ATTENUATED LIVE BACTERIA WITH INCREASED ACID RESISTANCE AND METHODS OF USE THEREOF

The present invention relates to inducing acid resistance in a bacterium and methods of increasing the acid resistance of an acid sensitive bacterium.

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Description
CROSS REFERENCE TO RELATED APPLICATIONS

This application claims the priority of U.S. provisional application No. 61/836,140, filed Jun. 17, 2013, which is hereby incorporated by reference in its entirety.

GOVERNMENTAL RIGHTS

This invention was made with government support under 1R21A1092307 awarded by the National Institutes of Health. The government has certain rights in the invention.

FIELD OF THE INVENTION

The present invention relates to inducing acid resistance in a bacterium and methods of increasing the acid resistance of an acid sensitive bacterium.

BACKGROUND OF THE INVENTION

In order to reach their intestinal habitat, enteric microbes must first survive the formidable low pH environment of the stomach, making an acid-coping strategy imperative. Wild-type Salmonella enterica serotypes have multiple ways to resist low pH. First, the acid tolerance response (ATR) upregulates acid shock proteins to temporarily prevent cellular damage. Second, the acid resistance systems (AR) consume protons to raise the intracellular pH. AR1 system is regulated by Crp and is poorly understood. The remaining systems, AR3, AR4 and AR5 (AR2 is not present in Salmonella) rely on arginine, lysine and ornithine decarboxylases, respectively. However, AR3-5 are typically repressed under standard laboratory growth conditions, and the ATR in many live attenuated Salmonella vaccines is impaired, making gastric transit challenging for these strains. In addition, many means used to attenuate Salmonella for virulence have a secondary effect of increasing sensitivity to acid, thereby increasing the effective dose required for immunogenicity. As a result, oral Salmonella vaccines are typically given with an agent designed to increase the gastric pH, such as bicarbonate. While this approach is helpful, it precludes the Salmonella vaccine from sensing important environmental signals (i.e. low pH) that optimize its ability to effectively interact with host tissues. This results in reduced immunogenicity as a vaccine.

SUMMARY OF THE INVENTION

In an aspect, the invention encompasses a recombinant attenuated derivative of a pathogenic enteric bacterium comprising at least one of the following: a regulatable promoter operably linked to a nucleic acid encoding an arginine decarboxylase and a nucleic acid encoding an arginine agmatine antiporter; a regulatable promoter operably linked to a nucleic acid encoding a glutamate decarboxylase and a nucleic acid encoding a glutamate/γ-aminobutyric acid antiporter; or a regulatable promoter operably linked to a nucleic acid encoding a lysine decarboxylase and a nucleic acid encoding a lysine/cadaverine antiporter.

In another aspect, the invention encompasses a method for increasing the acid resistance of an acid sensitive bacterium, the method comprising introducing into the acid sensitive bacterium a cassette comprising at least one of the following: a regulatable promoter operably linked to a nucleic acid encoding an arginine decarboxylase and a nucleic acid encoding an arginine agmatine antiporter; a regulatable promoter operably linked to a nucleic acid encoding a glutamate decarboxylase and a nucleic acid encoding a glutamate/γ-aminobutyric acid antiporter; or a regulatable promoter operably linked to a nucleic acid encoding a lysine decarboxylase and a nucleic acid encoding a lysine/cadaverine antiporter, such that in the absence of induction of the regulatable promoter, the recombinant bacterium is acid sensitive, but upon induction of the regulatable promoter, the recombinant bacterium displays an increase in acid resistance.

A recombinant Salmonella bacterium, the bacterium comprising a regulatable promoter operably linked to at least one nucleic acid selected from the group consisting of adiA and adiC; gadB and gadC; and cadB and cadA.

BRIEF DESCRIPTION OF THE FIGURES

The application file contains at least one drawing executed in color. Copies of this patent application publication with color drawing(s) will be provided by the Office upon request and payment of the necessary fee.

The following drawings form part of the present specification and are included to further demonstrate certain aspects of the present invention. The invention may be better understood by reference to one or more of these drawings in combination with the detailed description of specific embodiments presented herein.

FIG. 1. Schematic diagram of arginine decarboxylase mutations. The genes and associated regulatory sequences for the Δ(adiA-adiC), ΔPadiA::TT araC ParaBAD adiA, ΔPadiA:TT rhaSR PrhaBAD adiA, and Δ(PadiY-adiY-PadiC) adiC mutations are shown above, along with the archetypal strain number. The wild-type arginine decarboxylase locus (adi) of S. Typhi Ty2 is depicted for comparative purposes. The diagram is approximately to scale. () promoter; () transcription terminator.

FIG. 2. Regulation of adiA by the araC ParaBAD and rhaSR PrhaBAD promoters. χ11552 (ΔaroD ParaBAD adiA) and χ11564 (ΔaroD PrhaBAD adiA) were cultured in the presence of varying concentrations of arabinose or rhamnose (ranging from 10−1-10−5%), normalized and (A) assayed by semi-quantitative PCR for the level of adiA transcript, (B) probed for the presence of AdiA by western blot or (C) tested for arginine decarboxylase activity via colorimetric assay. mRNA data are plotted as the mean and SEM of three independent experiments. Western blot and enzyme assay data are representative of three independent assays. In the colorimetric arginine decarboxylase assay, a dark blue color is indicative of the presence of AdiA.

FIG. 3. Co-regulation of adiA and adiC by rhamnose is required for survival during pH 3 challenge. χ11564 (ΔaroD PrhaBAD adiA), χ11568 (ΔaroD PrhaBAD adiAC) and χ11636 (ΔaroD adiAC) were grown to stationary phase in EG medium in the presence of 0.1% rhamnose, then challenged with pH 3.0 EG medium containing 1 mM arginine. Survival was monitored by plating on LB agar containing all necessary supplements. Data shown are the mean and SEM of three independent assays.

FIG. 4. Acid resistance depends on the presence of rhamnose and arginine. Ty2, χ11548 (ΔaroD) and χ11568 (ΔaroD P rhaBAD adiAC) were grown to stationary phase in EG medium, then challenged with EG medium, pH 3.0. (A) Strains cultured in the presence or absence of 0.1% rhamnose. (B) Strains challenged in the presence or absence of 1 mM arginine. Survival in all assays was monitored by plating on LB agar containing all necessary supplements. Data shown are the mean and SEM of three independent assays.

FIG. 5. Acid resistance of an ΔaroD mutant containing rhamnose-regulated arginine decarboxylase at pH 2.5. Ty2, χ11500 (ΔadiA-adiC), χ11548 (ΔaroD) and χ11568 (ΔaroD PrhaBAD adiAC) were grown to stationary phase in EG medium containing 0.1% rhamnose, then challenged with EG medium containing 1 mM arginine at pH 2.5 for 1 hour. Survival in all assays was monitored by plating on LB agar containing all necessary supplements. Data shown are the mean and SEM of three independent assays. Pairs of data marked with an asterisk (*) are significantly different (p<0.05).

