that can be isolated and extracted from a perennial shrub, Stevia rebaudiana. Stevia is commonly grown in South America and Asia for commercial production of stevia extract. Stevia extract, purified to various degrees, is used commercially as a high intensity sweetener in foods and in blends or alone as a tabletop sweetener.
Extracts of the Stevia plant contain rebaudiosides and other steviol glycosides that contribute to the sweet flavor, although the amount of each glycoside often varies among different production batches. Typically, stevioside and rebaudioside A are the primary compounds in commercially-produced stevia extracts. Stevioside is reported to have a more bitter and less sweet taste than rebaudioside A. The composition of stevia extract can vary from lot to lot depending on the soil and climate in which the plants are grown. Depending upon the sourced plant, the climate conditions, and the extraction process, the amount of rebaudioside A in commercial preparations is reported to vary from 20 to 97% of the total steviol glycoside content. Other steviol glycosides are present in varying amounts in stevia extracts. For example, rebaudioside B is typically present at less than 1-2%, whereas rebaudioside C can be present at levels as high as 7-15%. Rebaudioside D is typically present in levels of 2% or less, Rebaudioside M is typically present in trace levels (<0.10%), and rebaudioside F is typically present in compositions at 3.5% or less of the total steviol glycosides. The amount of the minor steviol glycosides can affect the flavor profile of a Stevia extract.
Chemical structures for several of the compounds found in Stevia extracts are shown in
This document describes materials and methods that can be used to efficiently produce steviol glycoside compositions, by modification of transport systems in the recombinant host that are involved in excretion of steviol glycosides. In some embodiments, recombinant hosts described herein can produce at least one steviol glycoside and express a heterologous transporter such as a transporter that actively excretes antibiotics. In some embodiments, recombinant hosts described herein produce at least one steviol glycoside and the expression of an endogenous transporter gene is altered in the host and/or expression of a transcription factor gene is altered, wherein the transcription factor regulates expression of at least one endogenous transporter gene. Altering expression of endogenous transporters that actively secrete antibiotics is particularly useful. In some embodiments, expression of a plurality of endogenous transporter genes, transcription factor genes, or both is altered. Such recombinant hosts can include one or more biosynthesis genes whose expression results in production of steviol glycosides such as rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E, or rebaudioside M. Such biosynthesis genes include 13-monoglucoside beta 1,2 glycosyltransferases and/or 19-monoglucoside-beta 1,2-glucosyltransferases (e.g., 91D2e and EUGT11) and other UDP glycosyl transferases such as UGT74G1, UGT76G1, and/or UGT85C2, to allow the production of steviol glycosides in recombinant hosts.
This document also features methods for producing a steviol glycoside product. These methods include fermention methods using a recombinant microorganism (e.g., Saccharomyces cerevisiae) having altered expression of an endogenous transporter gene to produce the steviol glycoside, which, optionally, then can be purified from the fermentation broth.
In one aspect, this document features methods for identifying a gene or genes that affect excretion of a steviol glycoside as well as using recombinant embodiments thereof to genetically engineer recombinant cells, particularly microorganisms, to produce steviol glycosides as set forth herein. These methods include modifying expression of at least one endogenous transporter in a recombinant microorganism capable of producing steviol or a steviol glycoside; culturing the modified microorganism in a medium under conditions in which the steviol glycoside is synthesized; and measuring the amount of extracellular and/or intracellular steviol glycoside produced during the culturing step relative to the amount produced by a corresponding microorganism lacking the modification, thereby identifying the endogenous transporter as affecting excretion of the steviol glycoside.
This document also features alternative methods for identifying a gene or genes that affect excretion of a steviol glycoside as well as using recombinant embodiments thereof to genetically engineer recombinant cells, particularly microorganisms, to produce steviol glycosides as set forth herein. The method includes modifying expression of at least one endogenous transporter in a microorganism to generate a modified microorganism; introducing one or more recombinant genes capable of producing a steviol glycoside into the modified microorganism; culturing the modified microorganism in a medium under conditions in which the steviol glycoside is synthesized; and measuring the amount of extracellular and/or intracellular steviol glycoside produced during the culturing step relative to the amount produced by a corresponding microorganism lacking the modification, thereby identifying the endogenous transporter as affecting excretion of the steviol glycoside.
This document also features yet additional methods for identifying a gene or genes affecting excretion of a steviol glycoside. These methods include modifying expression of at least one endogenous transcription factor that regulates expression of an endogenous transporter gene in a recombinant microorganism capable of producing steviol or a steviol glycoside; culturing the modified microorganism in a medium under conditions in which the steviol glycoside is synthesized; and measuring the amount of extracellular and/or intracellular steviol glycoside produced during the culturing step relative to the amount produced by a corresponding microorganism lacking the modification, thereby identifying the transcription factor as affecting excretion of the steviol glycoside.
In another embodiment, this document features still further methods for identifying a gene or genes affecting excretion of a steviol glycoside. These methods include modifying expression of at least one endogenous transcription factor that regulates expression of an endogenous transporter gene in a microorganism to generate a modified microorganism; introducing one or more recombinant genes capable of producing a steviol glycoside into the modified microorganism; culturing the modified microorganism in a medium under conditions in which the steviol glycoside is synthesized; and measuring the amount of extracellular and/or intracellular steviol glycoside produced during the culturing step relative to the amount produced by a corresponding microorganism lacking the modification, thereby identifying the transcription factor as affecting excretion of the steviol glycoside.
In another aspect, this document relates to methods of increasing excretion of steviol glycosides by modifying expression of a gene or genes identified to affect excretion of a steviol glycoside, wherein the expression of the identified genes would be modified in recombinant microorganisms capable of producing steviol or a steviol glycoside. In some embodiments the gene or genes identified are endogenous genes that can be overexpressed or repressed by replacing the endogenous promoter with a stronger promoter or weaker promoter, respectively, as compared to the wildtype promoter. In other embodiments, the gene or genes identified can be endogenous genes that are overexpressed or repressed by introducing exogenous DNA engineered to overexpress or repress the endogenous gene or genes. In yet another embodiment, homologous or orthologous genes of an identified endogenous gene can be overexpressed. In a further embodiment, the endogenous gene can be induced to be overexpressed or repressed using native mechanisms to the recombinant microorganism (e.g. heat shock, stress, heavy metal or antibiotic exposure).
In any of the methods described herein, modifying expression can include increasing or decreasing expression or activity of the endogenous transporter or transcription factor at least 5% above or below the level of expression observed in a corresponding unmodified microorganism.
In any of the methods described herein, the recombinant genes can include one or more of the following genes encoded by exogenous nucleic acids:
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- (a) one or more recombinant genes encoding a sucrose transporter and a sucrose synthase;
- (b) a nucleic acid encoding a GGPPS polypeptide;
- (c) a nucleic acid encoding an ent-copalyl diphosphate synthase polypeptide;
- (d) a nucleic acid encoding a kaurene synthase (KS) polypeptide;
- (e) a nucleic acid encoding a kaurene oxidase (KO) polypeptide;
- (f) a nucleic acid encoding a steviol synthase (KAH) polypeptide;
- (g) a nucleic acid encoding a cytochrome P450 reductase (CPR) polypeptide; and also in appropriate combination,
- (h) a nucleic acid encoding a UGT85C2 polypeptide;
- (i) a nucleic acid encoding a UGT76G1 polypeptide;
- (j) a nucleic acid encoding a UGT74G1 polypeptide;
- (k) a nucleic acid encoding a UGT91D2 polypeptide; or
- (l) a nucleic acid encoding a EUGT11 polypeptide.
This document features methods for identifying a gene or genes affecting excretion of a steviol glycoside as well as using recombinant embodiments thereof to genetically engineer recombinant cells, particularly microorganisms, to produce steviol glycosides as set forth herein. The method includes expressing at least one heterologous transporter in a recombinant microorganism capable of producing steviol or a steviol glycoside; culturing the microorganism in a medium under conditions in which the steviol glycoside is synthesized; and measuring the amount of extracellular and/or intracellular steviol glycoside produced during the culturing step relative to the amount produced by a corresponding microorganism lacking the modification, thereby identifying a heterologous transporter affecting excretion of the steviol glycoside. The heterologous transporter can be a Stevia transporter.
In any of the methods described herein, the microorganism can include, but is not limited to suitable species from a genus selected from the group consisting of Agaricus, Aspergillus, Bacillus, Candida, Corynebacterium, Escherichia, Fusarium/Gibberella, Kluyveromyces, Laetiporus, Lentinus, Phaffia, Phanerochaete, Pichia, Physcomitrella, Rhodoturula, Saccharomyces, Schizosaccharomyces, Sphaceloma, Xanthophyllomyces and Yarrowia. Exemplary species from such genera include, but are not limited to, Saccharomyces cerevisiae, Schizosaccharomyces pombe, Yarrowia lipolytica, Candida glabrata, Ashbya gossypii, Cyberlindnera jadinii, Pichia pastoris, Kluyveromyces lactis, Hansenula polymorpha, Candida boidinii, Arxula adeninivorans, Xanthophyllomyces dendrorhous or Candida albicans species.
These and other features and advantages of the present invention will be more fully understood from the following detailed description of the invention taken together with the accompanying claims. It is noted that the scope of the claims is defined by the recitations therein and not by the specific discussion of features and advantages set forth in the present description.
Unless otherwise defined, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which the invention belongs. Although methods and materials similar or equivalent to those described herein can be used to practice the invention, suitable methods and materials are described below. All publications, patent applications, patents, and other references mentioned herein are incorporated by reference in their entirety. In case of conflict, the present specification, including definitions, will control. In addition, the materials, methods, and examples are illustrative only and are not intended to be limiting. Other features and advantages of the invention will be apparent from the following detailed description. Applicants reserve the right to alternatively claim any disclosed invention using the transitional phrase “comprising,” “consisting essentially of,” or “consisting of,” according to standard practice in patent law.
Methods well known to those skilled in the art can be used to construct genetic expression constructs and recombinant cells according to this invention. These methods include in vitro recombinant DNA techniques, synthetic techniques, in vivo recombination techniques, and polymerase chain reaction (PCR) techniques. See, for example, techniques as described in Maniatis et al., 1989, MOLECULAR CLONING: A LABORATORY MANUAL, Cold Spring Harbor Laboratory, New York; Ausubel et al., 1989, CURRENT PROTOCOLS IN MOLECULAR BIOLOGY, Greene Publishing Associates and Wiley Interscience, New York, and PCR Protocols: A Guide to Methods and Applications (Innis et al., 1990, Academic Press, San Diego, Calif.).
Before describing the present invention in detail, a number of terms will be defined. As used herein, the singular forms “a”, “an”, and “the” include plural referents unless the context clearly dictates otherwise. For example, reference to a “nucleic acid” means one or more nucleic acids.
It is noted that terms like “preferably”, “commonly”, and “typically” are not utilized herein to limit the scope of the claimed invention or to imply that certain features are critical, essential, or even important to the structure or function of the claimed invention. Rather, these terms are merely intended to highlight alternative or additional features that can or cannot be utilized in a particular embodiment of the present invention.
For the purposes of describing and defining the present invention it is noted that the term “substantially” is utilized herein to represent the inherent degree of uncertainty that can be attributed to any quantitative comparison, value, measurement, or other representation. The term “substantially” is also utilized herein to represent the degree by which a quantitative representation can vary from a stated reference without resulting in a change in the basic function of the subject matter at issue.
As used herein, the terms “polynucleotide”, “nucleotide”, “oligonucleotide”, and “nucleic acid” can be used interchangeably to refer to nucleic acid comprising DNA, RNA, derivatives thereof, or combinations thereof.
As used herein, the term “and/or” is utilized to describe multiple components in combination or exclusive of one another. For example, “x, y, and/or z” can refer to “x” alone, “y” alone, “z” alone, “x, y, and z,” “(x and y) or z,” “x and (y or z),” or “x or y or z.” In some embodiments, “and/or” is used to refer to the exogenous nucleic acids that a recombinant cell comprises, wherein a recombinant cell comprises one or more exogenous nucleic acids selected from a group. In some embodiments, “and/or” is used to refer to production of steviol glycosides, wherein one or more steviol glycosides selected from a group are produced. In some embodiments, “and/or” is used to refer to production of steviol glycosides, wherein one or more steviol glycosides are produced through one or more of the following steps: culturing a recombinant microorganism, synthesizing one or more steviol glycosides in a recombinant microorganism, and isolating one or more steviol glycosides.
This document describes materials and methods that can be used to efficiently produce steviol glycoside compositions, by modification of transport systems in the recombinant host that are involved in excretion of steviol glycosides. In some embodiments, recombinant hosts described herein can produce at least one steviol glycoside and express a heterologous transporter such as a transporter that actively excretes antibiotics. In some embodiments, recombinant hosts described herein produce at least one steviol glycoside and the expression of an endogenous transporter gene is altered in the host and/or expression of a transcription factor gene is altered, wherein the transcription factor regulates expression of at least one endogenous transporter gene. Altering expression of endogenous transporters that actively secrete antibiotics is particularly useful. In some embodiments, expression of a plurality of endogenous transporter genes, transcription factor genes, or both is altered. Such recombinant hosts can include one or more biosynthesis genes whose expression results in production of steviol glycosides such as rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E or rebaudioside M. Such biosynthesis genes include 13-monoglucoside beta 1,2 glycosyltransferases and/or 19-monoglucoside-beta 1,2-glucosyltransferases (e.g., UGT91D2e and EUGT11) and other UDP glycosyl transferases such as UGT74G1, UGT76G1, and/or UGT85C2, to allow the production of steviol glycosides in recombinant hosts.
In one aspect, this document relates to a recombinant microorganism capable of synthesizing at least one steviol glycoside comprising modified expression of at least one gene that is a transporter gene, a transcription factor gene that regulates expression of at least one transporter gene, or both. In one embodiment, the transporter gene can be an endogenous transporter gene or a heterologous transporter gene. In another embodiment, the transporter gene can encodes an ABC transporter or an MFS transporter, wherein the transporter gene transporter gene or transcription factor gene is PDR1, PDR3, PDR5, PDR8, PDR10, PDR11, PDR12, PDR15, PDR18, YOR1, AUS1, SNQ2, PDR12, STE6, THI73, NFT1, ADP1, FLR1, QDR1, QDR2, QDR3, DTR1, TPO1, TPO2, TPO4, TPO3, AQR1, AZR1, ENB1, SGE1, YHK8, GEX2, HOL1, ATR1, HXT11, ENB1, ARN1, ARN2, SSU1, THI7, TPN1, SEO1, SIT1 or DTR1.
In another embodiment, the modified expression of a target gene in the recombinant mircroorganism comprises overexpressing or reduced expression of the transporter gene or the transcription factor gene. In yet another embodiment, the recombinant microorganism comprises overexpressing or reduced expression of a plurality of endogenous transporter genes or transcription factor genes. In one embodiment, the recombinant microorganism comprises reduced expression of PDR5, PDR10, PDR15 and SNQ2 genes by disrupting each gene locus. In another embodiment, the recombinant microorganism comprises reduced expression of PDR1, PDR3, PDR5, PDR10, PDR15, SNQ2 and TPO1 genes by disrupting each gene locus.
In a further embodiment, the recombinant microorganism of this document comprises one or more of the following exogenous nucleic acids: one or more recombinant genes encoding a sucrose transporter and a sucrose synthase; a nucleic acid encoding a GGPPS polypeptide; a nucleic acid encoding an ent-copalyl diphosphate synthase polypeptide; a nucleic acid encoding a kaurene synthase (KS) polypeptide; a nucleic acid encoding a kaurene oxidase (KO) polypeptide; a nucleic acid encoding a steviol synthase (KAH) polypeptide; a nucleic acid encoding a cytochrome P450 reductase (CPR)polypeptide; a nucleic acid encoding a UGT85C2 polypeptide; a nucleic acid encoding a UGT76G polypeptide; a nucleic acid encoding a UGT74G1 polypeptide; a nucleic acid encoding a UGT91D2 polypeptide; or a nucleic acid encoding a EUGT11 polypeptide. In one embodiment, the recombinant microorganism, comprises the exogenous nucleic acids encoding UGT85C2, UGT76G1 and UGT91D2 polypeptides. In another embodiment, the recombinant microorganism comprises the exogenous nucleic acids encoding UGT85C2, UGT76G1, UGT74G1, and UGT91D2 polypeptides. In yet another embodiment, the recombinant microorganism comprises the exogenous nucleic acids encoding UGT85C2, UGT76G1, UGT74G1, and EUGT11 polypeptides. In yet another embodiment, the recombinant microorganism comprises the exogenous nucleic acids encoding UGT85C2, UGT76G1, UGT74G1, UGT91D2 (including inter alia 91D2e, 91D2m, 91D2e-b and functional homologs thereof) and EUGT11 polypeptides.
In another aspect, this document relates to a method of producing a Rebaudioside, comprising: culturing the recombinant microorganism described herein in a culture medium, under conditions in which the genes encoding a GGPPS; an ent-copalyl diphosphate synthase (CDPS) polypeptide; a kaurene oxidase (KO) polypeptide; a kaurene synthase (KS) polypeptide; a steviol synthase (KAH) polypeptide; a cytochrome P450 reductase (CPR) polypeptide; a UGT85C2 polypeptide; a UGT74G1 polypeptide; a UGT76G1 polypeptide; a UGT91D2 polypeptide; or a EUGT11 polypeptide are expressed, comprising inducing expression of said genes or constitutively expressing said genes; synthesizing one or more of a compound, comprising the Rebaudioside in the recombinant microorganism; and isolating one or more of the compounds comprising the Rebaudioside. In one embodiment, the Rebaudioside is Rebaudioside A, Rebaudioside B, Rebaudioside D, Rebaudioside E, or Rebaudioside M. In another embodiment, the recombinant microorganism overexpresses YOR1, SNQ2, PDR1 or FLR1.
In one embodiment, the recombinant microorganism is a microorganism described herein is selected from, but not limited to, a genus from Agaricus, Aspergillus, Bacillus, Candida, Corynebacterium, Escherichia, Fusarium/Gibberella, Kluyveromyces, Laetiporus, Lentinus, Phaffia, Phanerochaete, Pichia, Physcomitrella, Rhodoturula, Saccharomyces, Schizosaccharomyces, Sphaceloma, Xanthophyllomyces and Yarrowia. In another embodiment, the recombinant microorganism is a yeast cell from Saccharomyces cerevisiae, Schizosaccharomyces pombe, Yarrowia lipolytica, Candida glabrata, Ashbya gossypii, Cyberlindnera jadinii, Pichia pastoris, Kluyveromyces lactis, Hansenula polymorpha, Candida boidinii, Arxula adeninivorans, Xanthophyllomyces dendrorhous or Candida albicans species.