FIG. 6. Acid resistance of a ΔphoPQ mutant containing rhamnose-regulated arginine decarboxylase. Ty2, χ11500 (ΔadiA-adiC), χ8444 (ΔphoPQ) and χ11622 (ΔphoPQ PrhaBAD adiAC) were grown to stationary phase in EG medium containing 0.1% rhamnose, then challenged with EG medium containing 1 mM arginine at (A) pH 3.0 for 4 hours or (B) pH 2.5 for 1 hour. Survival in all assays was monitored by plating on LB agar containing all necessary supplements. Data shown are the mean and SEM of three independent assays. Pairs of data marked with an asterisk (*) are significantly different (p<0.05).

FIG. 7. Acid resistance of a ΔPfur::TT araC ParaBAD fur mutant containing rhamnose-regulated arginine decarboxylase. (A) Strains were grown overnight in purple broth ±0.2% arabinose, then probed for the presence of Fur by western blot. (B) χ11118 was grown to stationary phase in EG medium ±0.2% arabinose, then challenged with EG medium containing 1 mM arginine at pH 3.0 for 4 hours. Arginine decarboxylase rescue was performed by growing strains in EG medium to stationary phase in the absence of arabinose and presence of 0.1% rhamnose and challenging with EG medium containing 1 mM arginine at (C) pH 3.0 for 4 hours or (D) pH 2.5 for 1 hour. Survival in all assays was monitored by plating on LB agar containing all necessary supplements. Data shown are the mean and SEM of three independent assays. Pairs of data marked with an asterisk (*) are significantly different (p<0.05). χ11500=ΔadiA-adiC; χ11118=ParaBAD fur; χ11623=ParaBAD fur PrhaBAD adiAC; χ11742=Δfur

FIG. 8. Comparison of acid resistance provided by native and rhamnose-regulated arginine decarboxylase. Strains containing (A, B) ΔaroD (C, D) ΔphoPQ or (E, F) ΔPfur::TT araC ParaBAD fur attenuating mutations were grown overnight in TSB medium with 0.4% glucose and 0.1% rhamnose under anaerobic conditions. For χ11623, 0.4% rhamnose was supplied. Cells were challenged with EG medium containing 1 mM arginine, pH 3.0 (A, C, E) or pH 2.5 (B, D, F). Survival in all assays was monitored by plating on LB agar containing all necessary supplements. Data shown are the mean and SEM of three independent assays. 11500=ΔadiA-adiC; 11548=ΔaroD; 11568=ΔaroD PrhaBAD adiAC; 8444=ΔphoPQ; 11622=ΔphoPQ P rhaBAD adiAC; 11118=ParaBAD fur; 11623=ParaBAD fur PrhaBAD adiAC.

FIG. 9. Schematic diagram of glutamate decarboxylase constructions. The genes and associated regulatory sequences for the ΔcysG and ΔcysG::TT araC PBAD gadBC mutations are shown above along with the hypothetical sequence mutations ΔaraE and ΔaraE::TT araC PBAD gadA. The wild-type cysG and araE loci of S. Typhi Ty2 are depicted for comparative purposes. The diagram is approximately to scale. () promoter; () transcription terminator.

FIG. 10. Survival of S. Typhi strains during in vitro low pH challenge. Strains were grown to stationary phase in EGA medium, pH 7.0 containing arabinose with aeration, then washed and challenged in EG medium containing 1 mM glutamic acid. ΔguaBA, ΔphoPQ, and Δfur mutants were challenged at pH 3.0 (A) or pH 2.5 (B) for 1 h. Data are presented as the mean and SEM for each time point.

FIG. 11. Gastric pH following histamine injection. Following a 6 hour fast, mice were injected subcutaneously with 10 mg/kg histamine. Mice were anaesthetized with pentobarbital prior to gastric surgery. Gastric pH was measured at the mucosal surface of the stomach for up to 4 hours post histamine injection. Data shown are the mean and standard deviation of at least five mice per time point.

FIG. 12. Survival of strains cultured under non-acid resistance inducing conditions. Wild-type enteric strains were grown in LB medium to late log phase under aerobic conditions. (A) Cells were washed and challenged in EG medium (pH 3.0) containing 0.1% casamino acids. Survival during EG medium challenge was assayed hourly for 4 hours by plating onto LB agar. Data shown are the mean and SEM of three independent experiments. (B) Cells were washed and then resuspended in PBS containing 0.1% casamino acids. Mice were either fasted for 6 hours (fasted mouse model) or fasted and low gastric pH was induced by histamine injection (acid mouse model) and then inoculated with 109 CFU of each strain. Cells contained the pWSK129 plasmid (KanR) to enhance recovery from intestinal tissues. Sixty minutes after inoculation, mice were euthanized and the entire small intestine removed and homogenized. Survival was assayed by plating onto LB agar containing kanamycin. Data are expressed as the percent of initial inoculum recovered (% survival). The geometric mean and 95% confidence interval of two independent experiments (8 mice total) is depicted.

FIG. 13. Effect of arginine decarboxylase on the gastric survival of S. Typhi. Pairs of attenuated S. Typhi strains differing only in their arginine decarboxylase locus were grown to stationary phase in EGA medium under aerobic conditions. Cells were combined in a 1:1 ratio in PBS containing 1 mM arginine. Low gastric pH was induced by histamine injection in mice fasted for 6 h. Mice were inoculated with 109 CFU of each strain. Sixty min after inoculation, mice were euthanized and the entire small intestine removed and homogenized. Strain survival was assayed by plating onto LB agar containing kanamycin or streptomycin. Data shown are the competitive index of the two strains in each mouse with the geometric mean of two independent experiments (10 mice total) indicated as a solid line.

FIG. 14. Effect of glutamate decarboxylase on the gastric survival of S. Typhi. Pairs of attenuated S. Typhi strains differing only in their glutamate decarboxylase locus were grown to stationary phase in EGA medium under aerobic conditions. Cells were combined in a 1:1 ratio in PBS containing 1 mM glutamic acid. Low gastric pH was induced by histamine injection in mice fasted for 6 h. Mice were inoculated with 109 CFU of each strain. Sixty min after inoculation, mice were euthanized and the entire small intestine removed and homogenized. Strain survival was assayed by plating onto LB agar containing kanamycin or streptomycin. Data shown are the competitive index of the two strains in each mouse with the geometric mean of two independent experiments (10 mice total) indicated as a solid line.

FIG. 15. Survival of S. Gallinarum strains during low pH challenge. Mid-log aerobic cultures grown in LB broth were harvested, washed and challenged with E medium at pH 3.0. Samples were taken and numbers of surviving cells were determined by direct plating onto LB plates. Data are presented as the mean and SEM for each time point.

FIG. 16. Rescue of acid sensitive S. Gallinarum strains by arabinose-inducible gadBC system. Cultures were grown aerobically in LB broth to an optical density at 600 nm of 0.4. Cells were harvested, washed and challenged with E medium at pH 3.0 for one hour. Numbers of surviving cells were determined by direct plating onto LB plates. Data are presented as the mean and SEM for each time point.

FIG. 17. Survival of RASV strains during low pH gastric transit. Histamine-treated mice were inoculated orally with 109 CFU of (A) χ9633(pYA4088, pWSK129), (B) χ9639(pYA4088, pWSK129), (C) χ9640(pYA4088, pWSK129) or (D) χ9558(pYA4088, pWSK129). Mice received either 1.3% sodium bicarbonate, chocolate Ensure or nothing prior to and immediately following immunization to neutralize gastric acid. The number of viable vaccine cells in the small intestine was quantified one hour after immunization. Data are presented as the number of CFU/g intestine of individual mice, with the geometric mean of the group displayed as a solid horizontal line. Groups that exhibited a significant increase (p<0.05) in the number of viable vaccine cells in the small intestine over the control group are marked with an asterisk (*). Data are the combined results of two independent experiments (8 mice total).

 DETAILED DESCRIPTION

The present invention encompasses a bacterium with increased acid resistance, methods of increasing the acid resistance of a bacterium, and methods of use thereof. The invention also encompasses vaccine compositions comprised of a bacterium exhibiting an increase in acid resistance. Advantageously, a bacterium with an increase in acid resistance of the invention may be administered orally to a subject and substantially survive the low pH of the subject's stomach, while exposure to the low pH environment stimulates up-regulation of invasion and/or virulence related nucleic acid sequences.

I. Recombinant Attenuated Bacterium

A recombinant bacterium of the invention is typically a bacterial enteric pathogen, and belongs to a species or strain commonly used for a vaccine.

Enteric pathogenic bacteria are agents of intestinal disease typically acquired through ingestion. These pathogens include, but are not limited to, bacteria of the family Enterobacteriaceae, such as Salmonella species, Shigella species, Yersinia species (e.g. Y. pseudotuberculosis and Y. enterocolitica), certain pathovars of Escherichia coli, including enterotoxigenic E. coli (ETEC), enterohaemorrhagic E. coli (EHEC), enteropathogenic E. coli (EPEC) and extraintestinal E. coli (ExPEC). Other enteric pathogens include Vibrio species (e.g. V. cholerae) and the gram-positive bacterium Listeria monocytogenes.

To be safe for use as a vaccine, the bacterial enteric pathogen must be attenuated for virulence by deletion or regulated expression of a virulence gene. In the case of Salmonella, for instance, the following genes may be altered to achieve attenuation: pab, aroA, aroC, aroD, asdA, dapA, dam, murA, nadA, pncB, galE, pmi, fur, ompR, htrA, hemA, cdt, cya, crp, phoP, phoQ, rfc, rfaH, poxA, galU, guaB, guaA, hfq, msbB or genes required for the function of type 3 secretion systems in pathogenicity island 2, such as ssaV, or an effector molecule secreted by the type 3 secretion system, such as sopB. The genes may be deleted or a regulatable promoter may be inserted in front of the gene to achieve regulated delayed attenuation. As used herein, “regulated delayed attenuation” refers to the ability of the microbe to colonize a host and then display an attenuation phenotype to avoid actually causing a symptomatic infection.

In the case of Shigella, these genes may include guaA, guaB, senA, senB, set, aroA, virG, msbB, icsA, iuc, iutA, ipaB, ipaC, ipaD, ipaA. The genes may be deleted or a regulatable promoter may be inserted in front of the gene to achieve regulated delayed attenuation.

In the case of E. coli, attenuating mutations may include deletions in ompF, ompC, ompR, aroA, aroC, aroD, astA, eltB, eltA, estA, cya, crp. The genes may be deleted or a regulatable promoter may be inserted in front of the gene to achieve regulated delayed attenuation.

In some embodiments, a recombinant bacterium of the invention is a species or subspecies of the Salmonella genera. For instance, the recombinant bacterium may be a Salmonella enterica serovar. In an exemplary embodiment, a bacterium of the invention may be derived from S. Typhimurium, S. Typhi, S. Paratyphi, S. Gallinarum, S. Enteritidis, S. Choleraesius, S. Arizona, or S. Dublin. In another exemplary embodiment, a bacterium of the invention may be an S. Typhi bacterium. In yet another exemplary embodiment, a bacterium of the invention may be an S. Typhi Ty2 bacterium. In yet still another exemplary embodiment, a bacterium of the invention may be an S. Gallinarum bacterium. In still yet another exemplary embodiment, a bacterium of the invention may be an S. Dublin bacterium.

A recombinant bacterium of the invention derived from Salmonella may be particularly suited for use as a vaccine. Infection of a host with a Salmonella strain typically leads to colonization of the gut-associated lymphoid tissue (GALT) or Peyer's patches, which leads to the induction of a generalized mucosal immune response to the recombinant bacterium. Further penetration of the bacterium into the mesenteric lymph nodes, liver and spleen may augment the induction of systemic and cellular immune responses directed against the bacterium. Thus the use of recombinant Salmonella for oral immunization stimulates all three branches of the immune system, which is particularly important for immunizing against infectious disease agents that colonize on and/or invade through mucosal surfaces.

(a) Requlatable Cassette

A recombinant bacterium of the invention comprises a regulatable cassette. Such a cassette usually comprises a regulatable promoter operably linked to i) an arginine decarboxylase and an arginine agmatine antiporter; ii) a glutamate decarboxylase and a glutamate/γ-aminobutyric acid antiporter; or iii) a lysine decarboxylase and a lysine/cadaverine antiporter. Each of these elements is described in more detail below.

The term “operably linked,” as used herein, means that expression of a nucleic acid sequence is under the control of a promoter with which it is spatially connected. A promoter may be positioned 5′ (upstream) of the nucleic acid sequence under its control. The distance between the promoter and a nucleic acid sequence to be expressed may be approximately the same as the distance between that promoter and the native nucleic acid sequence it controls. As is known in the art, variation in this distance may be accommodated without loss of promoter function.