In yet another aspect, this document relates to a method of affecting excretion of steviol glycosides, comprising: using the methods described herein to produce a steviol glycoside, wherein at least one recombinant gene is expressed, and culturing the recombinant microorganism in a medium under conditions in which the steviol glycoside is synthesized; and expressing at least one gene that is a transporter gene, a transcription factor gene that regulates expression of at least one transporter gene, or both, and isolating the steviol glycoside produced during the culturing step.
I. Steviol and Steviol Glycoside Biosynthesis Polypeptides A. Steviol Biosynthesis PolypeptidesIn addition to expressing heterologous transporter and/or transcription factor genes, or modifying expression of endogenous transporter genes as described above, a host described herein contains and expresses gene products involved in the conversion of isoprenoid precursors to steviol.
The biochemical pathway to produce steviol involves formation of geranylgeranyl diphosphate, cyclization to (-) copalyl diphosphate, followed by oxidation and hydroxylation to form steviol. Thus, conversion of geranylgeranyl diphosphate to steviol in a recombinant microorganism involves the expression of a gene encoding a kaurene synthase (KS), a gene encoding a kaurene oxidase (KO), and a gene encoding a steviol synthetase (KAH). Steviol synthetase also is known as kaurenoic acid 13-hydroxylase.
Suitable KS polypeptides are known. For example, suitable KS enzymes include those made by Stevia rebaudiana, Zea mays, Populus trichocarpa, and Arabidopsis thaliana. See, Table 2 and PCT Application Nos. PCT/US2012/050021 and PCT/US2011/038967, which are incorporated herein by reference in their entirety.
Suitable KG polypeptides are known. For example, suitable KG enzymes include those made by Stevia rebaudiana, Arabidopsis thaliana, Gibberella fujikoroi and Trametes versicolor. See, Table 3 and PCT Application Nos. PCT/US2012/050021 and PCT/US2011/038967, which are incorporated herein by reference in their entirety.
Suitable KAH polypeptides are known. For example, suitable KAH enzymes include those made by Stevia rebaudiana, Arabidopsis thaliana, Vitis vinifera and Medicago trunculata. See, e.g., Table 4, PCT Application Nos. PCT/US2012/050021 and PCT/US2011/038967, U.S. Patent Publication Nos. 2008/0271205 and 2008/0064063, and Genbanik Accession No. gi 189098312 (SEQ ID NO: 11) and GenBanik Accession ABD60225; GI:89242710 (SEQ ID NO: 12), which are incorporated herein by reference in their entirety. The steviol synthetase from Arabidopsis thaliana is classified as a CYP714A2.
In addition, a KAH polypeptide from Stevia rebaudiana that was identified as described in PCT Application No. PCT/US2012/050021 is particularly useful in a recombinant host. Nucleotide sequences encoding S. rebaudiana KAH (SrKAHe1; SEQ ID NO: 18) and S. rebaudiana KAH that has been codon-optimized for expression in yeast are set forth in the same PCT application, as is the encoded amino acid sequence of the S. rebaudiana KAH (SEQ ID NO: 19). The S. rebaudiana KAH shows significantly higher steviol synthase activity as compared to the Arabidopsis thaliana ent-kaurenoic acid hydroxylase described by Yamaguchi et al. (U.S. Patent Publication No. 2008/0271205 A1) when expressed in S. cerevisiae. The S. rebaudiana KAH polypeptide has less than 20% identity to the KAH from U.S. Patent Publication No. 2008/0271205, and less than 35% identity to the KAH from U.S. Patent Publication No. 2008/0064063.
In some embodiments, a recombinant microorganism contains a recombinant gene encoding a KO and/or a KAH polypeptide. Such microorganisms also typically contain a recombinant gene encoding a cytochrome P450 reductase (CPR) polypeptide, since certain combinations of KO and/or KAH polypeptides require expression of an exogenous CPR polypeptide. In particular, the activity of a KO and/or a KAH polypeptide of transporter origin can be significantly increased by the inclusion of a recombinant gene encoding an exogenous CPR polypeptide. Suitable CPR polypeptides are known. For example, suitable CPR enzymes include those made by Stevia rebaudiana and Arabidopsis thaliana. See, e.g., Table 5 and PCT Application Nos. PCT/US2012/050021 and PCT/US2011/038967, which are incorporated herein by reference in their entirety.
For example, the steviol synthase encoded by Stevia rebaudiana KAHe1 is activated by the S. cerevisiae CPR encoded by gene NCP1 (YHR042W). Even better activation of the steviol synthase encoded by SrKAHe1 is observed when the Arabidopsis thaliana CPR encoded by the gene ATR2 (SEQ ID NO: 99) or the S. rebaudiana CPR encoded by the genes CPR7 (SEQ ID NO: 23) or CPR8 (SEQ ID NO: 24) are co-expressed. Amino acid sequence of the A. thaliana polypeptides ATR1 (SEQ ID NO: 25) and ATR2 (SEQ ID NO: 26) and S. rebaudiana CPR7 (SEQ ID NO: 27) and CPR8 (SEQ ID NO: 28) polypeptides are shown in PCT Application No. PCT/US2012/050021.
Expression in a recombinant microorganism of these genes results in the conversion of geranylgeranyl diphosphate to steviol.
B. Steviol Glycoside Biosynthesis PolypeptidesIn addition to the transport mutations described above, a host cell as described herein can convert steviol to a steviol glycoside. Such a host (e.g., microorganism) contains genes encoding one or more UDP Glycosyl Transferases, also known as UGTs. UGTs transfer a monosaccharide unit from an activated nucleotide sugar to an acceptor moiety, in this case, an —OH or —COOH moiety on steviol, the glucose moiety on a steviol glycoside, or steviol derivatives. UGTs have been classified into families and subfamilies based on sequence homology. Li et al. J. Biol. Chem. 276:4338-4343 (2001).
B.1 Rubusoside Biosynthesis PolypeptidesThe biosynthesis of rubusoside involves glycosylation of the 13-OH and the 19-COOH of steviol. See
A suitable UGT85C2 functions as a uridine 5′-diphospho glucosyl:steviol 13-OH transferase, and a uridine 5′-diphospho glucosyl:steviol-19-O-glucoside 13-OH transferase. Functional UGT85C2 polypeptides also may catalyze glucosyl transferase reactions that utilize steviol glycoside substrates other than steviol and steviol-19-O-glucoside.
A suitable UGT74G1 polypeptide functions as a uridine 5′-diphospho glucosyl: steviol 19-COOH transferase and a uridine 5′-diphospho glucosyl: steviol-13-O-glucoside 19-COOH transferase. Functional UGT74G1 polypeptides also may catalyze glycosyl transferase reactions that utilize steviol glycoside substrates other than steviol and steviol-13-O-glucoside, or that transfer sugar moieties from donors other than uridine diphosphate glucose.
A recombinant microorganism expressing a functional UGT74G1 and a functional UGT85C2 can make rubusoside and both steviol monosides (i.e., steviol 13-O-monoglucoside and steviol 19-O-monoglucoside) when steviol is used as a feedstock in the medium. One or more of such genes may be present naturally in the host. Typically, however, such genes are recombinant genes that have been transformed into a host (e.g., microorganism) that does not naturally possess them.
As used herein, the term recombinant host is intended to refer to a host, the genome of which has been augmented by at least one incorporated DNA sequence. Such DNA sequences include but are not limited to genes that are not naturally present, DNA sequences that are not normally transcribed into RNA or translated into a protein (“expressed”), and other genes or DNA sequences which one desires to introduce into the non-recombinant host. It will be appreciated that typically the genome of a recombinant host described herein is augmented through the stable introduction of one or more recombinant genes. Generally, the introduced DNA is not originally resident in the host that is the recipient of the DNA, but it is within the scope of the invention to isolate a DNA segment from a given host, and to subsequently introduce one or more additional copies of that DNA into the same host, e.g., to enhance production of the product of a gene or alter the expression pattern of a gene. In some instances, the introduced DNA will modify or even replace an endogenous gene or DNA sequence by, e.g., homologous recombination or site-directed mutagenesis. Suitable recombinant hosts include microorganisms.
The term “recombinant gene” refers to a gene or DNA sequence that is introduced into a recipient host, regardless of whether the same or a similar gene or DNA sequence may already be present in such a host. “Introduced,” or “augmented” in this context, is known in the art to mean introduced or augmented by the hand of man. Thus, a recombinant gene may be a DNA sequence from another species, or may be a DNA sequence that originated from or is present in the same species, but has been incorporated into a host by recombinant methods to form a recombinant host. It will be appreciated that a recombinant gene that is introduced into a host can be identical to a DNA sequence that is normally present in the host being transformed, and is introduced to provide one or more additional copies of the DNA to thereby permit overexpression or modified expression of the gene product of that DNA.
Suitable UGT74G1 and UGT85C2 polypeptides include those made by Stevia rebaudiana. Genes encoding functional UGT74G1 and UGT85C2 polypeptides from Stevia are reported in Richman et al. Plant J. 41: 56-67 (2005). Amino acid sequences of S. rebaudiana UGT74G1 (SEQ ID NO: 29) and UGT85C2 (SEQ ID NO: 30) polypeptides are set forth in as sequence identifiers numbers 1 and 3, respectively, of PCT Application No. PCT/US2012/050021). Nucleotide sequences that encode UGT74G1(SEQ ID NO: 100) and UGT85C2, (SEQ ID NO: 31) as well as UGT sequences that have been optimized for expression in yeast, for example UGTs 85C2 (SEQ ID NO: 32), 91D2e, 91D2e-b, EUGT11 and 76G1, are provided. See also the UGT85C2 and UGT74G1 variants described below in the “Functional Homolog” section. For example, a UGT85C2 polypeptide can contain substitutions at positions 65, 71, 270, 289, and 389 can be used (e.g., A65S, E71Q, T270M, Q289H, and A389V).
In some embodiments, the recombinant host is a microorganism. The recombinant microorganism can be grown on media containing steviol in order to produce rubusoside. In other embodiments, however, the recombinant microorganism expresses one or more recombinant genes involved in steviol biosynthesis, e.g., a CDPS gene, a KS gene, a KO gene and/or a KAH gene. Suitable CDPS polypeptides are known.
For example, suitable CDPS enzymes include those made by Stevia rebaudiana, Streptomyces clavuligerus, Bradyrhizobium japonicum, Zea mays, and Arabidopsis. See, e.g., Table 6 and PCT Application Nos. PCT/US2012/050021 and PCT/US2011/038967, which are incorporated herein by reference in their entirety.
In some embodiments, CDPS polypeptides that lack a chloroplast transit peptide at the amino terminus of the unmodified polypeptide can be used. For example, the first 150 nucleotides from the 5′ end of the Zea mays CDPS coding sequence shown in FIG. 14 of PCT Publication No. PCT/US2012/050021 can be removed. Doing so removes the amino terminal 50 residues of the amino acid sequence, which encode a chloroplast transit peptide. The truncated CDPS gene can be fitted with a new ATG translation start site and operably linked to a promoter, typically a constitutive or highly expressing promoter. When a plurality of copies of the truncated coding sequence are introduced into a microorganism, expression of the CDPS polypeptide from the promoter results in an increased carbon flux towards ent-kaurene biosynthesis.
CDPS-KS bifunctional proteins also can be used. Nucleotide sequences encoding the CDPS-KS bifunctional enzymes shown in Table 7 were modified for expression in yeast (see PCT Application Nos. PCT/US2012/050021). A bifunctional enzyme from Gibberella fujikuroi also can be used.
Thus, a microorganism containing a CDPS gene, a KS gene, a KG gene and a KAH gene in addition to a UGT74G1 and a UGT85C2 gene is capable of producing both steviol monosides and rubusoside without the necessity for using steviol as a feedstock.
In some embodiments, the recombinant microorganism further expresses a recombinant gene encoding a geranylgeranyl diphosphate synthase (GGPPS). Suitable GGPPS polypeptides are known. For example, suitable GGPPS enzymes include those made by Stevia rebaudiana, Gibberella fujikuroi, Mus musculus, Thalassiosira pseudonana, Streptomyces clavuligerus, Sulfulobus acidocaldarius, Synechococcus sp. and Arabidopsis thaliana. See, Table 8 and PCT Application Nos. PCT/US2012/050021 and PCT/US2011/038967, which are incorporated herein by reference in their entirety.
In some embodiments, the recombinant microorganism further can express recombinant genes involved in diterpene biosynthesis or production of terpenoid precursors, e.g., genes in the methylerythritol 4-phosphate (MEP) pathway or genes in the mevalonate (MEV) pathway discussed below, have reduced phosphatase activity, and/or express a sucrose synthase (SUS) as discussed herein. In other embodiments, endogenous genes (e.g. DPP1) may be inactivated or deleted in order to affect availability of some GGPP/FPP precursors.
B.2 Rebaudioside a, Rebaudioside B, Rebaudioside D, Rebaudioside E, and Rebaudioside M Biosynthesis PolypeptidesBiosynthesis of rebaudioside A involves glucosylation of the aglycone steviol. Specifically, rebaudioside A can be formed by glucosylation of the 13-OH of steviol which forms the 13-O-steviolmonoside, glucosylation of the C-2′ of the 13-O-glucose of steviolmonoside which forms steviol-1,2-bioside, glucosylation of the C-19 carboxyl of steviol-1,2-bioside which forms stevioside, and glucosylation of the C-3′ of the C-13-O-glucose of stevioside. The order in which each glucosylation reaction occurs can vary. See
Biosynthesis of rebaudioside B involves glucosylation of the aglycone steviol. Specifically, rebaudioside B can be formed by glucosylation of the 13-OH of steviol which forms the 13-O-steviolmonoside, glucosylation of the C-2′ of the 13-O-glucose of steviolmonoside which forms steviol-1,2-bioside, and glucosylation of the C-3′ of the C-13-O-glucose of steviol-1,2-bioside. The order in which each glucosylation reaction occurs can vary.
Biosynthesis of rebaudioside E and/or rebaudioside D involves glucosylation of the aglycone steviol. Specifically, rebaudioside E can be formed by glucosylation of the 13-OH of steviol which forms steviol-13-O-glucoside, glucosylation of the C-2′ of the 13-O-glucose of steviol-13-O-glucoside which forms the steviol-1,2-bioside, glucosylation of the C-19 carboxyl of the 1,2-bioside to form 1,2-stevioside, and glucosylation of the C-2′ of the 19-O-glucose of the 1,2-stevioside to form rebaudioside E. Rebaudioside D can be formed by glucosylation of the C-3′ of the C-13-O-glucose of rebaudioside E. The order in which each glycosylation reaction occurs can vary. For example, the glucosylation of the C-2′ of the 19-O-glucose may be the last step in the pathway, wherein Rebaudioside A is an intermediate in the pathway. See
It has been discovered that conversion of steviol to rebaudioside A, rebaudioside B rebaudioside D, rebaudioside M, and/or rebaudioside E in a recombinant host can be accomplished by expressing the following functional UGTs: EUGT11, 91D2, 74G1, 85C2, and 76G1. Thus, a recombinant microorganism expressing combinations of these UGTs can make rebaudioside A and rebaudioside D when steviol is used as a feedstock. Typically, one or more of these genes are recombinant genes that have been transformed into a microorganism that does not naturally possess them. It has also been discovered that UGTs designated herein as SM12UGT can be substituted for UGT91D2.
In some embodiments, less than five (e.g., one, two, three, or four) UGTs are expressed in a host. For example, a recombinant microorganism expressing a functional EUGT11 can make rebaudioside D when rebaudioside A is used as a feedstock. A recombinant microorganism expressing, UGTs 85C, 91D2e or EUGT11, but preferably 91D2e, and 76G1 can make rebaudioside B. A recombinant microorganism expressing EUGT11, 76G1, and 91D12 (e.g., 91D2e), can make rebaudioside D when rubusoside or 1,2-stevioside is used as a feedstock. As another alternative, a recombinant microorganism expressing three functional UGTs, EUGT11, 74G1, 76G1, and optionally 91D2, can make rebaudioside D when fed the monoside, steviol-13-O-glucoside, in the medium. Similarly, conversion of steviol-19-O-glucoside to rebaudioside D in a recombinant microorganism can be accomplished by the expression of genes encoding UGTs EUGT11, 85C2, 76G1, and 91D2 (e.g., 91D2e) when fed steviol-19-O-glucoside. Typically, one or more of these genes are recombinant genes that have been transformed into a host that does not naturally possess them.
Rebaudioside M PolypeptidesConversion of steviol to Rebaudioside M in a recombinant host can be accomplished by expressing combinations of the following functional UGTs: 91D2, EUGT11, 74G1, 85C2, and 76G1. See
Targeted production of individual Rebaudiosides, as shown in
A suitable EUGT11 or UGT91D2 polypeptide functions as a uridine 5′-diphospho glucosyl: steviol-13-O-glucoside transferase (also referred to as a steviol-13-monoglucoside 1,2-glucosylase), transferring a glucose moiety to the C-2′ of the 13-O-glucose of the acceptor molecule, steviol-13-O-glucoside.
A suitable EUGT11 or UGT91D2 polypeptide also functions as a uridine 5′-diphospho glucosyl: rubusoside transferase transferring a glucose moiety to the C-2′ of the 13-O-glucose of the acceptor molecule, rubusoside, to produce stevioside. EUGT11 polypeptides also can efficiently transfer a glucose moiety to the C-2′ of the 19-O-glucose of the acceptor molecule, rubusoside, to produce a 19-O-1,2-diglycosylated rubusoside. EUGT11 is particularly efficient at transfer of glucose molecules to 19-O-glucose substituted steviol glycoside molecules.
Functional EUGT11 or UGT91D2 polypeptides also can catalyze reactions that utilize steviol glycoside substrates other than steviol-13-O-glucoside and rubusoside. For example, a functional EUGT11 polypeptide may efficiently utilize stevioside as a substrate, transferring a glucose moiety to the C-2′ of the 19-O-glucose residue to produce Rebaudioside E. Functional EUGT11 and UGT91D2 polypeptides may also utilize Rebaudioside A as a substrate, transferring a glucose moiety to the C-2′ of the 19-O-glucose residue of Rebaudioside A to produce Rebaudioside D. EUGT11 (SEQ ID NO: 51) can convert Rebaudioside A to Rebaudioside D at a rate that is least 20 times faster (e.g., as least 25 times or at least 30 times faster) than the corresponding rate of UGT91D2e (SEQ ID NO: 54) when the reactions are performed under similar conditions, i.e., similar time, temperature, purity, and substrate concentration. As such, EUGT11 produces greater amounts of RebD than UGT91D2e when incubated under similar conditions.
In addition, a functional EUGT11 exhibits significant C-2′ 19-O-diglycosylation activity with rubusoside or stevioside as substrates, whereas UGT91D2e has less diglycosylation activity with these substrates. Thus, a functional EUGT11 can be distinguished from UGT91D2e by the differences in steviol glycoside substrate-specificity.