A regulatable cassette of the invention may be present in the chromosome of the recombinant bacterium, or may be present in an extrachromosomal vector. In one embodiment, a regulatable cassette may be present in the chromosome of the recombinant bacterium. Methods of chromosomally integrating a regulatable cassette are known in the art and detailed in the examples. Generally speaking, the regulatable cassette should not be integrated into a locus that disrupts colonization of the host by the recombinant bacterium, or that negatively impacts the use of the bacterium to evoke an immune response, such as in a vaccine. In one embodiment, the regulatable cassette may be chromosomally integrated into the locus that comprises nucleic acid encoding an arginine decarboxylase and/or an arginine agmatine antiporter. In another embodiment, the regulatable cassette may be chromosally integrated into the locus that comprises nucleic acid encoding a glutamate decarboxylase and/or a glutamate/γ-aminobutyric acid antiporter. In yet another embodiment, the regulatable cassette may be chromosomally integrated into the locus that comprises nucleic acid encoding a lysine decarboxylase and/or a lysing/cadaverine antiporter.

In another embodiment, a regulatable cassette of the invention may be present in an extrachromosomal vector. As used herein, “vector” refers to an autonomously replicating nucleic acid unit. The present invention can be practiced with any known type of vector, including viral, cosmid, phasmid, and plasmid vectors. The most preferred type of vector is a plasmid vector.

i) Regulatable Promoter

A regulatable cassette of the invention comprises a regulatable promoter. As used herein, the term “promoter” may mean a synthetic or naturally-derived molecule that is capable of conferring, activating or enhancing expression of a nucleic acid. A promoter may comprise one or more specific transcriptional regulatory sequences to further enhance expression and/or to alter the spatial expression and/or temporal expression of a nucleic acid.

The regulated promoter used herein generally allows transcription of a nucleic acid encoding an arginine decarboxylase and a nucleic acid encoding an arginine agmatine antiporter while in a permissive environment (i.e., in vitro aerobic growth), but ceases transcription while in a non-permissive environment (i.e., during anaerobic growth of the bacterium in an animal or human host). For instance, the promoter may be sensitive to a physical or chemical difference between the permissive and non-permissive environment. Stated another way, a regulated promoter of the invention allows for inducible expression of a nucleic acid encoding an arginine decarboxylase and a nucleic acid encoding an arginine agmatine antiporter, even under aerobic conditions. In another embodiment, the regulated promoter used herein generally allows transcription of a nucleic acid encoding a glutamate decarboxylase and a nucleic acid encoding a glutamate/γ-aminobutyric acid antiporter while in a permissive environment (i.e., in vitro aerobic growth), but ceases transcription while in a non-permissive environment (i.e., during anaerobic growth of the bacterium in an animal or human host). Stated another way, a regulated promoter of the invention allows for inducible expression of a nucleic acid encoding a glutamate decarboxylase and a nucleic acid encoding a glutamate/γ-aminobutyric acid antiporter, even under aerobic conditions. In still another embodiment, the regulated promoter used herein generally allows transcription of a nucleic acid encoding a lysine decarboxylase and a nucleic acid encoding a lysine/cadaverine antiporter while in a permissive environment (i.e., in vitro aerobic growth), but ceases transcription while in a non-permissive environment (i.e., during anaerobic growth of the bacterium in an animal or human host). Stated another way, a regulated promoter of the invention allows for inducible expression of a nucleic acid encoding a lysine decarboxylase and a nucleic acid encoding a lysine/cadaverine antiporter, even under aerobic conditions. Suitable examples of such regulatable promoters are known in the art.

In some embodiments, the promoter may be responsive to the level of arabinose in the environment. Generally speaking, arabinose may be present during the in vitro growth of a bacterium, while typically absent from host tissue. In one embodiment, the promoter is derived from an araC-PBAD system. The araC-PBAD system is a tightly regulated expression system, which has been shown to work as a strong promoter induced by the addition of low levels of arabinose. The araC-araBAD promoter is a bidirectional promoter controlling expression of the araBAD nucleic acid sequences in one direction, and the araC nucleic acid sequence in the other direction. For convenience, the portion of the araC-araBAD promoter that mediates expression of the araBAD nucleic acid sequences, and which is controlled by the araC nucleic acid sequence product, is referred to herein as PBAD. For use as described herein, a cassette with the araC nucleic acid sequence and the araC-araBAD promoter may be used. This cassette is referred to herein as araC-PBAD. The AraC protein is both a positive and negative regulator of PBAD. In the presence of arabinose, the AraC protein is a positive regulatory element that allows expression from PBAD. In the absence of arabinose, the AraC protein represses expression from PBAD. This can lead to a 1,200-fold difference in the level of expression from PBAD.

Other enteric bacteria contain arabinose regulatory systems homologous to the araC-araBAD system from E. coli. For example, there is homology at the amino acid sequence level between the E. coli and the S. Typhimurium AraC proteins, and less homology at the DNA level. However, there is high specificity in the activity of the AraC proteins. For example, the E. coli AraC protein activates only E. coli PBAD (in the presence of arabinose) and not S. Typhimurium PBAD. Thus, an arabinose regulated promoter may be used in a recombinant bacterium that possesses a similar arabinose operon, without substantial interference between the two, if the promoter and the operon are derived from two different species of bacteria.

Generally speaking, the concentration of arabinose necessary to induce expression is typically less than about 2%. In some embodiments, the concentration is less than about 1.5%, 1%, 0.5%, 0.2%, 0.1%, or 0.05%. In other embodiments, the concentration is 0.05% or below, e.g. about 0.04%, 0.03%, 0.02%, or 0.01%. In an exemplary embodiment, the concentration is about 0.05%.

In other embodiments, the promoter may be responsive to the level of maltose in the environment. Generally speaking, maltose may be present during the in vitro growth of a bacterium, while typically absent from host tissue. The malT nucleic acid sequence encodes MalT, a positive regulator of four maltose-responsive promoters (PPQ, PEFG, PKBM, and PS). The combination of malT and a mal promoter creates a tightly regulated expression system that has been shown to work as a strong promoter induced by the addition of maltose. Unlike the araC-PBAD system, malT is expressed from a promoter (PT) functionally unconnected to the other mal promoters. PT is not regulated by MalT. The malEFG-malKBM promoter is a bidirectional promoter controlling expression of the malKBM nucleic acid sequences in one direction, and the malEFG nucleic acid sequences in the other direction. For convenience, the portion of the malEFG-malKBM promoter that mediates expression of the malKBM nucleic acid sequence, and which is controlled by the malT nucleic acid sequence product, is referred to herein as PKBM, and the portion of the malEFG-malKBM promoter that mediates expression of the malEFG nucleic acid sequence, and that is controlled by the malT nucleic acid sequence product, is referred to herein as PEFG. Full induction of PKBM requires the presence of the MalT binding sites of PEFG. For use in the vectors and systems described herein, a cassette with the malT nucleic acid sequence and one of the mal promoters may be used. This cassette is referred to herein as malT-Pmal. In the presence of maltose, the MalT protein is a positive regulatory element that allows expression from Pmal.