A functional EUGT11 or UGT91D2 polypeptide typically does not transfer a glucose moiety to steviol compounds having a 1,3-bound glucose at the C-13 position, i.e., transfer of a glucose moiety to steviol 1,3-bioside and 1,3-stevioside does not occur at detectable levels under most conditions.
Suitable EUGT11 polypeptides can include the EUGT11 polypeptide from Oryza sativa (GenBank Accession No. AC133334; SEQ ID NO: 51). For example, an EUGT11 polypeptide can have an amino acid sequence with at least 70% sequence identity (e.g., at least 75, 80, 85, 90, 95, 96, 97, 98, or 99% sequence identity) to the amino acid sequence set forth in SEQ ID NO: 51. The nucleotide sequence encoding the amino acid sequence of EUGT11 also is set forth in SEQ ID NO: 52 as is a codon optimized nucleotide sequence for expression in yeast SEQ ID NO: 53.
Suitable functional UGT91D2 polypeptides include the polypeptides designated UGT91D2e and UGT91D2m. The amino acid sequence of an exemplary UGT91D2e polypeptide from Stevia rebaudiana is set forth in SEQ ID NO: 54 (encoded by nucleotide sequence identifier number 5 of PCT Application No. PCT/US2012/050021), which also discloses the S. rebaudiana nucleotide sequence encoding the polypeptide, a nucleotide sequence that encodes the polypeptide and that has been codon optimized (SEQ ID NO: 158) for expression in yeast, the amino acid sequences of exemplary UGT91D2m polypeptides from S. rebaudiana, and nucleic acid sequences encoding the exemplary UGT91D2m polypeptides. The amino acid sequence of exemplary UGT91D2m is shown as SEQ ID NO: 55. UGT91D2 variants containing a substitution at amino acid residues 206, 207, and 343 also can be used. For example, the amino acid sequence having G206R, Y207C, and W343R mutations with respect to wild-type UGT92D2e can be used. In addition, a UGT91D2 variant containing substitutions at amino acid residues 211 and 286 can be used. For example, a UGT91D2 variant can include a substitution of a methionine for leucine at position 211 and a substitution of an alanine for valine at position 286. See also the UGT91D2 variants descried in the “functional homolog” section.
As indicated above, UGTs designated herein as SM12UGT can be substituted for UGT91D2. Suitable functional SM12UGT polypeptides include those made by Ipomoea purpurea (Japanese morning glory) and described in Morita et al. Plant J. 42: 353-363 (2005). The amino acid sequence encoding the I. purpurea IP3GGT polypeptide (SEQ ID NO: 56) is set forth using sequence identifier number 76 in PCT Application No. PCT/US2012/050021, as is a nucleotide sequence (SEQ ID NO: 57) that encodes the polypeptide and that has been codon optimized for expression in yeast. Another suitable SM12UGT polypeptide is a Bp94B1 polypeptide having an R25S mutation. See Osmani et al. Plant Phys. 148: 1295-1308 (2008) and Sawada et al. J. Biol. Chem. 280: 899-906 (2005). The amino acid sequence of the Bellis perennis (red daisy) UGT94B1 polypeptide (SEQ ID NO: 58) is set forth using sequence identifier number 78 in PCT Application No. PCT/US2012/050021, as is a nucleotide sequence (SEQ ID NO: 59) that encodes the polypeptide and that has been codon optimized for expression in yeast.
In some embodiments, the recombinant microorganism is grown on media containing steviol-13-O-glucoside or steviol-19-O-glucoside in order to produce rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E and/or rebaudioside M. In such embodiments, the microorganism contains and expresses genes encoding a functional EUGT11, a functional UGT74G1, a functional UGT85C2, a functional UGT76G1, and a functional UGT91D2, and is capable of accumulating rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E and/or rebaudioside M when steviol, one or both of the steviolmonosides, or rubusoside is used as feedstock.
In other embodiments, the recombinant microorganism is grown on media containing rubusoside in order to produce rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E and/or rebaudioside M. In such embodiments, the microorganism contains and expresses genes encoding a functional EUGT11, a functional UGT76G1, and a functional UGT91D2, and is capable of producing rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E and/or rebaudioside M when rubusoside is used as feedstock.
In other embodiments the recombinant microorganism expresses one or more genes involved in steviol biosynthesis, e.g., a CDPS gene, a KS gene, a KO gene and/or a KAH gene. Thus, for example, a microorganism containing a CDPS gene, a KS gene, a KO gene and a KAH gene, in addition to a EUGT11, a UGT74G1, a UGT85C2, a UGT76G1, and optionally a functional UGT91D2 (e.g., UGT91D2e), is capable of producing rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E and/or rebaudioside M without the necessity for including steviol in the culture media. In another example, a microorganism containing a CDPS gene, a KS gene, a KO gene and a KAH gene, in addition to a UGT74G1, a UGT85C2, a UGT76G1, and optionally a functional UGT91D2 (e.g., UGT91D2e), is capable of producing rebaudioside A without the necessity for including steviol in the culture media. In yet another example, a microorganism containing a CDPS gene, a KS gene, a KO gene and a KAH gene, in addition to a UGT85C2, a UGT76G1, and optionally a functional UGT91D2 (e.g., UGT91D2e), is capable of producing rebaudioside B without the necessity for including steviol in the culture media.
In some embodiments, the recombinant host further contains and expresses a recombinant GGPPS gene in order to provide increased levels of the diterpene precursor geranylgeranyl diphosphate, for increased flux through the steviol biosynthetic pathway.
In some embodiments, the recombinant host further contains a construct to silence the expression of non-steviol pathways consuming geranylgeranyl diphosphate, ent-Kaurenoic acid or farnesyl pyrophosphate, thereby providing increased flux through the steviol and steviol glycosides biosynthetic pathways. For example, flux to sterol production pathways such as ergosterol may be reduced by downregulation of the ERG9 gene. See section C.4 below. In cells that produce gibberellins, gibberellin synthesis may be downregulated to increase flux of ent-kaurenoic acid to steviol. In carotenoid-producing organisms, flux to steviol may be increased by downregulation of one or more carotenoid biosynthetic genes. In some embodiments, the recombinant microorganism further can express recombinant genes involved in diterpene biosynthesis or production of terpenoid precursors, e.g., genes in the MEP or MEV) pathways, have reduced phosphatase activity, and/or express a SUS.
One with skill in the art will recognize that by modulating relative expression levels of different UGT genes, a recombinant host can be tailored to specifically produce steviol glycoside products in a desired proportion. Transcriptional regulation of steviol biosynthesis genes and steviol glycoside biosynthesis genes can be achieved by a combination of transcriptional activation and repression using techniques known to those in the art. For in vitro reactions, one with skill in the art will recognize that addition of different levels of UGT enzymes in combination or under conditions which impact the relative activities of the different UGTS in combination will direct synthesis towards a desired proportion of each steviol glycoside. One with skill in the art will recognize that a higher proportion of rebaudioside D or E or more efficient conversion to rebaudioside D or E can be obtained with a diglycosylation enzyme that has a higher activity for the 19-O-glucoside reaction as compared to the 13-O-glucoside reaction (substrates rebaudioside A and stevioside).
In some embodiments, a recombinant host such as a microorganism produces rebaudioside D-enriched steviol glycoside compositions that have greater than at least 3% rebaudioside D by weight total steviol glycosides, e.g., at least 4% rebaudioside D at least 5% rebaudioside D, 10-20% rebaudioside D, 20-30% rebaudioside D, 30-40% rebaudioside D, 40-50% rebaudioside D, 50-60% rebaudioside D, 60-70% rebaudioside D, 70-80% rebaudioside D.
In some embodiments, a recombinant host such as a microorganism produces steviol glycoside compositions that have at least 90% rebaudioside D, e.g., 90-99% rebaudioside D. Other steviol glycosides present may include steviol monosides, steviol glucobiosides, rebaudioside A, rebaudioside E, and stevioside. In some embodiments, the rebaudioside D-enriched composition produced by the host (e.g., microorganism) can be further purified and the rebaudioside D or rebaudioside E so purified can then be mixed with other steviol glycosides, flavors, or sweeteners to obtain a desired flavor system or sweetening composition. For instance, a rebaudioside D-enriched composition produced by a recombinant host can be combined with a rebaudioside A or F-enriched composition produced by a different recombinant host, with rebaudioside A or F purified from a Stevia extract, or with rebaudioside A or F produced in vitro.
In some embodiments, rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E and/or rebaudioside M can be produced using whole recombinant cells that are fed raw materials that contain precursor molecules such as steviol and/or steviol glycosides, including mixtures of steviol glycosides derived from plant extracts, wherein said recombinant cells express all or the appropriate combination of UGT polypeptides to effect glucosylation of said steviol to each of the particular glucosylated rebaudiosides. In some embodiments, the recombinant cells can optionally express a transporter, such that they efficiently excrete the rebaudioside without need for permeabilization agents to be added. The raw materials may be fed during cell growth or after cell growth. The whole cells may be in suspension or immobilized. The whole cells may be entrapped in beads, for example calcium or sodium alginate beads. The whole cells may be linked to a hollow fiber tube reactor system. The whole cells may be concentrated and entrapped within a membrane reactor system. The whole cells may be in fermentation broth or in a reaction buffer. In some embodiments, a permeabilizing agent is utilized for efficient transfer of substrate into the cells. In some embodiments, the cells are permeabilized with a solvent such as toluene, or with a detergent such as Triton-X or Tween. In some embodiments, the cells are permeabilized with a surfactant, for example a cationic surfactant such as cetyltrimethylammonium bromide (CTAB). In some embodiments, the cells are permeabilized with periodic mechanical shock such as electroporation or a slight osmotic shock. The cells can contain one recombinant UGT or multiple recombinant UGTs. For example, the cells can contain UGT 76G1 and EUGT11 such that mixtures of stevioside and RebA are efficiently converted to RebD. In some embodiments, the whole cells are the host cells described in section III A. In some embodiments, the whole cells are a Gram-negative bacterium such as E. coli. In some embodiments, the whole cell is a Gram-positive bacterium such as Bacillus. In some embodiments, the whole cell is a fungal species such as Aspergillus, or a yeast such as Saccharomyces. In some embodiments, the term “whole cell biocatalysis” is used to refer to the process in which the whole cells are grown as described above (e.g., in a medium and optionally permeabilized) and a substrate such as rebA or stevioside is provided and converted to the end product using the enzymes from the cells. The cells may or may not be viable, and may or may not be growing during the bioconversion reactions. In contrast, in fermentation, the cells are cultured in a growth medium and fed a carbon and energy source such as glucose and the end product is produced with viable cells.
C. Other PolypeptidesGenes for additional polypeptides whose expression facilitates more efficient or larger scale production of steviol or a steviol glycoside can also be introduced into a recombinant host. For example, a recombinant microorganism can also contain one or more genes encoding a geranylgeranyl diphosphate synthase (GGPPS, also referred to as GGDPS). As another example, the recombinant host can contain one or more genes encoding a rhamnose synthetase, or one or more genes encoding a UDP-glucose dehydrogenase and/or a UDP-glucuronic acid decarboxylase. As another example, a recombinant host can also contain one or more genes encoding a cytochrome P450 reductase (CPR). Expression of a recombinant CPR facilitates the cycling of NADP+ to regenerate NADPH, which is utilized as a cofactor for terpenoid biosynthesis. Other methods can be used to regenerate NADHP levels as well. In circumstances where NADPH becomes limiting; strains can be further modified to include exogenous transhydrogenase genes. See, e.g., Sauer et al. J. Biol. Chem. 279: 6613-6619 (2004). Other methods are known to those with skill in the art to reduce or otherwise modify the ratio of NADH/NADPH such that the desired cofactor level is increased.
As another example, the recombinant host can contain one or more genes encoding one or more enzymes in the MEP pathway or the mevalonate pathway. Such genes are useful because they can increase the flux of carbon into the diterpene biosynthesis pathway, producing geranylgeranyl diphosphate from isopentenyl diphosphate and dimethylallyl diphosphate generated by the pathway. The geranylgeranyl diphosphate so produced can be directed towards steviol and steviol glycoside biosynthesis due to expression of steviol biosynthesis polypeptides and steviol glycoside biosynthesis polypeptides.
As another example the recombinant host can contain one or more genes encoding a sucrose synthase, and additionally can contain sucrose uptake genes if desired. The sucrose synthase reaction can be used to increase the UDP-glucose pool in a fermentation host, or in a whole cell bioconversion process. This regenerates UDP-glucose from UDP produced during glycosylation and sucrose, allowing for efficient glycosylation. In some organisms, disruption of the endogenous invertase is advantageous to prevent degradation of sucrose. For example, the S. cerevisiae SUC2 invertase may be disrupted. The sucrose synthase (SUS) can be from any suitable organism. For example, a sucrose synthase coding sequence from, without limitation, Arabidopsis thaliana, Stevia rebaudiana, or Coffea arabica can be cloned into an expression plasmid under control of a suitable promoter, and expressed in a microorganism. The sucrose synthase can be expressed in such a strain in combination with a sucrose transporter (e.g., the A. thaliana SUC1 transporter or a functional homolog thereof) and one or more UGTs (e.g., one or more of UGT85C2, UGT74G1, UGT76G1, and UGT91D2e, EUGT11 or functional homologs thereof). Culturing the host in a medium that contains sucrose can promote production of UDP-glucose, as well as one or more glucosides (e.g., steviol glycosides).
Expression of the ERG9 gene, which encodes squalene synthase (SQS), also can be reduced in recombinant hosts such that there is a build-up of precursors to squalene synthase in the recombinant host. SQS is classified under EC 2.5.1.21 and is the first committed enzyme of the biosynthesis pathway that leads to the production of sterols. It catalyzes the synthesis of squalene from farnesyl pyrophosphate via the intermediate presqualene pyrophosphate. This enzyme is a critical branch point enzyme in the biosynthesis of terpenoids/isoprenoids and is thought to regulate the flux of isoprene intermediates through the sterol pathway. The enzyme is sometimes referred to as farnesyl-diphosphate famesyltransferase (FDFT1). The mechanism of SQS is to convert two units of farnesyl pyrophosphate into squalene. SQS is considered to be an enzyme of eukaryotes or advanced organisms, although at least one prokaryote has been shown to possess a functionally similar enzyme.
Genes for polypeptides whose inactivation facilitates more efficient or larger scale production of steviol or a steviol glycoside can be modified in a recombinant host. For example, an endogenous gene encoding a phosphatase such as the yeast diacylglycerol pyrophosphate phosphatase encoded by the DPP1 gene and/or the yeast lipid phosphate phosphatase encoded by the LPP1 gene can be inactivated such that the degradation of farnesyl pyrophosphate (FPP) to farnesol is reduced and the degradation of geranylgeranylpyrophosphate (GGPP)) to geranylgeraniol (GGOH) is reduced. Such genes can be inactivated or have expression reduced by known techniques such as homologous recombination, mutagenesis, or transcription activator-like effector nucleases (TALENs).
C.1 MEP Biosynthesis PolypeptidesIn some embodiments, a recombinant host contains one or more genes encoding enzymes involved in the methylerythritol 4-phosphate (MEP) pathway for isoprenoid biosynthesis. Enzymes in the MEP pathway include deoxyxylulose 5-phosphate synthase (DXS), D-1-deoxyxylulose 5-phosphate reductoisomerase (DXR), 4-diphosphocytidyl-2-C-methyl-D-erythritol synthase (CMS), 4-diphosphocytidyl-2-C-methyl-D-erythritol kinase (CMK), 4-diphosphocytidyl-2-C-methyl-D-erythritol 2,4-cyclodiphosphate synthase (MCS), 1-hydroxy-2-methyl-2(E)-butenyl 4-diphosphate synthase (HDS) and 1-hydroxy-2-methyl-2(E)-butenyl 4-diphosphate reductase (HDR). One or more DXS genes, DXR genes, CMS genes, CMK genes, MCS genes, HDS genes and/or HDR genes can be incorporated into a recombinant microorganism. See, Rodríguez-Concepción and Boronat, Plant Phys. 130: 1079-1089 (2002).
Suitable genes encoding DXS, DXR, CMS, CMK, MCS, HDS and/or HDR polypeptides include those made by E. coli, Arabidopsis thaliana and Synechococcus leopoliensis. Nucleotide sequences encoding DXR polypeptides are described, for example, in U.S. Pat. No. 7,335,815.
C.2 Mevalonate Biosynthesis PolypeptidesIn some embodiments, a recombinant host contains one or more genes encoding enzymes involved in the mevalonate pathway for isoprenoid biosynthesis. Genes suitable for transformation into a host encode enzymes in the mevalonate pathway such as a truncated 3-hydroxy-3-methyl-glutaryl (HMG)-CoA reductase (tHMG), and/or a gene encoding a mevalonate kinase (MK), and/or a gene encoding a phosphomevalonate kinase (PMK), and/or a gene encoding a mevalonate pyrophosphate decarboxylase (MPPD). Thus, one or more HMG-CoA reductase genes, MK genes, PMK genes, and/or MPPD genes can be incorporated into a recombinant host such as a microorganism.
Suitable genes encoding mevalonate pathway polypeptides are known. For example, suitable polypeptides include those made by E. coli, Paracoccus denitrificans, Sacchaiomyces cerevisiae, Arabidopsis thaliana, Kitasatospora griseola, Homo sapiens, Drosophila melanogaster, Gallus gallus, Streptomyces sp. KO-3988, Nicotiana attenuata, Kitasatospora griseola, Hevea brasiliensis, Enterococcus faecium and Haematococcus pluvialis. See, e.g., Table 9, U.S. Pat. Nos. 7,183,089, 5,460,949, and 5,306,862, and PCT Application Nos. PCT/US2012/050021 and PCT/US2011/038967, which are incorporated herein by reference in their entirety.
Sucrose synthase (SUS) can be used as a tool for generating UDP-sugar. SUS (EC 2.4.1.13) catalyzes the formation of UDP-glucose and fructose from sucrose and UDP. UDP generated by the reaction of UGTs thus can be converted into UDP-glucose in the presence of sucrose. See, e.g., Chen et al. (2001) J. Am. Chem. Soc. 123:8866-8867; Shao et al. (2003) Appl. Env. Microbiol. 69:5238-5242; Masada et al. (2007) FEBS Lett. 581:2562-2566; and Son et al. (2009) J. Microbiol. Biotechnol. 19:709-712.
Sucrose synthases can be used to generate UDP-glucose and remove UDP, facilitating efficient glycosylation of compounds in various systems. For example, yeast deficient in the ability to utilize sucrose can be made to grow on sucrose by introducing a sucrose transporter and a SUS. For example, Saccharomyces cerevisiae does not have an efficient sucrose uptake system, and relies on extracellular SUC2 to utilize sucrose. The combination of disrupting the endogenous S. cerevisiae SUC2 invertase and expressing recombinant SUS resulted in a yeast strain that was able to metabolize intracellular but not extracellular sucrose (Riesmeier et al. ((1992) EMBO J. 11:4705-4713). The strain was used to isolate sucrose transporters by transformation with a cDNA expression library and selection of transformants that had gained the ability to take up sucrose.
The combined expression of recombinant sucrose synthase and a sucrose transporter in vivo can lead to increased UDP-glucose availability and removal of unwanted UDP. For example, functional expression of a recombinant sucrose synthase, a sucrose transporter, and a glycosyltransferase, in combination with knockout of the natural sucrose degradation system (SUC2 in the case of S. cerevisiae) can be used to generate a cell that is capable of producing increased amounts of glycosylated compounds such as steviol glycosides. This higher glycosylation capability is due to at least (a) a higher capacity for producing UDP-glucose in a more energy efficient manner, and (b) removal of UDP from growth medium, as UDP can inhibit glycosylation reactions.
The sucrose synthase can be from any suitable organism. For example, a sucrose synthase coding sequence from, without limitation, Arabidopsis thaliana (e.g. SEQ ID NO: 78 or 79), or Coffea arabica (e.g., SEQ ID NO: 80) (see, e.g., SEQ ID NOs:178, 179, and 180 of PCT/US2012/050021) can be cloned into an expression plasmid under control of a suitable promoter, and expressed in a host (e.g., a microorganism or a plant). A SUS coding sequence may be expressed in a SUC2 (sucrose hydrolyzing enzyme) deficient S. cerevisiae strain, so as to avoid degradation of extracellular sucrose by the yeast. The sucrose synthase can be expressed in such a strain in combination with a sucrose transporter (e.g., the A. thaliana SUC1 transporter or a functional homolog thereof) and one or more UGTs (e.g., one or more of UGT85C2, UGT74G1, UGT76G1, EUGT11, and UGT91D2e, or functional homologs thereof). Culturing the host in a medium that contains sucrose can promote production of UDP-glucose, as well as one or more glucosides (e.g., steviol glucoside). It is to be noted that in some cases, a sucrose synthase and a sucrose transporter can be expressed along with a UGT in a host cell that also is recombinant for production of a particular compound (e.g., steviol).
C.4 Squalene Synthase PolypeptidesExpression of an endogenous squalene synthase gene can be altered in a recombinant host described herein using a nucleic acid construct containing, for example, two regions that are homologous to parts of the genome sequence within the promoter of a gene encoding a squalene synthase or 5′ end of the open reading frame (ORF) encoding squalene synthase, respectively. In yeast, for example, such a construct can contain two regions that are homologous to parts of the genome sequence within the ERG9 promoter or 5′ end of the ERG9 open reading frame, respectively. The construct further can include a promoter, such as either the wild type ScKex2 or wild type ScCyc1 for yeast. The promoter further can include a heterologous insert such as a hairpin at its 3′-end. The polypeptide encoded by the ORF has at least 70% identity to a squalene synthase (EC 2.5.1.21) or a biologically active fragment thereof, said fragment having at least 70% sequence identity to said squalene synthase in a range of overlap of at least 100 amino acids. See, for example, PCT/US2012/050021.
The heterologous insert can adapt the secondary structure element of a hairpin with a hairpin loop. The heterologous insert sequence has the general formula (I):
-X1-X2-X3-X4-X5
X2 comprises at least 4 consecutive nucleotides being complementary to, and forming a hairpin secondary structure element with at least 4 consecutive nucleotides of X4, and X3 is optional and if present comprises nucleotides involved in forming a hairpin loop between X2 and X4, and
X1 and X5 individually and optionally comprise one or more nucleotides, and X2 and X4 may individually consist of any suitable number of nucleotides, so long as a consecutive sequence of at least 4 nucleotides of X2 is complementary to a consecutive sequence of at least 4 nucleotides of X4. In some embodiments, X2 and X4 consist of the same number of nucleotides.
The heterologous insert is long enough to allow a hairpin to be completed, but short enough to allow limited translation of an ORF that is present in-frame and immediately 3′ to the heterologous insert. Typically, the heterologous insert is from 10-50 nucleotides in length, e.g., 10-30 nucleotides, 15-25 nucleotides, 17-22 nucleotides, 18-21 nucleotides, 18-20 nucleotides, or 19 nucleotides in length.
X2 may for example consist of in the range of 4 to 25 nucleotides, such as in the range of 4 to 20, 4 to 15, 6 to 12, 8 to 12, or 9 to 11 nucleotides.
X4 may for example consist of in the range of 4 to 25 nucleotides, such as in the range of 4 to 20, 4 to 15, 6 to 12, 8 to 12, or 9 to 11 nucleotides.
In some embodiments, X2 consists of a nucleotide sequence that is complementary to the nucleotide sequence of X4, all nucleotides of X2 are complementary to the nucleotide sequence of X4.
X3 may be absent, i.e., X3 may consist of zero nucleotides. It is also possible that X3 consists of in the range of 1 to 5 nucleotides, such as in the range of 1 to 3 nucleotides.
X1 may be absent, i.e., X1 may consist of zero nucleotides. It is also possible that X1 consists of in the range of 1 to 25 nucleotides, such as in the range of 1 to 20, 1 to 15, 1 to 10, 1 to 5, or 1 to 3 nucleotides.
X5 may be absent, i.e., X5 may consist of zero nucleotides. It is also possible that X5 may consist of in the range 1 to 5 nucleotides, such as in the range of 1 to 3 nucleotides.
The heterologous insert can be any suitable sequence fulfilling the requirements defined herein. For example, the heterologous insert may comprise tgaattcgttaacgaattc (SEQ ID NO: 81), tgaattcgttaacgaactc (SEQ ID NO: 82), tgaattcgttaacgaagtc (SEQ ID NO: 83), or tgaattcgttaacgaaatt (SEQ ID NO: 84).
Without being bound to a particular mechanism, ERG9 expression in yeast can be decreased by at least partly, sterically hindering binding of the ribosome to the RNA thus reducing the translation of squalene synthase. Using a construct can decrease turnover of farnesyl-pyrophosphate to squalene and/or enhance accumulation of a compound selected from the group consisting of farnesyl-pyrophosphate, isopentenyl-pyrophosphate, dimethylallyl-pyrophosphate, geranyl-pyrophosphate and geranylgeranyl-pyrophosphate.
Occasionally it may be advantageous to include a squalene synthase inhibitor when culturing recombinant hosts described herein. Chemical inhibition of squalene synthase, e.g., by lapaquistat, is known in the art. Other squalene synthase inhibitors include Zaragozic acid and RPR 107393. Thus, in one embodiment the culturing step of the method(s) defined herein are performed in the presence of a squalene synthase inhibitor.
In some embodiments, the recombinant yeast hosts described herein contain a mutation in the ERG9 open reading frame.
In some embodiments, the recombinant yeast hosts described herein contain an ERG9[Δ]::HIS3 deletion/insertion allele.
D. Functional HomologsFunctional homologs of polypeptides described herein are also suitable for use in producing steviol or steviol glycosides in a recombinant host. A functional homolog is a polypeptide that has sequence similarity to a reference polypeptide, and that carries out one or more of the biochemical or physiological function(s) of the reference polypeptide. A functional homolog and the reference polypeptide may be natural occurring polypeptides, and the sequence similarity may be due to convergent or divergent evolutionary events. As such, functional homologs are sometimes designated in the literature as homologs, or orthologs, or paralogs. Variants of a naturally occurring functional homolog, such as polypeptides encoded by mutants of a wild type coding sequence, may themselves be functional homologs. Functional homologs can also be created via site-directed mutagenesis of the coding sequence for a polypeptide, or by combining domains from the coding sequences for different naturally-occurring polypeptides (“domain swapping”). Techniques for modifying genes encoding functional UGT polypeptides described herein are known and include, inter alia, directed evolution techniques, site-directed mutagenesis techniques and random mutagenesis techniques, and can be useful to increase specific activity of a polypeptide, alter substrate specificity, alter expression levels, alter subcellular location, or modify polypeptide:polypeptide interactions in a desired manner. Such modified polypeptides are considered functional homologs. The term “functional homolog” is sometimes applied to the nucleic acid that encodes a functionally homologous polypeptide.
Functional homologs can be identified by analysis of nucleotide and polypeptide sequence alignments. For example, performing a query on a database of nucleotide or polypeptide sequences can identify homologs of steviol or steviol glycoside biosynthesis polypeptides or transporter genes or proteins or transcription factor genes or proteins that regulate expression of at least one transporter gene. Sequence analysis can involve BLAST, Reciprocal BLAST, or PSI-BLAST analysis of no redundant databases using a GGPPS, a CDPS, a KS, a KO, a KAH or a transporter or transcription factor amino acid sequence as the reference sequence. Amino acid sequence is, in some instances, deduced from the nucleotide sequence. Those polypeptides in the database that have greater than 40% sequence identity are candidates for further evaluation for suitability as a functional homolog for a steviol or steviol glycoside biosynthesis polypeptide or as a functional homolog for a transporter protein or transcription factor that regulates expression of at least one transporter gene. Amino acid sequence similarity allows for conservative amino acid substitutions, such as substitution of one hydrophobic residue for another or substitution of one polar residue for another. If desired, manual inspection of such candidates can be carried out in order to narrow the number of candidates to be further evaluated. Manual inspection can be performed by selecting those candidates that appear to have domains present in steviol biosynthesis polypeptides or transporter protein or transcription factor that regulates expression of at least one transporter gene, e.g., conserved functional domains.
Conserved regions can be identified by locating a region within the primary amino acid sequence of a steviol or a steviol glycoside biosynthesis polypeptide or a transporter gene or transcription factor that regulates expression of at least one transporter gene that is a repeated sequence, forms some secondary structure (e.g., helices and beta sheets), establishes positively or negatively charged domains, or represents a protein motif or domain. See, e.g., the Pfam web site describing consensus sequences for a variety of protein motifs and domains on the World Wide Web at sanger.ac.uk/Software/Pfam/and pfam.janelia.org/. The information included at the Pfam database is described in Sonnhammer et al. Nucl. Acids Res. 26: 320-322 (1998); Sonnhammer et al. Proteins 28: 405-420 (1997); and Bateman et al. Nucl. Acids Res. 27: 260-262 (1999). Conserved regions also can be determined by aligning sequences of the same or related polypeptides from closely related species. Closely related species preferably are from the same family. In some embodiments, alignment of sequences from two different species is adequate.
Typically, polypeptides that exhibit at least about 40% amino acid sequence identity are useful to identify conserved regions. Conserved regions of related polypeptides exhibit at least 45% amino acid sequence identity (e.g., at least 50%, at least 60%, at least 70%, at least 80%, or at least 90% amino acid sequence identity). In some embodiments, a conserved region exhibits at least 92%, 94%, 96%, 98%, or 99% amino acid sequence identity.
For example, polypeptides suitable for producing steviol glycosides in a recombinant host include functional homologs of EUGT11, UGT91D2e, UGT91D2m, UGT85C, and UGT76G. Such homologs have greater than 90% (e.g., at least 95% or 99%) sequence identity to the amino acid sequence of EUGT11, UGT91D2e, UGT91D2m, UGT85C, or UGT76G as set forth in PCT Application No. PCT/US2012/050021. Variants of EUGT11, UGT91D2, UGT85C, and UGT76G polypeptides typically have 10 or fewer amino acid substitutions within the primary amino acid sequence, e.g., 7 or fewer amino acid substitutions, 5 or conservative amino acid substitutions, or between 1 and 5 substitutions. However, in some embodiments, variants of EUGT11, UGT91D2, UGT85C, and UGT76G polypeptides can have 10 or more amino acid substitutions (e.g., 10, 15, 20, 25, 30, 35, 10-20, 10-35, 20-30, or 25-35 amino acid substitutions). The substitutions may be conservative, or in some embodiments, non-conservative. Non-limiting examples of non-conservative changes in UGT91D2e polypeptides include glycine to arginine and tryptophan to arginine. Non-limiting examples of non-conservative substitutions in UGT76G polypeptides include valine to glutamic acid, glycine to glutamic acid, glutamine to alanine, and serine to proline. Non-limiting examples of changes to UGT85C polypeptides include histidine to aspartic acid, proline to serine, lysine to threonine, and threonine to arginine.
In some embodiments, a useful UGT91D2 homolog can have amino acid substitutions (e.g., conservative amino acid substitutions) in regions of the polypeptide that are outside of predicted loops, e.g., residues 20-26, 39-43, 88-95, 121-124, 142-158, 185-198, and 203-214 are predicted loops in the N-terminal domain and residues 381-386 are predicted loops in the C-terminal domain of UGT91D2e (see SEQ ID NO: 54). For example, a useful UGT91D2 homolog can include at least one amino acid substitution at residues 1-19, 27-38, 44-87, 96-120, 125-141, 159-184, 199-202, 215-380, or 387-473. In some embodiments, a UGT91D2 homolog can have an amino acid substitution at one or more residues selected from the group consisting of residues 30, 93, 99, 122, 140, 142, 148, 153, 156, 195, 196, 199, 206, 207, 211, 221, 286, 343, 427, and 438. For example, a UGT91D2 functional homolog can have an amino acid substitution at one or more of residues 206, 207, and 343, such as an arginine at residue 206, a cysteine at residue 207, and an arginine at residue 343. See, for example SEQ ID NO: 86. Other functional homologs of UGT91D2 can have one or more of the following: a tyrosine or phenylalanine at residue 30, a proline or glutamine at residue 93, a serine or valine at residue 99, a tyrosine or a phenylalanine at residue 122, a histidine or tyrosine at residue 140, a serine or cysteine at residue 142, an alanine or threonine at residue 148, a methionine at residue 152, an alanine at residue 153, an alanine or serine at residue 156, a glycine at residue 162, a leucine or methionine at residue 195, a glutamic acid at residue 196, a lysine or glutamic acid at residue 199, a leucine or methionine at residue 211, a leucine at residue 213, a serine or phenylalanine at residue 221, a valine or isoleucine at residue 253, a valine or alanine at residue 286, a lysine or asparagine at residue 427, an alanine at residue 438, and either an alanine or threonine at residue 462. In another embodiment, a UGT91D2 functional homolog contains a methionine at residue 211 and an alanine at residue 286.
In some embodiments, a useful UGT85C homolog can have one or more amino acid substitutions at residues 9, 10, 13, 15, 21, 27, 60, 65, 71, 87, 91, 220, 243, 270, 289, 298, 334, 336, 350, 368, 389, 394, 397, 418, 420, 440, 441, 444, and 471. Non-limiting examples of useful UGT85C homologs include polypeptides having substitutions (with respect to SEQ ID NO: 30) at residue 65 (e.g., a serine at residue 65), at residue 65 in combination with residue 15 (a leucine at residue 15), 270 (e.g., a methionine, arginine, or alanine at residue 270), 418 (e.g., a valine at residue 418), 440 (e.g., an aspartic acid at residue at residue 440), or 441 (e.g., an asparagine at residue 441); residues 13 (e.g., a phenylalanine at residue 13), 15, 60 (e.g., an aspartic acid at residue 60), 270, 289 (e.g., a histidine at residue 289), and 418; substitutions at residues 13, 60, and 270; substitutions at residues 60 and 87 (e.g., a phenylalanine at residue 87); substitutions at residues 65, 71 (e.g., a glutamine at residue 71), 220 (e.g., a threonine at residue 220), 243 (e.g., a tryptophan at residue 243), and 270; substitutions at residues 65, 71, 220, 243, 270, and 441; substitutions at residues 65, 71, 220, 389 (e.g., a valine at residue 389), and 394 (e.g., a valine at residue 394); substitutions at residues 65, 71, 270, and 289; substitutions at residues 220, 243, 270, and 334 (e.g., a serine at residue 334); or substitutions at residues 270 and 289. The following amino acid mutations did not result in a loss of activity in 85C2 polypeptides: V13F, F15L, H60D, A65S, E71Q, 187F, K220T, R243W, T270M, T270R, Q289H, L334S, A389V, 1394V, P397S, E418V, G440D, and H441N. Additional mutations that were seen in active clones include K9E, K10R, Q21H, M27V, L91P, Y298C, K350T, H368R, G420R, L431P, R444G, and M471T. In some embodiments, an UGT85C2 contains substitutions at positions 65 (e.g., a serine), 71 (a glutamine), 270 (a methionine), 289 (a histidine), and 389 (a valine).
The amino acid sequence of Stevia rebaudiana UGTs 74G1,76G1 and 91D2e with N-terminal, in-frame fusions of the first 158 amino acids of human MDM2 protein, and Stevia rebaudiana UGT85C2 with an N-terminal in-frame fusion of 4 repeats of the synthetic PMI peptide (4× TSFAEYWNLLSP, SEQ ID NO:87) as set forth in SEQ ID NOs: 88, 89, 90, and 91.
In some embodiments, a useful UGT76G homolog can have one or more amino acid substitutions at residues 29, 74, 87, 91, 116, 123, 125, 126, 130, 145, 192, 193, 194, 196, 198, 199, 200, 203, 204, 205, 206, 207, 208, 266, 273, 274, 284, 285, 291, 330, 331, and 346 of SEQ ID NO: 85.
Non-limiting examples of useful UGT76G homologs include polypeptides having substitutions at residues 74, 87, 91, 116, 123, 125, 126, 130, 145, 192, 193, 194, 196, 198, 199, 200, 203, 204, 205, 206, 207, 208, and 291; residues 74, 87, 91, 116, 123, 125, 126, 130, 145, 192, 193, 194, 196, 198, 199, 200, 203, 204, 205, 206, 207, 208, 266, 273, 274, 284, 285, and 291; or residues 74, 87, 91, 116, 123, 125, 126, 130, 145, 192, 193, 194, 196, 198, 199, 200, 203, 204, 205, 206, 207, 208, 266, 273, 274, 284, 285, 291, 330, 331, and 346. See, Table 10.
Methods to modify the substrate specificity of, for example, EUGT11 or UGT91D2e, are known to those skilled in the art, and include without limitation site-directed/rational mutagenesis approaches, random directed evolution approaches and combinations in which random mutagenesis/saturation techniques are performed near the active site of the enzyme. For example see Osmani et al. Phytochemistry 70: 325-347 (2009).
A candidate sequence typically has a length that is from 80 percent to 200 percent of the length of the reference sequence, e.g., 82, 85, 87, 89, 90, 93, 95, 97, 99, 100, 105, 110, 115, 120, 130, 140, 150, 160, 170, 180, 190, or 200 percent of the length of the reference sequence. A functional homolog polypeptide typically has a length that is from 95 percent to 105 percent of the length of the reference sequence, e.g., 90, 93, 95, 97, 99, 100, 105, 110, 115, or 120 percent of the length of the reference sequence, or any range between. A percent identity for any candidate nucleic acid or polypeptide relative to a reference nucleic acid or polypeptide can be determined as follows. A reference sequence (e.g., a nucleic acid sequence or an amino acid sequence) is aligned to one or more candidate sequences using the computer program ClustalW (version 1.83, default parameters), which allows alignments of nucleic acid or polypeptide sequences to be carried out across their entire length (global alignment). Chenna et al., Nucleic Acids Res., 31(13):3497-500 (2003).