In still other embodiments, the promoter may be sensitive to the level of rhamnose in the environment. Analogous to the araC-PBAD system described above, the rhaRS-PrhaB activator-promoter system is tightly regulated by rhamnose. Expression from the rhamnose promoter (Prha) is induced to high levels by the addition of rhamnose, which is common in bacteria but rarely found in host tissues. The nucleic acid sequences rhaBAD are organized in one operon that is controlled by the PrhaBAD promoter. This promoter is regulated by two activators, RhaS and RhaR, and the corresponding nucleic acid sequences belong to two transcription units that are located in the opposite direction of the rhaBAD nucleic acid sequences. If L-rhamnose is available, RhaR binds to the PrhaRS promoter and activates the production of RhaR and

RhaS. RhaS together with L-rhamnose in turn binds to the PrhaBAD and the PrhaT promoter and activates the transcription of the structural nucleic acid sequences. Full induction of rhaBAD transcription also requires binding of the Crp-cAMP complex, which is a key regulator of catabolite repression.

Generally speaking, the concentration of rhamnose necessary to induce expression is typically less than about 2%. In some embodiments, the concentration is less than about 1.5%, 1%, 0.5%, 0.2%, 0.1%, or 0.05%. In other embodiments, the concentration is about 0.6%, about 0.5%, about 0.4%, about 0.3%, about 0.2%, or about 0.1%. In an exemplary embodiment, the concentration is about 0.1%. In another exemplary embodiment, the concentration is about 0.4%

Although both L-arabinose and L-rhamnose act directly as inducers for expression of regulons for their catabolism, important differences exist in regard to the regulatory mechanisms. L-Arabinose acts as an inducer with the activator AraC in the positive control of the arabinose regulon. However, the L-rhamnose regulon is subject to a regulatory cascade; it is therefore subject to even tighter control than the araC PBAD system. L-Rhamnose acts as an inducer with the activator RhaR for synthesis of RhaS, which in turn acts as an activator in the positive control of the rhamnose regulon. In the present invention, rhamnose may be used to interact with the RhaR protein and then the RhaS protein may activate transcription of a nucleic acid sequence operably-linked to the PrhaBAD promoter. In some embodiments, the rhaRS-PrhaB activator-promoter cassette from an E. coli K-12 strain may be used.

In still other embodiments, the promoter may be sensitive to the level of xylose in the environment. The xylR-PxylA system is another well-established inducible activator-promoter system. Xylose induces xylose-specific operons (xylE, xylFGHR, and xylAB) regulated by XylR and the cyclic AMP-Crp system. The XylR protein serves as a positive regulator by binding to two distinct regions of the xyl nucleic acid sequence promoters. As with the araC-PBAD system described above, the xylR-PxylAB and/or xylR-PxylFGH regulatory systems may be used in the present invention. In these embodiments, xylR PxylAB xylose interacting with the XylR protein activates transcription of nucleic acid sequences operably-linked to either of the two Pxyl promoters.

The nucleic acid sequences of the promoters detailed herein are known in the art, and methods of operably-linking them to a nucleic acid sequence encoding an arginine decarboxylase and a nucleic acid encoding an arginine agmatine antiporter are known in the art and detailed in the examples.

ii) A Nucleic Acid Sequence Encoding an Arginine Decarboxylase

A regulatable cassette of the invention further comprises an arginine decarboxylase. An arginine decarboxylase is an enzyme that catalyzes the chemical reaction L-arginine agmatine and CO2, and is classified as EC 4.1.1.19. Generally speaking, an arginine decarboxylase useful in the present invention will have acitivity similar to AdiA (e.g. protect a cell from low pH). Suitable examples of arginine decarboxylase are known in the art, and may include the following enzymes (referenced by UNIPROT identifiers, available at www.uniprot.org): Q5L5E7, AAXB_CHLAB; Q822F3, AAXB_CHLCV; Q255I0, AAXB_CHLFF; Q9PK21, AAXB_CHLMU; Q9Z6M7, AAXB_CHLPN; P0C8R4, AAXB_CHLT2; Q3KLY3, AAXB_CHLTA; P0C8R5, AAXB_CHLTB; O84378, AAXB_CHLTR; Q7XRA1, ADC2_ORYSJ; Q96A70, ADC_HUMAN; P28629, ADIA_ECOLI; Q9YG22, ARGDC_AERPE; A8MBV3, ARGDC_CALMQ; A2BM05, ARGDC_HYPBU; A8AAB6, ARGDC_IGNH4; A4YH98, ARGDC_METS5; Q8ZWK3, ARGDC_PYRAE; A4WIW6, ARGDC_PYRAR; A3MTU5, ARGDC_PYRCJ; A1RV83, ARGDC_PYRIL; B1YD10, ARGDC_PYRNV; A3DLU8, ARGDC_STAMF; Q4J932, ARGDC_SULAC; C3N6F7, ARGDC_SULIA; C4KHX2, ARGDC_SULIK; C3MQN7, ARGDC_SULIL; C3MWN7, ARGDC_SULIM; C3NGS9, ARGDC_SULIN; C3NEW5, ARGDC_SULIY; Q9UWU1, ARGDC_SULSO; Q971 K9, ARGDC_SULTO; O27983, PDAD1_ARCFU; Q8TLM4, PDAD1_METAC; P58889, PDAD1_METMA; O30240, PDAD2_ARCFU; Q8TKB4, PDAD2_METAC; P58890, PDAD2_METMA; B3EGI2, PDAD_CHLL2; B3QM53, PDAD_CHLP8; B3ELD9, PDAD_CHLPB; B3QWJ5, PDAD_CHLT3; Q8KEX0, PDAD_CHLTE; B0R6U7, PDAD_HALS3; Q9HNQ0, PDAD_HALSA; A6UUL7, PDAD_META3; Q12UX3, PDAD_METBU; Q57764, PDAD_METJA; Q8TXD4, PDAD_METKA; A4G0Z0, PDAD_METM5; A9A979, PDAD_METM6; A6VHH0, PDAD_METM7; Q6LWX2, PDAD_METMP; O26956, PDAD_METTH; A6UQM7, PDAD_METVS; A9A5S1, PDAD_NITMS; Q3B5D1, PDAD_PELLD; Q6KZS5, PDAD_PICTO; B4S6J7, PDAD_PROA2; A4SFG2, PDAD_PROVI; Q9V173, PDAD_PYRAB; Q8U0G6, PDAD_PYRFU; O59240, PDAD_PYRHO; Q5JFI4, PDAD PYRKO; Q9HK30, PDAD_THEAC; C6A2R5, PDAD_THESM; Q97AN7, PDAD_THEVO; Q0W1C7, or PDAD_UNCMA.