ClustalW calculates the best match between a reference and one or more candidate sequences, and aligns them so that identities, similarities and differences can be determined. Gaps of one or more residues can be inserted into a reference sequence, a candidate sequence, or both, to maximize sequence alignments. For fast pairwise alignment of nucleic acid sequences, the following default parameters are used: word size: 2; window size: 4; scoring method: percentage; number of top diagonals: 4; and gap penalty: 5. For multiple alignment of nucleic acid sequences, the following parameters are used: gap opening penalty: 10.0; gap extension penalty: 5.0; and weight transitions: yes. For fast pairwise alignment of protein sequences, the following parameters are used: word size: 1; window size: 5; scoring method: percentage; number of top diagonals: 5; gap penalty: 3. For multiple alignment of protein sequences, the following parameters are used: weight matrix: blosum; gap opening penalty: 10.0; gap extension penalty: 0.05; hydrophilic gaps: on; hydrophilic residues: Gly, Pro, Ser, Asn, Asp, Gln, Glu, Arg, and Lys; residue-specific gap penalties: on. The ClustalW output is a sequence alignment that reflects the relationship between sequences. ClustalW can be run, for example, at the Baylor College of Medicine Search Launcher site on the World Wide Web (searchlauncher.bcm.tmc.edu/multi-align/multi-align.html) and at the European Bioinformatics Institute site on the World Wide Web (ebi.ac.uk/clustalw).
To determine percent identity of a candidate nucleic acid or amino acid sequence to a reference sequence, the sequences are aligned using ClustalW, the number of identical matches in the alignment is divided by the length of the reference sequence, and the result is multiplied by 100. It is noted that the percent identity value can be rounded to the nearest tenth. For example, 78.11, 78.12, 78.13, and 78.14 are rounded down to 78.1, while 78.15, 78.16, 78.17, 78.18, and 78.19 are rounded up to 78.2.
It will be appreciated that functional UGTs can include additional amino acids that are not involved in glucosylation or other enzymatic activities carried out by the enzyme, and thus such a polypeptide can be longer than would otherwise be the case. For example, a EUGT11 polypeptide can include a purification tag (e.g., HIS tag or GST tag), a chloroplast transit peptide, a mitochondrial transit peptide, an amyloplast peptide, signal peptide, or a excretion tag added to the amino or carboxy terminus. In some embodiments, a EUGT11 polypeptide includes an amino acid sequence that functions as a reporter, e.g., a green fluorescent protein or yellow fluorescent protein.
II. Steviol and Steviol Glycoside Biosynthesis Nucleic AcidsA recombinant gene encoding a polypeptide described herein comprises the coding sequence for that polypeptide, operably linked in sense orientation to one or more regulatory regions suitable for expressing the polypeptide. Because many microorganisms are capable of expressing multiple gene products from a polycistronic mRNA, multiple polypeptides can be expressed under the control of a single regulatory region for those microorganisms, if desired. A coding sequence and a regulatory region are considered to be operably linked when the regulatory region and coding sequence are positioned so that the regulatory region is effective for regulating transcription or translation of the sequence. Typically, the translation initiation site of the translational reading frame of the coding sequence is positioned between one and about fifty nucleotides downstream of the regulatory region for a monocistronic gene.
In many cases, the coding sequence for a polypeptide described herein is identified in a species other than the recombinant host, i.e., is a heterologous nucleic acid. Thus, if the recombinant host is a microorganism, the coding sequence can be from other prokaryotic or eukaryotic microorganisms, from plants or from animals. In some case, however, the coding sequence is a sequence that is native to the host and is being reintroduced into that organism. A native sequence can often be distinguished from the naturally occurring sequence by the presence of non-natural sequences linked to the exogenous nucleic acid, e.g., non-native regulatory sequences flanking a native sequence in a recombinant nucleic acid construct. In addition, stably transformed exogenous nucleic acids typically are integrated at positions other than the position where the native sequence is found. “Regulatory region” refers to a nucleic acid having nucleotide sequences that influence transcription or translation initiation and rate, and stability and/or mobility of a transcription or translation product. Regulatory regions include, without limitation, promoter sequences, enhancer sequences, response elements, protein recognition sites, inducible elements, protein binding sequences, 5′ and 3′ untranslated regions (UTRs), transcriptional start sites, termination sequences, polyadenylation sequences, introns, and combinations thereof. A regulatory region typically comprises at least a core (basal) promoter. A regulatory region also may include at least one control element, such as an enhancer sequence, an upstream element or an upstream activation region (UAR). A regulatory region is operably linked to a coding sequence by positioning the regulatory region and the coding sequence so that the regulatory region is effective for regulating transcription or translation of the sequence. For example, to operably link a coding sequence and a promoter sequence, the translation initiation site of the translational reading frame of the coding sequence is typically positioned between one and about fifty nucleotides downstream of the promoter. A regulatory region can, however, be positioned as much as about 5,000 nucleotides upstream of the translation initiation site, or about 2,000 nucleotides upstream of the transcription start site.
The choice of regulatory regions to be included depends upon several factors, including, but not limited to, efficiency, selectability, inducibility, desired expression level, and preferential expression during certain culture stages. It is a routine matter for one of skill in the art to modulate the expression of a coding sequence by appropriately selecting and positioning regulatory regions relative to the coding sequence. It will be understood that more than one regulatory region may be present, e.g., introns, enhancers, upstream activation regions, transcription terminators, and inducible elements.
One or more genes can be combined in a recombinant nucleic acid construct in “modules” useful for a discrete aspect of steviol and/or steviol glycoside production. Combining a plurality of genes in a module, particularly a polycistronic module, facilitates the use of the module in a variety of species. For example, a steviol biosynthesis gene cluster, or a UGT gene cluster, can be combined in a polycistronic module such that, after insertion of a suitable regulatory region, the module can be introduced into a wide variety of species. As another example, a UGT gene cluster can be combined such that each UGT coding sequence is operably linked to a separate regulatory region, to form a UGT module. Such a module can be used in those species for which monocistronic expression is necessary or desirable. In addition to genes useful for steviol or steviol glycoside production, a recombinant construct typically also contains an origin of replication, and one or more selectable markers for maintenance of the construct in appropriate species.
It will be appreciated that because of the degeneracy of the genetic code, a number of nucleic acids can encode a particular polypeptide; i.e., for many amino acids, there is more than one nucleotide triplet that serves as the codon for the amino acid. Thus, codons in the coding sequence for a given polypeptide can be modified such that optimal expression in a particular host is obtained, using appropriate codon bias tables for that host (e.g., microorganism). As isolated nucleic acids, these modified sequences can exist as purified molecules and can be incorporated into a vector or a virus for use in constructing modules for recombinant nucleic acid constructs.
In some cases, it is desirable to inhibit one or more functions of an endogenous polypeptide in order to divert metabolic intermediates towards steviol or steviol glycoside biosynthesis. For example, it may be desirable to downregulate synthesis of sterols in a yeast strain in order to further increase steviol or steviol glycoside production, e.g., by downregulating squalene epoxidase. As another example, it may be desirable to inhibit degradative functions of certain endogenous gene products, e.g., glycohydrolases that remove glucose moieties from secondary metabolites or phosphatases as discussed herein. As another example, expression of membrane transporters involved in transport of steviol glycosides can be inhibited, such that excretion of glycosylated steviosides is inhibited. Such regulation can be beneficial in that excretion of steviol glycosides can be inhibited for a desired period of time during culture of the microorganism, thereby increasing the yield of glycoside product(s) at harvest. In such cases, a nucleic acid that inhibits expression of the polypeptide or gene product may be included in a recombinant construct that is transformed into the strain. Alternatively, mutagenesis can be used to generate mutants in genes for which it is desired to inhibit function.
III. Expressing TransportersThe present document is directed to recombinant host cells in which expression of endogenous transporter genes is modified or in which heterologous transporter genes are expressed. In some embodiments, expression of an endogenous transporter can be modified by replacing the endogenous promoter with a different promoter that results in increased expression of the transporter protein (e.g., at least a 5% increase in expression, such as at least a 10%, 15%, 20%, or 25% increase in expression). For example, an endogenous promoter can be replaced with a constitutive or inducible promoter that results in increased expression of the transporter. Homologous recombination can be used to replace the promoter of an endogenous gene with a different promoter that results in increased expression of the transporter. In other embodiments the inducible or constitutive promoter and endogenous transporter or transcription factor gene can be integrated into another locus of the genome using homologous recombination. In other embodiments, the transporter gene can be introduced into a microorganism using exogenous plasmids with a promoter that results in overexpression of the transporter in the microorganim. In yet another embodiment, the exogenous plasmids may also contain multiple copies of the transporter gene. In a further embodiment, the endogenous transporter can be induced to be overexpressed using native mechanisms to the recombinant microorganism (e.g. heat shock, stress, heavy metal or antibiotic exposure). For example, oligomycin and/or cadmium can be added to the culture media (wherein YOR1 expression can be induced by said molecules) to increase expression of YOR1 and thereby excretion of steviol glycosides. See, for example Hallstrom & Moye-Rowley (1998) JBC 273(4): 2098-104; Nagy et al., (2006) Biochimie. 88(11):1665-71; and Katzmann et al., (1995) Mol Cell Biol. 15(12):6875-83.
As described herein, increasing expression of certain endogenous transporters or expressing a heterologous transporter in a recombinant host (e.g., expressing an S. rebaudiana transporter in a microorganism such as S. cerevisiae) can confer the ability to more efficiently produce and secrete steviol glycosides upon that host. The amount of extracellular and/or intracellular steviol glycoside produced during culturing the host can be measured by liquid chromatography-mass spectrometry (LC-MS) as described herein.
A transporter (also referred to as a membrane transport protein) is a membrane protein involved in the movement of molecules and ions across a biological membrane. Transporters span the membrane in which they are localized and across which they transport substances. Transporters can operate to move substances by facilitated diffusion or by active transport. Transport proteins have been classified according to various criteria at the Transporter Classification Database. See, Saier Jr. et al., Nucl. Acids Res., 37:D274-278 (2009). Two families of plasma membrane transporters are thought to be ubiquitous among living organisms: the ATP-Binding Cassette (ABC) transporters and the Major Facilitator Superfamily (MFS) transporters. ATP-binding cassette transporters (ABC transporters) are transmembrane proteins that utilize the energy of adenosine triphosphate (ATP) hydrolysis to carry out translocation of various substrates across membranes. They can transport a wide variety of substrates across extra- and intracellular membranes, including metabolic products, lipids and sterols, and drugs. Proteins are classified as ABC transporters based on the sequence and organization of their ATP-binding cassette domain. Typically, ABC family transporters are multicomponent primary active transporters, capable of transporting molecules in response to ATP hydrolysis. Non-limiting examples of endogenous ABC transporter genes include the genes at the PDR5, PDR10, PDR15, SNQ2, YOR1, YOL075c and PDR18 (or a functional homolog thereof).
The Major Facilitator Superfamily (MFS) transporters are polypeptides that can transport small solutes in response to chemiosmotic ion gradients. Saier, Jr. et al., J. Mol. Microbiol. Biotechnol. 1:257-279 (1999). The MFS transporter family is sometimes referred to as the uniporter-symporter-antiporter family. MFS transporters function in, inter alia, in sugar uptake and drug efflux systems. MFS transporters typically contain conserved MFS-specific motifs. Non-limiting examples of endogenous MFS transporter genes include the genes at the TPO1, TPO3, and FLR1 loci (or a functional homolog thereof).
Other transporter families include the SMR (small multidrug resistant) family, RND (Resistance-Nodulation-Cell Division) family, and the MATE (multidrug and toxic compound extrusion) family. The SMR family members are integral membrane proteins characterized by four alpha-helical transmembrane strands that confer resistance to a broad range of antiseptics, lipophilic quaternary ammonium compounds (QAC), and aminoglycoside resistance in bacteria. See, Bay and Turner, BMC Evol Biol., 9: 140 (2009). For example, EmrE efflux transporter of Escherichia coli (GenBank: BAE76318.1; SEQ ID NO: 92) is involved with aminoglycoside resistance. It is a homooligomer that extrudes positively charged aromatic drugs (i.e., methyl viologen or ethidium) in exchange for two protons.
The RND family members are widespread, including among Gram-negative bacteria, and catalyze the active efflux of many antibiotics and chemotherapeutic agents. See, Nikaido and Takatsuk, Biochim Biophys Acta., 1794(5):769-81 (2009). An exemplary protein is AcrAB from Escherichia coli that is involved in erythromycin D transport (GenBank: BAE76241.1; SEQ ID NO: 93, and AAA23410.1; SEQ ID NO: 94).
The MATE family members contain 12 transmembrane (TM) domains. Members of the MATE family have been identified in prokaryotes, yeast such as Saccharomyces cerevisiae and Schizosaccharomyces pombe, and plants. Diener et al., Plant Cell. 13(7): 1625-1638 (2001). The MATE family members are sodium or proton antiporters. An exemplary target molecule is ydhE from E. coli (GenBank AAB47941.1; SEQ ID NO: 95), which transports fluoroquinolones, kanamycin, streptomycin, other aminoglycosides and Berberine.
A. Transcription FactorsModification of transcription factor expression can also be used to increase transporter expression. For example, the yeast transcriptions factors PDR1 and/or PDR3 regulate expression of the genes encoding ABC transporters PDR5, SNQ2 and YOR1. Therefore, in some embodiments, promoters for the endogenous PDR1 and PDR3 loci can be replaced with a different promoter that results in increased expression of the transcription factors, which can increase production of endogenous transporters. In other embodiments, the transcription factors can be introduced into a microorganism using exogenous plasmids with a promoter that results in overexpression of the transcription factor in the microorganims. In yet another embodiment, the exogenous plasmids may also contain multiple copies of the transcription factor. In a further embodiment, the endogenous transcription factor can be activated or induced to be overexpressed using native mechanisms to the recombinant microorganism (e.g. heat shock, stress, heavy metal or antibiotic exposure).
B. Identifying Genes Affecting Excretion of Steviol Pathway IntermediatesMethods for identifying a gene affecting excretion of steviol pathway intermediates are disclosed herein. Such methods can involve inactivating at least one endogenous transporter gene or modifying expression of at least one transporter gene. Typically, a library of mutant microorganisms is prepared, each mutant in the library having a different endogenous transporter gene inactivated. In some embodiments, expression of a different endogenous transporter gene is modified in each microorganism in the library. The parent microorganism in which the modifications are generated can lack steviol glycoside pathway genes, although it can contain one or more of such genes if desired. Generally, it is more convenient to generate modifications in the absence of steviol glycoside pathway genes, and subsequently introduce those pathway genes that facilitate production of a desired different target glycoside product. The mutant microorganisms containing one or more steviol glycoside pathway genes are cultured in a medium under conditions in which steviol or a steviol glycoside is synthesized, and the amount of extracellular and/or intracellular steviol glycoside pathway intermediates produced by the microorganism is measured (e.g., using LC-MS) as described herein.
The intermediate(s) that is characterized depends upon the particular pathway of interest in the microorganism. For example, a microorganism expressing the 76G1, 74G1, 91D2e, and 85C2 UGTs (described below) can synthesize the target product rebaudioside A from steviol, via intermediate compounds steviol-19-O-glucoside (19-SMG), rubusoside and stevioside. See
The present document can be directed to recombinant hosts comprising one or more inactivated endogenous transporter genes. An endogenous transporter gene typically is inactivated by disrupting expression of the gene or introducing a mutation to reduce or even completely eliminate transporter activity in a host comprising the mutation, e.g., a disruption in one or more endogenous transporter genes, such that the host has reduced transporter expression or activity for the transporter encoded by the disrupted gene.
In some embodiments, a transporter that is knocked out can also have specificity for excretion of larger molecular weight rebaudiosides (for example, RebA), and therefore, can be useful to overexpress in strains where excretion of RebA into the medium is desired. With appropriate balancing of the rate of glycosylation activity through expression of pathway UGTs, smaller molecular weight steviol glycosides are further glycosylated before they are excreted into the medium. For example, higher expression levels of a UGT76G1 and UGT91D2e and/or EUGT11 as compared to the UGT74G1 and UGT85C2 enzymes can prevent accumulation of the steviol monoglucosides that are excreted more readily. If the UGT activity level is higher (so the glycosylation rate is faster) than the rate of transport, then more larger molecular weight steviol glycosides will be produced.
Since many transporters have overlapping substrate specificity and since disruptions in certain transporters are compensated for by up-regulation of other transporters, it is often useful to generate a host that contains a plurality of inactivated transporter genes. For example, as described herein, the PDR5, PDR10, PDR15 and SNQ2 loci can be disrupted as set forth in the Examples below. In some embodiments, the TPO1, PDR5, PDR10, PDR15 and SNQ2 loci can be disrupted as set forth in the Examples below.
Additional transporter genes that can be inactivated can be identified based on the function of related sequences, e.g., the sequences found at the yeast PDR5, PDR10, PDR15 and SNQ2 loci. Endogenous transporter genes can be inactivated by mutations that disrupt the gene. For example, a gene replacement vector can be constructed in such a way to include a selectable marker gene flanked at both the 5′ and 3′ ends by portions of the transporter gene of sufficient length to mediate homologous recombination. The selectable marker can be one of any number of genes that complement host cell auxotrophy, provide antibiotic resistance, or result in a color change. Linearized DNA fragments of the gene replacement vector, containing no plasmid DNA or ars element, are then introduced into cells using known methods. Integration of the linear fragment into the genome and the disruption of the transporter gene can be determined based on the selection marker and can be verified by, for example, Southern blot analysis. The resulting cells contain an inactivated mutant transporter gene, due to insertion of the selectable marker at the locus for the transporter. A deletion-disruption gene replacement vector can be constructed in a similar way using known techniques and, by way of homologous recombination, integrated in the endogenous transporter gene, thereby inactivating it. In some embodiments, the selectable marker can be removed from the genome of the host cell after determining that the desired disruption mutation has been introduced. See, e.g., Gossen et al. (2002) Ann. Rev. Genetics 36:153-173 and U.S. Application Publication No. 20060014264.
Endogenous transporter genes can also be inactivated by utilizing transcription activator-like effector nucleases (TALENs) or modified zinc finger nucleases to introduce desired insertion or deletion mutations. See, US Patent Publication No. 2012-0178169. In some embodiments, an endogenous transporter gene is inactivated by introducing a mutation that results in insertions of nucleotides, deletions of nucleotides, or transition or transversion point mutations in the wild-type transporter gene sequence. Other types of mutations that may be introduced in a transporter gene include duplications and inversions in the wild-type sequence. Mutations can be made in the coding sequence at a transporter locus, as well as in noncoding sequences such as regulatory regions, introns, and other untranslated sequences. Mutations in the coding sequence can result in insertions of one or more amino acids, deletions of one or more amino acids, and/or non-conservative amino acid substitutions in the corresponding gene product. In some cases, the sequence of a transporter gene comprises more than one mutation or more than one type of mutation. Insertion or deletion of amino acids in a coding sequence can, for example, disrupt the conformation of a substrate binding pocket of the resulting gene product.
Amino acid insertions or deletions can also disrupt catalytic sites important for gene product activity. It is known in the art that the insertion or deletion of a larger number of contiguous amino acids is more likely to render the gene product non-functional, compared to a smaller number of inserted or deleted amino acids. Non-conservative substitutions can make a substantial change in the charge or hydrophobicity of the gene product. Non-conservative amino acid substitutions can also make a substantial change in the bulk of the residue side chain, e.g., substituting an alanine residue for a isoleucine residue. Examples of non-conservative substitutions include a basic amino acid for a non-polar amino acid, or a polar amino acid for an acidic amino acid.
In some embodiments, a mutation in a transporter gene may result in no amino acid changes but, although not affecting the amino acid sequence of the encoded transporter, may alter transcriptional levels (e.g., increasing or decreasing transcription), decrease translational levels, alter secondary structure of DNA or mRNA, alter binding sites for transcriptional or translational machinery, or decrease tRNA binding efficiency.
Mutations in transporter loci can be generated by site-directed mutagenesis of the transporter gene sequence in vitro, followed by homologous recombination to introduce the mutation into the host genome as described above. However, mutations can also be generated by inducing mutagenesis in cells of the host, using a mutagenic agent to induce genetic mutations within a population of cells. Mutagenesis is particularly useful for those species or strains for which in vitro mutagenesis and homologous recombination is less well established or is inconvenient. The dosage of the mutagenic chemical or radiation for a particular species or strain is determined experimentally such that a mutation frequency is obtained that is below a threshold level characterized by lethality or reproductive sterility.
A. Transcription FactorsModification of transcription factor expression can also be used to reduce or eliminate transporter expression. For example, the yeast transcriptions factors PDR1 and/or PDR3 regulate expression of the genes encoding ABC transporters PDR5, SNQ2 and YOR1. Disrupting the loci or reducing expression of PDR1 and/or PDR3 can result in a detectable decrease in excretion of steviol glycoside intermediates. Therefore, in some embodiments, a yeast host contains inactivated endogenous PDR1 and PDR3 loci in combination with a plurality of inactivated transporter genes, to provide a larger reduction in excretion of intermediates than that provided by inactivation of any single transporter or transcription factor. In another embodiment, a transcription factor identified to decrease steviol glycoside excretion by disrupting or reducing the transcription factor's expression, can then be overexpressed in a recombinant microorganism in order to increase excretion of steviol glycosides.
B. Identifying Genes Affecting Excretion of Steviol Pathway IntermediatesMethods for identifying a gene affecting excretion of steviol pathway intermediates are disclosed herein. Such methods involve inactivating, disrupting or decreasing expression of at least one endogenous transporter gene. Typically, a library of mutant microorganisms is prepared, each mutant in the library having a different endogenous transporter gene inactivated, disrupted or with decreased expression. The parent microorganism in which the mutations are generated can lack steviol glycoside pathway genes, although it can contain one or more of such genes. Generally, it is more convenient to generate mutations in the absence of steviol glycoside pathway genes, and subsequently introduce those pathway genes that facilitate production of a desired different target glycoside product. The mutant microorganisms containing one or more steviol glycoside pathway genes can be cultured in a medium under conditions in which steviol or a steviol glycoside is synthesized, and the amount of extracellular and/or intracellular steviol glycoside pathway intermediates produced by the microorganism can be measured.
The intermediate(s) that is characterized depends upon the particular pathway of interest in the microorganism. For example, a microorganism expressing the 76G1, 74G1, 91D2e, and 85C2 UGTs (described below) can synthesize the target product rebaudioside A from steviol, via intermediate compounds steviol-19-O-glucoside (19-SMG), steviol-13-O-glucose (13-SMG), rubusoside and stevioside. See
A number of prokaryotes and eukaryotes are suitable for use in constructing the recombinant microorganisms described herein, e.g., gram-negative bacteria, yeast and fungi. A species and strain selected for use as a steviol or steviol glycoside production strain is first analyzed to determine which production genes are endogenous to the strain and which genes are not present. Genes for which an endogenous counterpart is not present in the strain are assembled in one or more recombinant constructs, which are then transformed into the strain in order to supply the missing function(s).
Exemplary prokaryotic and eukaryotic species are described in more detail below. However, it will be appreciated that other species may be suitable. For example, suitable species may be in Saccharomycetes. Additional suitable species may be in a genus selected from the group consisting of Agaricus, Aspergillus, Bacillus, Candida, Corynebacterium, Escherichia, Fusarium/Gibberella, Kluyveromyces, Laetiporus, Lentinus, Phaffia, Phanerochaete, Pichia, Physcomitrella, Rhodoturula, Saccharomyces, Schizosaccharomyces, Sphaceloma, Xanthophyllomyces and Yarrowia.
Exemplary species from such genera include Lentinus tigrinus, Laetiporus sulphureus, Phanerochaete chrysosporium, Pichia pastoris, Physcomitrella patens, Rhodoturula glutinis 32, Rhodoturula mucilaginosa, Phaffia rhodozyma UBV-AX, Xanthophyllomyces dendrorhous, Fusarium fujikuroi/Gibberella fujikuroi, Candida utilis and Yarrowia lipolytica. In some embodiments, a microorganism can be an Ascomycete such as Gibberella fujikuroi, Kluyveromyces lactis, Schizosaccharomyces pombe, Aspergillus niger, or Saccharomyces cerevisiae. In some embodiments, a microorganism can be a prokaryote such as Escherichia coli, Rhodobacter sphaeroides, or Rhodobacter capsulatus. It will be appreciated that certain microorganisms can be used to screen and test genes of interest in a high throughput manner, while other microorganisms with desired productivity or growth characteristics can be used for large-scale production of steviol glycosides.
Saccharomyces cerevisiae and Related Yeast Species
Saccharomyces cerevisiae is a widely used chassis organism in synthetic biology, and can be used as the recombinant microorganism platform. There are libraries of mutants, plasmids, detailed computer models of metabolism and other information available for S. cerevisiae, allowing for rational design of various modules to enhance product yield. Methods are known for making recombinant microorganisms. A steviol biosynthesis gene cluster can be expressed in yeast, particularly Saccharomycetes, using any of a number of known promoters. Strains that overproduce terpenes are known and can be used to increase the amount of geranylgeranyl diphosphate available for steviol and steviol glycoside production. Saccharomyces cerevisiae is an exemplary Saccharomyces species.
Aspergillus spp.
Aspergillus species such as A. oryzae, A. niger and A. sojae are widely used microorganisms in food production, and can also be used as the recombinant microorganism platform. Nucleotide sequences are available for genomes of A. nidulans, A. fumigatus, A. oryzae, A. clavatus, A. flavus, A. niger, and A. terreus, allowing rational design and modification of endogenous pathways to enhance flux and increase product yield. Metabolic models have been developed for Aspergillus, as well as transcriptomic studies and proteomics studies. A. niger is cultured for the industrial production of a number of food ingredients such as citric acid and gluconic acid, and thus species such as A. niger are generally suitable for the production of food ingredients such as steviol and steviol glycosides.
Escherichia coli
Escherichia coli, another widely used platform organism in synthetic biology, can also be used as the recombinant microorganism platform. Similar to Saccharomyces, there are libraries of mutants, plasmids, detailed computer models of metabolism and other information available for E. coli, allowing for rational design of various modules to enhance product yield. Methods similar to those described above for Saccharomyces can be used to make recombinant E. coli microorganisms.
Agaricus, Gibberella, and Phanerochaete spp.
Agaricus, Gibberella, and Phanerochaete spp. can be useful because they are known to produce large amounts of gibberellin in culture. Thus, the terpene precursors for producing large amounts of steviol and steviol glycosides are already produced by endogenous genes. Thus, modules containing recombinant genes for steviol or steviol glycoside biosynthesis polypeptides can be introduced into species from such genera without the necessity of introducing mevalonate or MEP pathway genes.
Arxula adeninivorans (Blastobotrys adeninivorans)
Arxula adeninivorans is a dimorphic yeast (it grows as a budding yeast like the baker's yeast up to a temperature of 42° C., above this threshold it grows in a filamentous form) with unusual biochemical characteristics. It can grow on a wide range of substrates and can assimilate nitrate. It has successfully been applied to the generation of strains that can produce natural plastics or the development of a biosensor for estrogens in environmental samples.
Yarrowia lipolytica
Yarrowia lipolytica is a dimorphic yeast (see Arxula adeninivorans) that can grow on a wide range of substrates. It has a high potential for industrial applications but there are no recombinant products commercially available yet.
Rhodobacter spp.
Rhodobacter can be use as the recombinant microorganism platform. Similar to E. coli, there are libraries of mutants available as well as suitable plasmid vectors, allowing for rational design of various modules to enhance product yield. Isoprenoid pathways have been engineered in membraneous bacterial species of Rhodobacter for increased production of carotenoid and CoQ10. See, U.S. Patent Publication Nos. 20050003474 and 20040078846. Methods similar to those described above for E. coli can be used to make recombinant Rhodobacter microorganisms.
Candida boidinii
Candida boidinii is a methylotrophic yeast (it can grow on methanol). Like other methylotrophic species such as Hansenula polymorpha and Pichia pastoris, it provides an excellent platform for the production of heterologous proteins. Yields in a multigram range of a excreted foreign protein have been reported. A computational method, IPRO, recently predicted mutations that experimentally switched the cofactor specificity of Candida boidinii xylose reductase from NADPH to NADH.
Hansenula polymorpha (Pichia angusta)
Hansenula polymorpha is another methylotrophic yeast (see Candida boidinii). It can furthermore grow on a wide range of other substrates; it is thermo-tolerant and can assimilate nitrate (see also Kluyveromyces lactis). It has been applied to the production of hepatitis B vaccines, insulin and interferon alpha-2a for the treatment of hepatitis C, furthermore to a range of technical enzymes.
Kluyveromyces lactis
Kluyveromyces lactis is a yeast regularly applied to the production of kefir. It can grow on several sugars, most importantly on lactose which is present in milk and whey. It has successfully been applied among others to the production of chymosin (an enzyme that is usually present in the stomach of calves) for the production of cheese. Production takes place in fermenters on a 40,000 L scale.
Pichia pastoris
Pichia pastoris is a methylotrophic yeast (see Candida boidinii and Hansenula polymorpha). It provides an efficient platform for the production of foreign proteins. Platform elements are available as a kit and it is worldwide used in academia for the production of proteins. Strains have been engineered that can produce complex human N-glycan (yeast glycans are similar but not identical to those found in humans).
Physcomitrella spp.
Physcomitrella mosses, when grown in suspension culture, have characteristics similar to yeast or other fungal cultures. This genera is becoming an important type of cell for production of plant secondary metabolites, which can be difficult to produce in some other types of cells.
VI. Methods of Producing Steviol GlycosidesRecombinant microorganisms described herein can be used in methods to produce steviol or steviol glycosides. For example, the method can include growing the recombinant microorganism in a culture medium under conditions in which steviol and/or steviol glycoside biosynthesis genes are expressed. The recombinant microorganism may be grown in a fed batch or continuous process. Typically, the recombinant microorganism is grown in a fermentor at a defined temperature(s) for a desired period of time. Depending on the particular microorganism used in the method, other recombinant genes such as isopentenyl biosynthesis genes and terpene synthase and cyclase genes may also be present and expressed. Levels of substrates and intermediates, e.g., isopentenyl diphosphate, dimethylallyl diphosphate, geranylgeranyl diphosphate, kaurene and kaurenoic acid, can be determined by extracting samples from culture media for analysis according to published methods.
After the recombinant microorganism has been grown in culture for the desired period of time, steviol and/or one or more steviol glycosides can then be recovered from the culture using various techniques known in the art. In some embodiments, a permeabilizing agent can be added to aid the feedstock entering into the host and product getting out. For example, a crude lysate of the cultured microorganism can be centrifuged to obtain a supernatant. The resulting supernatant can then be applied to a chromatography column, e.g., a C-18 column, and washed with water to remove hydrophilic compounds, followed by elution of the compound(s) of interest with a solvent such as methanol. The compound(s) can then be further purified by preparative HPLC. See also WO 2009/140394.
The amount of steviol glycoside (e.g., rebaudioside A or rebaudioside D) produced can be from about 1 mg/L to about 2000 mg/L, e.g., about 1 to about 10 mg/L, about 3 to about 10 mg/L, about 5 to about 20 mg/L, about 10 to about 50 mg/L, about 10 to about 100 mg/L, about 25 to about 500 mg/L, about 100 to about 1,500 mg/L, or about 200 to about 1,000 mg/L, at least about 1,000 mg/L, at least about 1,200 mg/L, at least about at least 1,400 mg/L, at least about 1,600 mg/L, at least about 1,800 mg/L, or at least about 2,000 mg/L. In general, longer culture times will lead to greater amounts of product. Thus, the recombinant microorganism can be cultured for from 1 day to 7 days, from 1 day to 5 days, from 3 days to 5 days, about 3 days, about 4 days, or about 5 days.
It will be appreciated that the various genes and modules discussed herein can be present in two or more recombinant microorganisms rather than a single microorganism. When a plurality of recombinant microorganisms is used, they can be grown in a mixed culture to produce steviol and/or steviol glycosides. For example, a first microorganism can comprise one or more biosynthesis genes for producing steviol and null mutations in a first group of endogenous transporters, while a second microorganism comprises steviol glycoside biosynthesis genes and null mutations in a second group of endogenous transporters.
Alternatively, the two or more microorganisms each can be grown in a separate culture medium and the product of the first culture medium, e.g., steviol, can be introduced into second culture medium to be converted into a subsequent intermediate, or into an end product such as rebaudioside A. The product produced by the second, or final microorganism is then recovered. The microorganisms can have the same or a different group of mutations in endogenous transporters. It will also be appreciated that in some embodiments, a recombinant microorganism is grown using nutrient sources other than a culture medium and utilizing a system other than a fermentor.
Steviol glycosides do not necessarily have equivalent performance in different food systems. It is therefore desirable to have the ability to direct the synthesis to steviol glycoside compositions of choice. Recombinant hosts described herein can produce compositions that are selectively enriched for specific steviol glycosides (e.g., rebaudioside D) and have a consistent taste profile. Thus, the recombinant microorganisms described herein can facilitate the production of compositions that are tailored to meet the sweetening profile desired for a given food product and that have a proportion of each steviol glycoside that is consistent from batch to batch. Microorganisms described herein do not produce the undesired plant byproducts found in Stevia extracts. Thus, steviol glycoside compositions produced by the recombinant microorganisms described herein are distinguishable from compositions derived from Stevia plants.
VII. Steviol Glycosides, Compositions, and Food ProductsSteviol glycosides and compositions obtained by the methods disclosed herein can be used to make food products, dietary supplements and sweetener compositions. For example, substantially pure steviol or steviol glycoside such as rebaudioside A or rebaudioside D can be included in food products such as ice cream, carbonated beverages, fruit juices, yogurts, baked goods, chewing gums, hard and soft candies, and sauces. Substantially pure steviol or steviol glycoside can also be included in non-food products such as pharmaceutical products, medicinal products, dietary supplements and nutritional supplements. Substantially pure steviol or steviol glycosides may also be included in animal feed products for both the agriculture industry and the companion animal industry. Alternatively, a mixture of steviol and/or steviol glycosides can be made by culturing recombinant microorganisms separately, each producing a specific steviol or steviol glycoside, recovering the steviol or steviol glycoside in substantially pure form from each microorganism and then combining the compounds to obtain a mixture containing each compound in the desired proportion. The recombinant microorganisms described herein permit more precise and consistent mixtures to be obtained compared to current Stevia products. In another alternative, a substantially pure steviol or steviol glycoside can be incorporated into a food product along with other sweeteners, e.g. saccharin, dextrose, sucrose, fructose, erythritol, aspartame, sucralose, monatin, or acesulfame potassium. The weight ratio of steviol or steviol glycoside relative to other sweeteners can be varied as desired to achieve a satisfactory taste in the final food product. See, e.g., U.S. Patent Publication No. 2007/0128311. In some embodiments, the steviol or steviol glycoside may be provided with a flavor (e.g., citrus) as a flavor modulator.
Compositions produced by a recombinant microorganism described herein can be incorporated into food products. For example, a steviol glycoside composition produced by a recombinant microorganism can be incorporated into a food product in an amount ranging from about 20 mg steviol glycoside/kg food product to about 1800 mg steviol glycoside/kg food product on a dry weight basis, depending on the type of steviol glycoside and food product. For example, a steviol glycoside composition produced by a recombinant microorganism can be incorporated into a dessert, cold confectionary (e.g., ice cream), dairy product (e.g., yogurt), or beverage (e.g., a carbonated beverage) such that the food product has a maximum of 500 mg steviol glycoside/kg food on a dry weight basis. A steviol glycoside composition produced by a recombinant microorganism can be incorporated into a baked good (e.g., a biscuit) such that the food product has a maximum of 300 mg steviol glycoside/kg food on a dry weight basis. A steviol glycoside composition produced by a recombinant microorganism can be incorporated into a sauce (e.g., chocolate syrup) or vegetable product (e.g., pickles) such that the food product has a maximum of 1000 mg steviol glycoside/kg food on a dry weight basis. A steviol glycoside composition produced by a recombinant microorganism can be incorporated into a bread such that the food product has a maximum of 160 mg steviol glycoside/kg food on a dry weight basis. A steviol glycoside composition produced by a recombinant microorganism, plant, or plant cell can be incorporated into a hard or soft candy such that the food product has a maximum of 1600 mg steviol glycoside/kg food on a dry weight basis. A steviol glycoside composition produced by a recombinant microorganism, plant, or plant cell can be incorporated into a processed fruit product (e.g., fruit juices, fruit filling, jams, and jellies) such that the food product has a maximum of 1000 mg steviol glycoside/kg food on a dry weight basis.
For example, such a steviol glycoside composition can have from 90-99% rebaudioside A and an undetectable amount of stevia plant-derived contaminants, and be incorporated into a food product at from 25-1600 mg/kg, e.g., 100-500 mg/kg, 25-100 mg/kg, 250-1000 mg/kg, 50-500 mg/kg or 500-1000 mg/kg on a dry weight basis.
Such a steviol glycoside composition can be a rebaudioside B-enriched composition having greater than 3% rebaudioside B and be incorporated into the food product such that the amount of rebaudioside B in the product is from 25-1600 mg/kg, e.g., 100-500 mg/kg, 25-100 mg/kg, 250-1000 mg/kg, 50-500 mg/kg or 500-1000 mg/kg on a dry weight basis. Typically, the rebaudioside B-enriched composition has an undetectable amount of stevia plant-derived contaminants.