In some embodiments, an arginine decarboxylase of the invention is from a Salmonella species. In particular embodiments, an arginine decarboxylase of the invention is from a Salmonella Typhi strain. In still other embodiments, an arginine decarboxylase of the invention is from a S. Typhi Ty2 strain. In an exemplary embodiment, an arginine decarboxylase of the invention has the amino acid sequence of the protein at accession number Q8Z1 P1.

iii) A Nucleic Acid Encoding an Arginine Agmatine Antiporter

A regulatable cassette of the invention comprises an arginine agmatine antiporter. An arginine agmatine antiporter exchanges extracellular arginine for its intracellular decarboxylation product agmatine (Agm) thereby expelling intracellular protons. Generally speaking, an arginine agmatine antiporter useful in the present invention will have activity similar to AdiC (e.g. protect a cell from low pH). Suitable examples of a arginine agmatine antiporter are known in the art, and may include the following enzymes (referenced by UNIPROT identifiers, available at www.uniprot.org):

Q5L5E6 Q822F2 Q255I1 Q9PK20 Q9Z6M8 B0B7U3 Q3KLY0 B0BC08 O84379 P60063 P60062 P60061 P60065 P60066 P60064 Q8ZGS9 F9I2W4 L0ZZ71 K5SRC8 L2XUK4 L0ZZ90 L3LBG0 K3L3A1 I7RFE4 K5JIM6 H4VPM7 K3ECI9 K5JII2 L4W4Y5 H4VPK5 F3NW25 K3B3S5 I7V0V1 K3SS41 K5U1P0 L4F2K6 L5IZK9 L4VBA1 E1IV59 L8T7H9 E1IV81 I6FGU1 L8RFY1 J1FC03 I5XD20 F1ZQN0 L3RY40 L4T3H6 L4T549 B3H9N6 L0X6N1 L0X6Q1 B5NPC3 B5MPV9 I6JZL9 I7UDX0 A9ZUE1 L1GKB6 L4YQS8 I2SQ31 B5PIR2 L2AD21 B3YHW3 F9A052 G1ZS25 I6I720 L3ANK2 I8L5B5 I7V0M1 B2P2P0 I6K2D0 D1TQ94 B3XCN3 L4TIY7 E7UJV3 G7AK02 I2ZAI5 I5DC16 F5MWJ7 K5U1M6 L3XAL9 L5DBB6 C0AU61 I8AEV7 I7S457 J9XI24 C0AU59 C0AU62 F4UGH3 L9HFX9 I5XWG2 L3EKM3 L3VWN3 L3DTY3 K3RCT8 L8CSG7 I5VI26 K2X636 L2E4E2 K3AGX2 I7UAZ0 L1ZHH6 L3M033 D7ZE63 I5D8I3 I7X7J6 I5Q9Q8 I5M3V3 J1YF14 D7ZE41 L2ZZ90 L2ZV57 L4FNN9 L1R3X9 L1R3Z5 L3YQ74 D8AX24 J9XD49 D8AX02 L3BVT4 L2Y3Z0 L3AQT2 K3L9D5 I5S6B5 D2ZGU0 H4W4R4 L3IJA7 L4JLJ2 K2ZXC3 I8BDE6 H4W4P4 D6KD06 L4A9N4 G5RNX8 I4JEM2 K2ZDJ2 D8AKJ4 L3XEU2 I8P6H8 E7K6V9 L8Z8R4 L8YKJ3 D8AKL7 L3NNJ6 L3BFQ8 K3MKD0 H4KAZ1 H4KAX3 L4IHB5 L2BF09 E7V2M9 G9WDQ0 F1Y6E3 K3JZ37 L2BX70 J9X347 B3IGV7 L4CV86 K5SPP8 L8BQC1 L3NN06 K3U457 F4T7G8 E3Y474 B3AHE0 L4H192 E9TP44 I6G8F1 I6GL91 I6GBL6 L8YEL4 E9TP22 G7B431 E9U4M4 I6GBF5 I6F968 L0X7G9 L0X7I9 K3QB35 I5EN09 L1GNR1 L1GNP4 K5QU54 L4ZG30 J1W870 I7XHW6 G5WM30 L2WZD7 L1AB99 L1AB78 I7V7C5 G5NFS9 I8NA30 G1YHG9 G5NFT1 E3XKM9 L1EFJ6 L4QDY7 L1EFL8 K2W2K4 F4V9D8 G2CT24 I7PI89 C8T226 I5W5W6 B5P6C4 H5N2D9 L4EP61 I5HRC9 H5N267 I7UST4 L1F849 L1F871 K5T2Y1 E7JIF7 F5QPJ9 H4WZP7 L3RSY3 H4WZM8 I2R8G7 B5Q4D3 I5MJT7 L8C1L1 I2UGJ6 F3VDW4 H1FJ08 G5MRE2 I5MTW8 G5MRE4 K3KCA8 L4XNM3 K5DXC6 K5ISM6 K5F1V1 K5ISH8 I8AKN2 I6CMX1 G7A768 G0F4S0 E6B426 J1C6G7 L4SYQ4 K3S724 I8H5G7 J5CMZ3 I5M6S7 J1W394 L4KR23 I6BD24 K3GSB1 L4UGY3 B2NQU7 E9TK06 E9TK28 I2ZLX4 F5QBC2 I5D999 B0GR46 D8C1N4 D8BQX0 L3IMN2 E5ZS94 L2X415 B3WYW2 E5ZSB7 L8SVA7 L3MX95 D7ZVD8 I7ZAY6 F9ALT1 I5S787 K2XVU7 H1DRT2 G5U5M4 I5EVB1 I8SH69 G9Y8K8 H1E1A5 G9Y4C6 G9Y9L2 L8SLE6 I3A6R7 G9Y813 E7TTL9 I2T1Y1 J1GHD8 G5X1P1 L1BFR5 L1BFT3 G5UZS2 F9C3H2 G5QBN3 I5G8K3 L1BCM1 L1BCJ8 K2V6L4 G9SB43 B0GG51 L2CSK5 L5D1W2 J1EY15 G5VHH0 G2CCI8 K3GZI0 E1HK03 K3PN87 L4XCP6 I6DUZ6 I6EXQ7 I5QHY5 E1HJY3 D4E2F3 G5LHQ4 L3CJQ8 L2UQB9 L3FKD7 K3TEP7 L9EA37 I6DE79 F3WRA4 I2V7B6 L0YSU5 K5I296 L0YQH4 L2AJI5 F4LZD4 G2B2X5 G0DBW7 L3MTD6 I8IDI1 I6IKD0 K3ADY5 L5AR67 L4ZY81 I5Z6K3 B3BTH9 G5SJZ9 B0HEW5 G5QT01 B2N252 K3J5D8 I5IS05 E7JBV5 L3NM54 K5HAC9 L4PPI9 K5J592 E1JCI2 L4TRI3 L5C0A6 D4F0D4 D4F4Y3 D4F2I3 E1JCG1 I7SA11 I6KTI0 J9XCX8 D4F0F6 K3HBW8 L4YWU8 L2UUC4 I2RRR4 K5SHK1 H4USI6 L3SMZ0 I2TWS7 I7UER9 I7RDJ7 F3W5J5 