Such a steviol glycoside composition can be a rebaudioside D-enriched composition having greater than 3% rebaudioside D and be incorporated into the food product such that the amount of rebaudioside D in the product is from 25-1600 mg/kg, e.g., 100-500 mg/kg, 25-100 mg/kg, 250-1000 mg/kg, 50-500 mg/kg or 500-1000 mg/kg on a dry weight basis. Typically, the rebaudioside D-enriched composition has an undetectable amount of stevia plant-derived contaminants.
Such a steviol glycoside composition can be a rebaudioside E-enriched composition having greater than 3% rebaudioside E and be incorporated into the food product such that the amount of rebaudioside E in the product is from 25-1600 mg/kg, e.g., 100-500 mg/kg, 25-100 mg/kg, 250-1000 mg/kg, 50-500 mg/kg or 500-1000 mg/kg on a dry weight basis. Typically, the rebaudioside E-enriched composition has an undetectable amount of stevia plant-derived contaminants.
Such a steviol glycoside composition can be a rebaudioside M-enriched composition having greater than 3% rebaudioside M and be incorporated into the food product such that the amount of rebaudioside M in the product is from 25-1600 mg/kg, e.g., 100-500 mg/kg, 25-100 mg/kg, 250-1000 mg/kg, 50-500 mg/kg or 500-1000 mg/kg on a dry weight basis. Typically, the rebaudioside M-enriched composition has an undetectable amount of stevia plant-derived contaminants.
In some embodiments, a substantially pure steviol or steviol glycoside is incorporated into a tabletop sweetener or “cup-for-cup” product. Such products typically are diluted to the appropriate sweetness level with one or more bulking agents, e.g., maltodextrins, known to those skilled in the art. Steviol glycoside compositions enriched for rebaudioside A, rebaudioside B, rebaudioside D, rebaudioside E, or rebaudioside M, can be package in a sachet, for example, at from 10,000 to 30,000 mg steviol glycoside/kg product on a dry weight basis, for tabletop use.
The invention will be further described in the following examples, which do not limit the scope of the invention described in the claims.
EXAMPLES Example 1. LC-MS Analytical ProceduresLC-MS analyses were performed using an Ultimate 3000 UPLC system (Dionex) fitted with a waters acquity UPLC® BEH shield RP18 column (2.1×50 mm, 1.7 m particles, 130 Å pore size) connected to a TSQ Quantum Access (ThermoFisher Scientific) triple quadropole mass spectrometer with a heated electrospray ion (HESI) source, unless otherwise indicated. Elution was carried out using a mobile phase of eluent B (MeCN with 0.1% Formic acid) and eluent A (water with 0.1% Formic acid) by increasing the gradient from 25% to 4700 B from min. 0.0 to 4.0, increasing 47% to 100% B in min. 4.0 to 5.0, holding 100% B from min. 5.0 to 6.5 re-equilibration. The flow rate was 0.4m/min and the column temperature 35° C. The steviol glycosides were detected using SIM (Single Ion Monitoring) with the following m/z-traces.
The levels of steviol glycosides were quantified by comparing with calibration curves obtained with authentic standards from LGC Standards. For example, standard solutions of 0.5 to 100 μM Rebaudioside A were typically utilized to construct a calibration curve.
Example 2. Construction of Rebaudioside Producing Yeast StrainsA. Yeast strain EFSC2772 was constructed from a wild type Saccharomyces cerevisiae strain containing three auxotrophic modifications, namely the deletions of URA3, LEU2 and HIS3. The wild type strain can be manipulated using standard genetic methods and can be used as a regular diploid or haploid yeast strain. EFSC2772 was converted to a steviol glycoside producing yeast by genomic-integration of four DNA constructs. Each construct contained multiple genes that were introduced into the yeast genome by homologous recombination. Furthermore, construct one and two were assembled by homologous recombination.
The first construct contained eight genes and was inserted in the DPP1 locus and disrupts and partially deletes DPP1 (phosphatase). The DNA inserted contains: the Ashbya gossypii TEF promoter expressing the natMX gene (selectable marker) followed by the TEF terminator from A. gossypii; Gene Art codon optimized Stevia rebaudiana UGT85C2 (GenBank AAR06916.1; SEQ ID NO: 32) expressed from the native yeast GPD1 promoter and followed by the native yeast CYC1 terminator; S. rebaudiana CPR-8 (SEQ ID NO: 24) expressed using the native yeast TPI1 promoter followed by the native yeast TDH1 terminator; Arabidopsis thaliana Kaurene synthase (similar to GenBank AEE36246.1; SEQ ID NO: 96) expressed from the native yeast PDC1 promoter and followed by the native yeast FBA1 terminator; Synechococcus sp. GGPPS (GenBank ABC98596.1, SEQ ID NO: 97) expressed using the native yeast TEF2 promoter and followed by the native yeast PGI1 terminator; DNA2.0 codon-optimized S. rebaudiana KAHe1 (SEQ ID NO: 18), expressed from the native yeast TEF1 promoter and followed by the native yeast ENO2 terminator; S. rebaudiana KO-1 (GenBank ABA42921.1, gi 76446107; SEQ ID NO: 98) expressed using the native yeast FBA1 promoter and followed by the native yeast TDH2 terminator; and Zea mays truncated CDPS expressed using the native yeast PGK1 promoter and followed by the native yeast ADH2 terminator.
The second construct was inserted at the YPRCA15 locus and contained the TEF1 promoter from A. gossypii in front of the kanMX gene (selectable marker) followed by the TEF1 terminator from A. gossypii, the Gene Art codon optimized A. thaliana ATR2 (SEQ ID NO: 99) expressed from the native yeast PGK1 promoter followed by the native yeast ADH2 terminator, S. rebaudiana UGT74G1 (GenBank AAR06920.1; SEQ ID NO: 100) expressed from the native yeast TPI1 promoter followed by the native yeast TDH1 terminator, Gene Art codon-optimized S. rebaudiana UGT76G1 (GenBank AAR06912; SEQ ID NO: 101) expressed from the native yeast TEF1 promoter followed by the native yeast ENO2 terminator, and GeneArt codon-optimized S. rebaudiana UGT91D2e-b which produces a UGT91D2e polypeptide with the amino acid modifications: L211M and V286A, (SEQ ID NO: 54 for UGT91D2e amino acid sequence for the wild type sequence; codon optimized nucleotide sequence is set forth in SEQ ID NO: 102) expressed from the native yeast GPD1 promoter and followed by the native yeast CYC1 terminator.
The first and the second construct were combined in the same spore clone by mating and dissection. This yeast strain was subsequently transformed with construct three and four in two successive events.
Construct three was integrated between genes PRP5 and YBR238C and contained the Kluyveromyces lactis LEU2 promoter expressing the K. lactis LEU2 gene followed by the LEU2 terminator from K. lactis, the native yeast GPD1 promoter expressing the DNA2.0-optimized S. rebaudiana KAHe1(SEQ ID NO: 18) followed by the native yeast CYC1 terminator, and the native yeast TPI1 promoter expressing the Zea mays truncated CDPS (SEQ ID NO: 103) followed by the native yeast TPI1 terminator.
Construct four was integrated in the genome between genes ECM3 and YOR093C and contained the TEF promoter from A. gossypii expressing the K. pneumoniae hphMX gene, followed by the TEF1 terminator from A. gossypii; Synechococcus sp. GGPPS (SEQ ID NO: 97) expressed from the native yeast GPD1 promoter, followed by the native yeast CYC1 terminator, followed by the native yeast TPI1 promoter expressing the A. thaliana Kaurene synthase (SEQ ID NO: 96) followed by the native yeast TPI1 terminator.
The strain was made prototrophic by introduction of the two plasmids p413TEF (CEN/ARS shuttle plasmid with HIS3 marker) and p416-TEF (CEN/ARS shuttle plasmid with URA3 marker) by transformation, and designated EFSC2772.
As evidenced by LC-MS, combined cellular and extracellular product concentrations were between 920-1660 mg/L of RebA and approximately 300-320 mg/L of RebD in two different batches of EFSC2772, approximately 700 mg/L of RebA was detected in the broth when the higher titer results were obtained. Additionally a large peak was seen for RebB, and one skilled in the art will recognize that additional copies of UGT74G1 or upregulation of UGT74G1 will further increase the conversion of RebB to RebA. Conversely, if RebB is the target glycoside, then UGT74G1 can be disrupted or deleted from the chromosome.
B. EFSC2763 yeast strain is derived from a wild type Saccharomyces cerevisiae strain containing three auxotrophic modifications, namely the deletions of URA3, LEU2 and HIS3. The genetics of the strain have been stabilized and can be used as a regular diploid or haploid yeast strain. EFSC2763 has been converted to a steviol glycoside producing yeast by genomic-integration of four DNA constructs. Each construct contains multiple genes that were introduced into the yeast genome by homologous recombination. Furthermore, construct one and two were assembled by homologous recombination.
The first construct contains eight genes and is inserted in the DPP1 locus and disrupts and partially deletes DPP1. The DNA inserted contains: the A. gossypii TEF promoter expressing the NatMX gene (selectable marker) followed by the TEF terminator from A. gossypii; Gene Art codon optimized S. rebaudiana UGT85C2 (SEQ ID NO: 32) expressed from the native yeast GPD1 promoter and followed by the native yeast CYC1 terminator; S. rebaudiana CPR-8 (SEQ ID NO: 24) expressed using the TPI1 promoter followed by the native yeast TDH1 terminator; A. thaliana Kaurene synthase (KS-5; SEQ ID NO: 96) expressed from the PDC1 promoter and followed by the native yeast FBA1 terminator; Synechococcus sp. GGPPS (GGPPS-7; SEQ ID NO: 97) expressed using the TEF2 promoter and followed by the native yeast PFI1 terminator; DNA2.0 codon-optimized S. rebaudiana KAHe1 (SEQ ID NO: 18), expressed from the TEF1 promoter and followed by the ENO2 terminator; S. rebaudiana KO-1 (SEQ ID NO: 98) expressed using the FBA1 promoter and followed by the native yeast TDH2 terminator; and Zea mays truncated CDPS (SEQ ID NO: 103) expressed using the PGK1 promoter and followed by the native yeast ADH2 terminator.
The second construct was inserted at the YPRCA15 locus and contains the native yeast TEF promoter from A. gossypii in front expressing the KanMX gene (selectable marker) followed by the TEF terminator from A. gossypii, the Gene Art codon optimized A. thaliana ATR2 (SEQ ID NO: 9) expressed from the PGK1 promoter followed by the yeast ADH2 terminator, S. rebaudiana UGT74G1 (SEQ ID NO: 100) expressed from the TPI1 promoter followed by the yeast TDH1 terminator, Gene Art codon-optimized S. rebaudiana UGT76G1 (SEQ ID NO: 101) expressed from the TEF1 promoter followed by the yeast ENO2 terminator, and GeneArt codon-optimized S. rebaudiana UGT91D2e-b (SEQ ID NO: 102) expressed from the GPD1 promoter and followed by the yeast CYC1 terminator.
The first and the second construct were combined in the same spore clone by mating and dissection. This yeast strain was subsequently transformed with construct three and four in two successive events.
Construct three was integrated between genes PRP5 and YBR238C and contained the TEF promoter from A. gossypii expressing the K. lactis LEU2 gene followed by the TEF terminator from A. gossypii, the GPD1 promoter expressing the DNA2.0-optimized S. rebaudiana KAHe1 (SEQ ID NO: 18) followed by the CYC1 terminator, and the TPI1 promoter expressing the Zea mays truncated CDPS (SEQ ID NO: 103).
Construct four was integrated in the genome between genes ECM3 and YOR093C with an expression cassette containing the TEF promoter from A. gossypii expressing the K. pneumoniae hph gene (SEQ ID NO: 157; see Gritz et al., (1983) Gene 25:179-88) followed by the TEF terminator from A. gossypii, Synechococcus sp. GGPPS expressed from the GPD1 promoter followed by the CYC1 terminator, and the TPI1 promoter expressing the A. thaliana Kaurene synthase. The four utilized genetic markers were subsequently removed.
As analyzed by LC-MS following the DMSO-extraction of total steviol glycosides from cells and broth, EFSC2763 produces between 40-50 μM or 2-3 μM/OD600 Rebaudioside A, after growth for four days in 3 ml SC (Synthetic Complete) media at 30° C. with 320 RPM shaking in deep-well plates.
C. Strain EFSC2797 was created from strain EFSC2763 by the addition of one more assembly construct at the YORW locus. The additional construct is as follows. The A. gossypii TEF promoter expressing the HIS gene (selectable marker) from S. pombe followed by the TEF terminator from A. gossypii; S. rebaudiana KO-1 (SEQ ID NO: 98) expressed using the GPD1 promoter and followed by the native yeast tCYC1 terminator; S. rebaudiana CPR-8 (SEQ ID NO: 24) expressed using the TPI1 promoter followed by the native yeast TDH1 terminator; A. thaliana Kaurene synthase (KS-5; SEQ ID NO: 96) expressed from the PDC1 promoter and followed by the native yeast FBA1 terminator; Oryza sativa EUGT11 (SEQ ID NO: 53) expressed from the TEF2 promoter followed by the yeast PGI1 terminator; DNA2.0 codon-optimized S. rebaudiana KAHe1 (SEQ ID NO: 18) expressed from the TEF1 promoter and followed by the ENO2 terminator; Zea mays truncated CDPS (SEQ ID NO: 103) expressed from the PGK1 promoter and followed by the ADH2 terminator.
LC-MS analysis following the DMSO-extraction of total steviol glycosides from cells (cells grown in 24-well plates for 4 days at 30° C.) and broth demonstrated that EFSC2797 produces varying amounts of RebA, RebB, RebD, RebM and Rubusoside, see Table 12 below.
D. EFSC3248 yeast strain was derived from the same parent wild type Saccharomyces cerevisiae strain described above and the following genes described in Table 13 were integrated using methods similar to the above. In addition this strain is HO— to prevent switching in mating types.
Yeast strains that produce Rebaudiosides are described in Example 2 above, and International Application No's.: PCT/US2011/038967 (WO/2011/153378) and PCT/US2012/050021 (WO/2013/022989) both incorporated by reference herein in their entirety. Observations from shake flask studies of similar strains indicated that the fraction of RebA in the supernatant increases with time, and the effect was determined not to be the result of cell lysis. To determine the effect of various transporters on steviol glycoside excretion in Saccharomyces cerevisiae, a library of Saccharomyces cerevisiae strains was constructed by substituting the TEF1 constitutive promoter for the endogenous promoter for a transporter gene.
A cassette was constructed consisting of the TEF promoter and the HIS5 (Schizosaccharomyces pombe) marker flanked by lox P sites. Primers with specific tails were used for PCR amplification of the cassette and the product was integrated upstream from the gene of interest by homologous recombination in the RebA producer EFC2763 described above. A Kosak sequence was added to the primer tails that anneal to the start of the gene so it was positioned just in front of the start codon. Correct insertion of the cassette was confirmed by PCR using a forward primer annealing to the TEF1 promoter and a gene specific reverse primer annealing to the specific transporter genes. Table 14 contains a list of 44 transport related genes where the TEF1 constitutive promoter was used to replace the endogenous promoter.
The 44 strains were tested for RebA excretion. Duplicate cultures were incubated in 3 ml synthetic complete (SC) medium for 48 hours (30° C., 310 rpm, 24 well plates). Supernatant samples were obtained by centrifugation of 100 μl of the culture (4000 rcf, 7 min). Twenty-five μl of the supernatant was added to the double amount of 50% DMSO.
These samples were analyzed by LC-MS as supernatant (cell-free) samples. The LC-MS method utilized was similar to Example 1 except a Phenomenex® kinetex C18 column (150×2.1 mm, 2.6 μm particles, 100 Å pore size) was utilized, and a more shallow gradient was employed from 40-50% B, resulting in typically longer retention times. The remaining supernatant from the original sample was removed and the pellet washed in 100 μl water. The pellet was resuspended in 100 μl 50% DMSO and heated to 80° C. for 10 minutes before the sample was centrifuged (4000 rcf, 5 min). Twenty-five μl of supernatant obtained from the resuspended pellet was added to an equal amount of 50% DMSO and an equal amount of water before transferring the sample to a filter plate. The samples were harvested from the filter plate (2000 rcf, 2 min) and measured on the LC-MS as pellet samples. Results are shown in
Strain “12_YOR1” showed a higher percentage of RebA in the supernatant than in the pellet as compared to the EFSC2763 control strain. The “18_ADP1” and the “EFSC2763” strains produced less RebA in total than the other strains and “40_THI7” had a large deviation between samples. The YOR1 overexpressing strain was tested again. In the second experiment, the YOR1 overexpressing strain “YOR1_OE” produced less total RebA than the EFSC2763 control strain, but still showed a higher percentage of RebA in the supernatant than the control strain (
Nine candidates (PDR1, PDR3, PDR13, SNQ2, YOR1_BY, YOR1_IS1, FLR1, AZR1 and DTR1) were re-tested for rebaudioside production and excretion in another producing strain, EFSC2797 (described above), and on a 2 micron plasmid (PSB314). Duplicate cultures were incubated in 3 ml synthetic complete (SC) medium for 48 hours (30° C., 310 rpm, 24 well plates). Supernatant samples were obtained by centrifugation of 100 μl of the culture (13,000 rcf, 5 min). Fifty microliters of the supernatant was added to an equal amount of 100% DMSO. These samples were analyzed by LC-MS as supernatant samples. A total broth sample was mixed with an equal volume of 100% DMSO and heated to 80° C. for 10 minutes before the sample was centrifuged (4000 rcf, 5 min), and the liquid portion was analyzed by LC-MS as “total” steviol glycoside levels. The amount of various steviol glycosides (including RebA, RebB, RebD, RebM, Rubusoside, 13-SMG, 1.2 Stevioside, 1.2 Bioside and an unknown steviol glycoside (LC-MS peak at 4.13 min.)) excreted into the culture supernatant as well as the total amount in the whole culture broth were measured by LC-MS as described in Example 1. Results are seen in
Independent overexpression of each nine candidate genes (PDR1, PDR3, PDR13, SNQ2, YOR1_BY, YOR1_IS1, FLR1, AZR1 and DTR1) demonstrated that various steviol glycosides were excreted at a higher percentage and/or concentration in the supernatant compared to the control strain (the control is EFSC2797 with empty PSB314 plasmid; shown as “PSB314” in
Four of the nine candidates above were tested again for rebaudioside production and excretion in the producing EFSC2797 strain, and using the PSB3142 micron plasmid to overexpress the transporters. Cultures were incubated in 3 ml synthetic complete (SC) medium—URA (selection pressure) for 72 hours (30° C., 310 rpm, 24 well plates). Supernatant samples were obtained by centrifugation of 100 μl of the culture (13,000 rcf, 5 min). Fifty microliters of the supernatant was added to 50 ul of 100% DMSO. These samples were anaylzed by LC-MS as supernatant samples. 50 μl of cell suspension were mixed with 50 μl of 100% DMSO and heated to 80° C. for 10 minutes before the sample was centrifuged (4000 rcf, 5 min); the liquid portion was measured on the LC-MS as “total” samples. The amount of various steviol glycosides (including RebA, RebB, RebD, RebM, Rubusoside, 13-SMG, 1.2 Stevioside, 1.2 Bioside and an unknown steviol glycoside (LC-MS peak at 4.13 min.)) excreted into the culture supernatant as well as the total amount in the whole culture broth were measured by LC-MS as described in Example 1. The area under the curve (AUC) is determined by integration during data processing using Xcalibur software (Thermo). Results showing amount excreted (AUC) are seen in
Overexpression of each the four candidate genes separately (PDR1, SNQ2, YOR1_BY, YOR1_IS1 and FLR1) demonstrated that various steviol glycosides were excreted at a higher percentage and/or concentration in the supernatant compared to the control strain (EFSC2797 with empty PSB314 plasmid; shown as “PSB314” in
Six putative S. rebaudiana RebA transporters were identified in pyrosequencing data: SrDTX24 (SEQ ID NO: 150), SrMRP10 (SEQ ID NO: 151), SrPDR12 (SEQ ID NO: 152), SrMRP2 (SEQ ID NO: 153), SrMRP4a (SEQ ID NO: 154), and SrMRP4b (SEQ ID NO: 155). Five of the putative transporters, SrDTX24, SrMRP10, SrPDR12, SrMRP4a and SrMRP4b, were chosen for further study and cloned. The cloned transporter sequences were expressed in a stable RebA-producing S. cerevisiae. The levels of steviol-glycoside excretion were measured and are shown in
Yeast strains that produce Rebaudiosides are described in Example 2 above, and International Application No's.: PCT/US2011/038967 (WO/2011/153378) and PCT/US2012/050021 (WO/2013/022989) both incorporated by reference herein in their entirety. Observations from shake flask studies of similar strains indicated that steviol glycosides were excreted from S. cerevisiae cells with an efficiency that appeared to decrease as the molecular weight of the molecule increased. To determine the effect of various transporters on steviol glycoside excretion in S. cerevisiae, a library of S. cerevisiae mutants, each carrying a disruption in an endogenous transporter, was constructed.
Plasma membrane-located ABC and MFS transporters were singly disrupted in S. cerevisiae strains BY4741 and/or BY4742 (BY4741 is available as ATCC 201388, and BY4742 is available as ATCC 201389; see Brachmann, et al. “Designer deletion strains derived from Saccharomyces cerevisiae S288C: a useful set of strains and plasmids for PCR-mediated gene disruption and other applications.” Yeast 14:115-32, 1998), using an antibiotic marker cassette amplified with primers having 45-65 bp gene specific long-tails. The cassettes were transformed into the strains and specific transporter genes were disrupted by homologous recombination of the antibiotic marker cassette. Disruption of native transporter genes was confirmed by PCR, using a forward primer specific to the upstream sequence of the native gene and a reverse primer located internally in the antibiotic marker cassette. The mutant library encompassed a total of 34 transporters (14 ABCs, 19 MFSs, and 1 other) and two transcription factors. See Table 15.
The initial analysis showed that among the mutants of these 36 genes, transporters encoded by the yeast PDR5, PDR10, PDR15 and SNQ2 loci had a detectable effect on excretion of steviol glycosides such as 19-SMG and rubusoside into the culture media. Yeast endogenous transporters encoded by the TPO1, TPO3, YOR1, YOL075c, PDR18, and FLR1 loci, as well as the transcription factors encoded by the PDR1 and PDR3 loci, also had a detectable effect on steviol glycoside excretion, although to a lesser extent than that of PDR5, PDR10, PDR15 and SNQ2. Since several transporters were identified that affected excretion of steviol glycosides, no single transporter appears to be solely responsible for excretion of steviol glycosides in yeast.
To determine the effect of disruptions of more than one transporter on steviol glycoside excretion, a quadruple disruption mutant (pdr5, pdr10, pdr15, snq2) was created. Deletion mutant pdr15 (created in a S. cerevisiae strain based on BY4742) was transformed with a selection marker deletion cassette prepared from a PCR using primers with PDR10 flanking sequences as tails, allowing homologous recombination upon transformation. In the same way, a snq2 deletion strain was created (based on BY4741) and was transformed with a second selection marker deletion cassette using PDR5 flanking sequences as primer tails. The resulting two double mutant strains (pdr15-pdr10 and snq2-pdr5) were mated to create spore products disrupted in all four transporter genes. Disruptions were verified by PCR using a primer strategy as described for the single disruption mutants, resulting in the formation of a quadruple pdr5, pdr10, pdr15, snq2 disruption mutant, referred to as the 4× disruption mutant.
The 4× disruption mutant was transformed with 2 micron plasmids encoding four Stevia rebaudiana UGTs: 76G1, 74G1, 91D2e, and 85C2. See WO 2011/153378A1. A culture of the 4× disruption mutant expressing the four UGTs was pre-grown overnight in 13-ml culture tubes containing 2-3 ml of synthetic complete (SC) medium lacking histidine and uracil. A culture of the parent strain with the UGT plasmids, but wild type at the PDR5, PDR10, PDR15, SNG2 loci, served as the control.
The next day, 0.25 OD600 units were spun down, resuspended in fresh medium containing 100 μM steviol, and shaken at 30° C. for 2 h in culture tubes. An aliquot of 100 μL of culture was spun down, and an equal volume of DMSO was added to the supernatant. The cell pellet was washed with H2O and subsequently resuspended in 200 μL of 50% DMSO. The mixture was then vortexed, heated at 80° C. for 10 minutes and centrifuged to remove debris. The resulting solution (cell pellet sample) was analyzed for the amount of 19-SMG by LC-MS utilizing a method similar to that described in Example 1, except a Phenomenex® kinetex C18 column (150×2.1 mm, 2.6 μm particles, 100 Å pore size) was used, and a more shallow gradient was employed from 40-50% B, resulting in typically longer retention times. The results, shown in
The 4× disruption mutant strain expressing the four S. rebaudiana UGTs was tested for Rebaudioside A production. Pre-cultured cells were concentrated to an OD600=20 in 250 μl steviol containing medium (SC-His-Ura, 100 μM steviol). After a 24 hour incubation (at 30° C. and 200 rpm), the cells were harvested. A 100 μL aliquot of the culture was spun down and an equal volume of DMSO was added to the supernatant of this sample. The cell pellet was washed one time in H2O and 200 μL of 50% DMSO was added to the pellet. Samples were vortexed, heated to 80° C. for 10 minutes and centrifuged. The supernatants from two DMSO mixtures were pooled and steviol glycoside content analyzed by LC-MS utilizing a Phenomenex® kinetex C18 column. The results are shown in
Based on the quadruple transporter mutant results described above, a 7× transporter disruption mutant (pdr15-pdr10-snq2-pdr5-tpo1-pdr1-pdr3) was generated. A pdr1 and pdr3 double mutant was created in a BY4741 background. The markers used to generate the double mutant were then removed. The resulting double mutant was transformed with a selection marker deletion cassette. The cassette was prepared from PCR using primers with TPO1 flanking sequences as tails allowing homologous recombination upon transformation. The triple mutant pdr1-pdr3-tpo1 was mated with the 4× disruption mutant described above (based on BY4742). In the resulting spores, a strain disrupted in all seven locations was found. Disruption of genes was confirmed by PCR. In the case of cassettes replacing targeted genes, the PCR strategy described above was applied to confirm disruption of genes. For the pdr1 and pdr3 loci, disruptions were confirmed using forward and reverse primers designed to anneal to the sequence upstream and downstream from each gene. PCR products were present in all clones, and short PCR products indicated a loss of the targeted gene.
The four S. rebaudiana UGTs described above were integrated into the genome of the 4× and 7× transporter disruption mutants as well as the wild-type strain, using homologous recombination. A steviol-gradient, time-course experiment was performed to investigate the effect on steviol-glycoside accumulation in the wild-type, 4×, and 7× mutant strains. Pre-cultured cells of the 4× and 7× disruption mutant strains, each expressing the four S. rebaudiana UGTs, were concentrated to an OD600=1 in 400 μl steviol containing medium (SC-Ura, 0 μM, 20 μM, 50 μM, 100 μM, or 250 μM steviol). Strains were grown in a 96 deep well plate at 30° C., 320 rpm, and after approximately 0, 1, 2, 4, 8 or 24 hours of culture, a 50 μL aliquot of each culture was spun down and an equal volume of DMSO was added to the supernatant of each aliquot. Steviol glycoside content was analyzed by LC-MS as described above, with the Phenomenex® kinetex C18 column.
The results are shown in
The above data illustrate that knockouts of endogenous transporters in yeast singly or in combination and screening for increased retention of steviol glycosides, is a good method for identifying potential transporters for overexpression to improve steviol glycoside excretion in the medium.
Further Screening of Transporter MutantsThe effect of yeast gene knockouts on excretion of higher molecular weight rebaudiosides was tested in yeast strain EFSC3248, described in Example 2. Disruption of each specific transporter gene (PDR5, SNQ2, YOR1, YHK8 and FLR1) on the chromosome was performed by homologous recombination as described previously. After a 96 hour incubation (at 30° C. and 200 rpm), cells were harvested. A 100 μL aliquot of the culture was spun down and an equal volume of 100% DMSO was added to the supernatant. Eighty microliters of the mixture were analyzed by LC-MS as ‘supernatant’ sample. One-hundred microliters of cell suspension in 100 uL of 100% DMSO was heated at 80° C. for 10 minutes and then centrifuged. The mixture was vortexed, heated at 80° C. for 10 minutes, and centrifuged to remove any remaining debris. Forty microliters of the resulting solution was mixed with 40 uL DMSO (50%) and samples were analyzed by LC-MS as ‘total’ sample. The amount of various steviol glycosides (including RebA, RebB, RebD, RebM, Rubusoside, 13-SMG, 1.2 Stevioside, 1.2 Bioside and an unknown steviol glycoside (LC-MS peak at 4.13 min.)) excreted into the culture supernatant, as well as the total amount in the whole culture broth were measured by LC-MS as described in Example 1. The data demonstrate that disruption of single endogenous yeast transporter genes results in the decrease in the percentage (
Having described the invention in detail and by reference to specific embodiments thereof, it will be apparent that modifications and variations are possible without departing from the scope of the invention defined in the appended claims. More specifically, although some aspects of the present invention are identified herein as particularly advantageous, it is contemplated that the present invention is not necessarily limited to these particular aspects of the invention.
Claims
1. A recombinant microorganism capable of producing a steviol glycoside in a cell culture,
- wherein the microorganism has a modified expression of at least one endogenous transporter gene and at least one endogenous transcription factor gene that regulates expression of the at least one endogenous transporter gene,
- wherein the modified expression comprises reduced expression or activity of the at least one endogenous transporter gene, having at least 80% sequence identity to the amino acid sequence set forth in SEQ ID NO:113;
- wherein the reduced expression is produced in the microorganism by disrupting or deleting the gene locus for the at least one endogenous transporter gene;
- wherein the microorganism further expresses at least one heterologous transporter gene;
- wherein the steviol glycoside is Rebaudioside A, Rebaudioside B, Rebaudioside D, Rebaudioside E, Rebaudioside M, or an isomer thereof.
2. The recombinant microorganism of claim 1, wherein the endogenous and/or the heterologous transporter gene encodes an ATP-Binding Cassette (ABC) transporter.
3. The recombinant microorganism of claim 1, wherein the heterologous transporter gene is a Stevia transporter gene.
4. The recombinant microorganism of claim 1, further comprising a gene encoding a polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside; wherein the gene has a copy number of 2 or more; and wherein the polypeptide comprises a polypeptide having at least 90% sequence identity to one of the amino acid sequences set forth in any one of SEQ ID NOs:51, 54, 55, 86, or 90.
5. The recombinant microorganism of claim 4, wherein the gene is codon optimized for expression in the microorganism.
6. The recombinant microorganism of claim 5, wherein the gene is codon optimized for expression in Saccharomyces cerevisiae.
7. The recombinant microorganism of claim 1, wherein the recombinant microorganism is a yeast cell from Saccharomyces.
8. A method of affecting excretion of a steviol glycoside from a cell culture, comprising culturing the recombinant microorganism of claim 1 under conditions in which the genes are expressed;
- wherein the steviol glycoside is produced by the recombinant microorganism.
9. A method of producing a steviol glycoside in a cell culture, comprising culturing the recombinant microorganism of claim 1 under conditions in which the at least one endogenous transporter gene, the at least one endogenous transcription factor gene that regulates expression of the at least one endogenous transporter gene, or both are expressed; wherein the steviol glycoside is produced by the recombinant microorganism.
10. The method of claim 9, wherein culturing includes inducing expression of the at least one endogenous transporter gene, the at least one endogenous transcription factor gene that regulates expression of the at least one endogenous transporter gene, or both.
11. The method of claim 9, wherein culturing includes constitutively expressing the at least one endogenous transporter gene, the at least one endogenous transcription factor gene that regulates expression of the at least one endogenous transporter gene, or both.
12. The method of claim 9, wherein:
- (a) Rebaudioside A is synthesized in the recombinant microorganism expressing a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-13 hydroxyl group; a polypeptide capable of beta 1,3 glycosylation of the C3′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside; a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-19 carboxyl group; and a polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside;
- (b) Rebaudioside B is synthesized in the recombinant microorganism expressing a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-13 hydroxyl group; a polypeptide capable of beta 1,3 glycosylation of the C3′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside; and polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside;
- (c) Rebaudioside D is synthesized in the recombinant microorganism expressing a polypeptide capable of glycosylating steviol or the steviol glycoside at its C-13 hydroxyl group; a polypeptide capable of beta 1,3 glycosylation of the C3′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside; a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-19 carboxyl group; and a polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside;
- (d) Rebaudioside E is synthesized in the recombinant microorganism expressing a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-13 hydroxyl group; a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-19 carboxyl group; and a polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside; and/or
- (e) Rebaudioside M is synthesized in the recombinant microorganism expressing a polypeptide capable of glycosylation of the 13-OH of steviol; a polypeptide capable of beta 1,3 glycosylation of the C3′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside; a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-19 carboxyl group; and a polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside.
13. The method of claim 9, wherein Rebaudioside A is synthesized in the recombinant microorganism expressing a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-13 hydroxyl group; a polypeptide capable of beta 1,3 glycosylation of the C3′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-0-glucose of a steviol glycoside; a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-19 carboxyl group; and a polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside.
14. The method of claim 9, wherein Rebaudioside D is synthesized in the recombinant microorganism expressing a polypeptide capable of glycosylating steviol or the steviol glycoside at its C-13 hydroxyl group; a polypeptide capable of beta 1,3 glycosylation of the C3′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-0-glucose of a steviol glycoside; a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-19 carboxyl group; and a polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside.
15. The method of claim 10, wherein Rebaudioside M is synthesized in the recombinant microorganism expressing a polypeptide capable of glycosylation of the 13-OH of steviol; a polypeptide capable of beta 1,3 glycosylation of the C3′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside; a polypeptide capable of glycosylating steviol or a steviol glycoside at its C-19 carboxyl group; and a polypeptide capable of beta 1,2 glycosylation of the C2′ of the 13-O-glucose, 19-O-glucose, or both 13-O-glucose and 19-O-glucose of a steviol glycoside.
16. The method of claim 9, wherein steviol glycoside is produced at a concentration of at least 500 mg/L of cell culture.
17. The method of claim 15, that further comprises isolating the Rebaudioside M, alone or together with at least one other steviol glycoside from the cell culture.
18. The method of claim 17, wherein the isolating step comprises separating a liquid phase of the cell culture from a solid phase of the cell culture to obtain a supernatant comprising Rebaudioside M, alone or together with at least one other steviol glycoside, and:
- (a) contacting the supernatant with one or more adsorbent resins in order to obtain at least a portion of Rebaudioside M, alone or together with at least one other steviol glycoside; or
- (b) contacting the supernatant with one or more ion exchange or reversed-phase chromatography columns in order to obtain at least a portion of Rebaudioside M, alone or together with at least one other steviol glycoside; or
- (c) crystallizing or extracting Rebaudioside M, alone or together with at least one other steviol glycoside;
- thereby isolating Rebaudioside M, alone or together with at least one other steviol glycoside.
19. The method of claim 9, that further comprises recovering a steviol glycoside composition comprising Rebaudioside M, alone or together with at least one other steviol glycoside from the cell culture.
20. The method of claim 19, wherein the recovered steviol glycoside composition is enriched for Rebaudioside M relative to a steviol glycoside composition of Stevia plant and has a reduced level of Stevia plant-derived components relative to a steviol glycoside composition obtained from a plant-derived Stevia extract.
21. The method of claim 9, wherein the recombinant microorganism is grown in a fermentor at a temperature for a period of time, wherein the temperature and the period of time facilitate the production of the steviol glycoside composition.
22. A cell culture, comprising the recombinant microorganism of claim 1, the cell culture further comprising:
- (a) the steviol glycoside produced by the recombinant microorganism;
- (b) glucose, fructose, sucrose, xylose, rhamnose, uridine diphosphate (UDP)-glucose, UDP-rhamnose, UDP-xylose, and/or N-acetyl-glucosamine; and
- (c) supplemental nutrients comprising trace metals, vitamins, salts, YNB, and/or amino acids;
- wherein the steviol glycoside is present at a concentration of at least 1 mg/liter of the cell culture.
23. The recombinant microorganism of claim 1, wherein the recombinant microorganism is a plant cell, a mammalian cell, an insect cell, a fungal cell from Aspergillus genus, or a yeast cell from Saccharomyces cerevisiae, Schizosaccharomyces pombe, Yarrowia lipolytica, Candida glabrata, Ashbya gossypii, Cyberlindnera jadinii, Pichia pastoris, Kluyveromyces lactis, Hansenula polymorpha, Candida boidinii, Arxula adeninivorans, Xanthophyllomyces dendrorhous, or Candida albicans species, an algal cell or a bacterial cell from Escherichia coli species, or Bacillus genus.
24. A steviol glycoside produced by the recombinant microorganism of claim 1.
25. A sweetener composition, comprising the steviol glycoside of claim 24.
26. A food product, comprising the sweetener composition of claim 25.
27. A beverage or a beverage concentrate, comprising the sweetener composition of claim 25.
Type: Application
Filed: Apr 29, 2021
Publication Date: Jan 20, 2022
Inventors: Ernesto Simon (Glostrup), Iben Nordmark Anderson (Vedbaek), Michael Dalgaard Mikkelsen (Vaerløse), Jorgen Hansen (Frederiksberg), Veronique Douchin (Copenhagen)
Application Number: 17/244,089