G6ZAS1 H4USG6 H4YPM0 L5HV94 H4YPH3 I5QW95 I7WAW3 A9Z9Y2 E9U9I3 L1CQU5 L4QRV7 L4TFJ6 D7YA60 L1CQW4 I2SBG7 L8S2L4 J5XTX4 H4Z4M5 E9U9G3 D7YA80 K3R0A0 K3DX62 L3ZGY3 L3KR37 G5PW35 K2V9Y3 B2PJH9 I7W0J5 G5PW33 G5PGS6 L3GF20 L5EKI8 K5GG82 L5BZY9 L1KR74 K3C1C8 L3H308 D8E3L6 C4U4Q1 I2XLP9 I5WJG5 D8E3J4 H6P1D1 L3VT02 L5GSI7 I5TR12 J1LTN0 L4NC45 G5VX93 L9BGL3 I7WXF3 I5J6Y3 L9IJ71 L2VEC8 J9WRB0 I5S9Y5 G1YK68 H3KCD0 I5V8Q8 L9HX28 L4L951 L1VUB5 L4AJL2 I6HT62 I5HAV4 I5U539 I7P7U1 L9ERL8 G2D7C4 L4I9E1 M3V1I3 H5JRD7 K5G7H8 K5FEJ8 L9AVL2 I5XA14 F5MT32 I7W894 H5JRS9 L1BGE1 L1BGG3 K3GB62 F8YV39 B1EQG3 J1NUH4 L2XN23 I6CJ09 F4UWB4 I6CSL5 J1ZYA9 L1ED04 L4T2N7 L3EV49 L1EE45 F5PH59 K2VYG0 L5A3N0 L3I4F5 L1FUJ6 L5EEA8 L1FUB8 K3I8N8 L5EBV4 L4MLC0 L3SMU3 G5R8V8 L1WZ84 D7YJ24 L4SIF7 B3BAY7 I7QIR7 D7YJ03 I6E3S5 I6E2M6 L1FFZ9 L1FHA6 L3XNJ9 L3AIS0 L3DCM3 L2ZQW7 G9Z382 G9Z6T2 F9B733 L3CTW1 K5GGB1 K5GGC9 L3RU66 K5V7V7 B5CDU5 K2W084 L3R3T7 L3H2Z3 I5KPM2 G5WDR4 I8HN84 K2XEQ7 J1XSN7 L4B207 J2LYB6 L9EWN3 H7E8B6 H7EFP3 G2BH56 I7TE46 G5N5X9 I2VCV4 K3R9D1 K3U183 L4RNN6 L3FZ43 G5XKR7 F8Z5T6 K5SMQ6 L4NUX8 H5HFY0 L5FEK0 K3F8X8 H5HFW1 I7PQR4 L3LTC8 L4A672 G5NWE6 I2Y4M6 G5UG24 E7THT7 J9WX42 G5NWE4 K3DHG1 L4YF33 K5ERV4 L4IQR3 L3J974 K5ERT7 C4UFE9 F9AC54 J1EAB4 F3QA56 L3PA82 L4WDV5 L3CZZ0 K3MPZ0 J2LWC7 I7Q7C5 I8QBE8 I5L1L1 L8DAI2 L3WLQ1 I5SND2 L8T8F8 E7T215 I7W989 L8QUU4 L4BBX6 L5C5U6 E2KBB2 L9B483 L9G1R7 L0Z001 L4RL04 L0YXM5 E2X4N1 L9FCW5 G5Y4V3 H1ENB2 L5AT29 K2Z1I4 F7N4C2 E7UCF3 I8HE83 K2XZX6 H1F466 G6Z285 I5KRA0 F7N4C1 L4KGB0 M1SKM5 L4QZX7 M1RQ73 F5P3T9 L4CN89 L4V0U9 L3U4Y7 I5JAK7 I7WZT3 G7C0I5 F8XI69 K3FB12 L3K5K6 I6FQ39 F8ZRQ5 I6FQG6 I2VUS4 F8X8V9 K2XJA0 L5E756 L4F8M8 L3ZJ80 K5H5J8 L1ZPU4 F9AYU6 F4QX28 H4UB16 L4I150 L2DP62 B5PY28 H4UD30 L9CGU3 I6CE72 L1WYU6 L3Q752 E1I8N2 I0A439 I2YEN5 E1I8Q3 I2XF31 L2B6G5 L4DSI6 I2X267 K2UME8 L9HY73 G5S484 L9G6W1 G5RY80 L5J565 L3UUU8 L4C5Y5 L4MNW4 L4DPM8 L3U3J6 L4A9T1 L8RSC0 B6ZV29 L8SCJ8 L3L740 L5D6D0 K3CQ23 I6BGH7 I6KUL9 F4VPI9 J1P1K1 G6ZP97 B5MYN3 D8BNH2 L0XFR8 E6AW46 E6BPS4 K3EY17 L0XFT6 L1DUJ6 L1DUH5 E9A511 E6AW24 E9A9Z5 E6BPQ3 I5PCC2 D8BNF2 D8BKR1 M1YQ20 M1YQL5 H5HXX1 L5FNP9 D8EPN7 L4J9M5 G1ZD77 H5HXV2 I5FZI4 G5MBY2 D8EPL5 F1XKZ5 L3R5N4 I2PFB7 K3CLI6 I8GHM8 G5YAK0 I5Z8Y0 L0YEQ2 L5GS53 L0YFU2 L2Z6T1 I7YZ57 J1GJF9 K3SPI8 L1R4J3 L1R4N9 B0H3G9 L8R4H6 D0YZT1 L8ZV52 E2KS00 G7ATI2 B3I3F2 I7NQ44 L4FPP1 L1YEC5 L3G7A2 L4PN37 E2JZ15 G7BEV7 L2CG18 K6BMP2 K3IBQ9 L4NAX4 L4UVT9 L1YFF5 K6AQQ4 E7SMJ3 H4LD96 I5TK17 K2YQG0 B5N8X1 D4BKK1 H4LD94 L1ZB17 L5FGA8 L2VPB6 I5UWQ2 G7BSL0 K2W4M5 G2A7N1 I8ABI5 E6A679 L3EMC4 B5BW09 J1EEU3 J9XAE9 G2BXS5 L8ZU36 I2RDZ7 E6A6A0 L5BAV4 L1D8C7 L1D8A4 F9BI15 L9GKG1 G5TR25 I5GHK7 E7IWX0 L5HY14 K3BUT3 I5JSB7 I5PZ94 L4HCK1 L9DIV7 B0HU12 I8R9N2 F9BVG9 B4AA00 J9WX07 D7Z320 L3W464 L4WBE5 D7XTM6 L1VQ23 D7XTK5 D7Z341 I5YHQ1 F4VMA3 K3MDC6 F5NAH0 K3KB42 L9AF12 L4DM02 L1X3N5 H5ISJ7 B3A6E6 I2DXM6 I6D2V7 I6D2V9 H1BTG9 H5ISL6 I2WGN2 I6D2W0 I6CR58 K5FVW8 K5HMA4 K5HM79 I7TD77 I2Z670 I5EQF3 K2T9K2 I7Z9Z3 I6J638 F8ZDV2 L9CEA9 B3B061 E7HSW8 K3MX00 F4TP19 K2V813 L4K1S5 L3PUI4 H4J2D2 G2AP22 H4J2B4 E7IDB4 E2X267 F5PWY4 J9X778 D8CBL7 L1Y967 L4KWW5 L0ZZ14 L0ZZ44 D7X582 L4XFS7 L3UDG0 L4EEY0 D8CBN6 I5NVZ9 I2TLP7 D7X560 L5HPI1 H5IBZ7 L2WC77 I6J919 L9CH33 H5IBX8 J1LJU9 I5HMY4 L2D672 L4QAI1 L1CM27 L3PH92 L1CMJ2 L2TZ71 L9DKJ3 F4U276 K2W210 C4S0N7 L4MQ21 L3YTD0 K3GPD1 K3NAF9 G6ZZN4 J1D607 L2VLJ7 L5GJS3 K3P2I6 L1VS42 L3ITJ5 D8AFI1 D8AFF8 D8AFF9 B3HVQ4 F4SSI1 L4GNN4 L3UXG7 G4C9J0 E7HCX1 G4C3K1 C3SGT2 C6ED09 A9ANX5 B1LQD3 A4JQ30 B7NG51 G8W1Q4 B4TED3 B7MSM8 D2TNK2 A9R299 D3GTZ4 B4TS79 B5F2H0 D2ADB4 B7M8M5 Q399G7 E1WEY4 B2TXC1 Q0B7H7 B7NSS7 B7LB57 B4T2J5 E3PD34 A8A7L1 F8L8H9 F8L8H8 B5Z2C3 A7ZUY5 E8P6N2 B5FRG8 E8P6N3 A7FKG8 B7MJY9

In some embodiments, an arginine agmatine antiporter of the invention is from a Salmonella species. In particular embodiments, an arginine agmatine antiporter of the invention is from a Salmonella Typhi strain. In still other embodiments, an arginine agmatine antiporter of the invention is from a S. Typhi Ty2 strain. In an exemplary embodiment, an arginine agmatine antiporter of the invention has the amino acid sequence of the protein at accession number P60065.

In certain embodiments of the invention the nucleic acid encoding an arginine agmatine antiporter is fused with an arginine decarboxylase encoding sequence such that the intervening regulatory gene adiY is deleted. For instance, in certain embodiments, a Salmonella adiA sequence is fused to a Salmonella adiC sequence.

iv) A Nucleic Acid Encoding a Glutamate Decarboxylase

In some embodiments, a regulatable cassette may comprise a glutamate decarboxylase. A glutamate decarboxylase is an enzyme that catalyzes the chemical reaction L-glutamate γ-aminobutyric acid (GABA) and CO2, and is classified as EC 4.1.1.15. Generally speaking, a glutamate decarboxylase useful in the present invention will have activity similar to GadA and/or GadB (e.g. protect a cell from low pH). Suitable examples of glutamate decarboxylase are known in the art, and may include the following enzymes (referenced by UNIPROT identifiers, available at www.uniprot.org): GadB—P69910, O0418, Q928R9, P69909, P69912; GadA—P69908, Q83QR1, P58288, P69912, or Q9F5P3.

In some embodiments, a glutamate decarboxylase of the invention is from Escherichia coli. In particular embodiments, a glutamate decarboxylase of the invention is from an Escherichia coli O157 strain. In still other embodiments, a glutamate decarboxylase of the invention is from a Shigella species. In some embodiments, two glutamate decarboxylases may be present in the same strain (GadA and GadB). In an exemplary embodiment, a glutamate decarboxylase of the invention has the amino acid sequence of P69910.

v) A Nucleic Acid Encoding a Glutamate/γ-aminobutyric Acid Antiporter

In other embodiments, a regulatable cassette of the invention may comprise a glutamate/γ-aminobutyric acid antiporter. A glutamate/γ-aminobutyric acid antiporter exchanges extracellular glutamate for its intracellular decarboxylation product/γ-aminobutyric acid thereby expelling intracellular protons. Generally speaking, a glutamate/γ-aminobutyric acid antiporter useful in the present invention will have activity similar to GadC (e.g. protect a cell from low pH). Suitable examples of a glutamate/γ-aminobutyric acid antiporter are known in the art, and may include the following enzymes (referenced by UNIPROT identifiers, available at www.uniprot.org): C8U8G2, C6UU78, P58229, P63235, Q8FHG6, EOJ6C9, C9QVX6, Q9CG19, O30417, C7LH11, Q8YBJ1, Q577E9, C4PPM2, B1LFC4, BOBBJ6, B7LZ92, B7L7J1, B6J3P9, Q03U70, A8A049, B0B9W6, E1P9D3, Q3KME6, D5D2L2, C8U8G2, or B7LRF2.

In some embodiments, a glutamate/γ-aminobutyric acid antiporter of the invention may be from Escherichia coli. In particular embodiments, a glutamate/γ-aminobutyric acid antiporter of the invention is from an Escherichia coli O157 strain. In still other embodiments, a glutamate/γ-aminobutyric acid antiporter of the invention is from a Shigella species. In an exemplary embodiment, a glutamate/γ-aminobutyric acid antiporter of the invention has the amino acid sequence of a protein with accession number C6UU78.

vi) A Nucleic Acid Encoding a Lysine Decarboxylase

In certain embodiments, a regulatable cassette of the invention further comprises a lysine decarboxylase. A lysine decarboxylase is an enzyme that catalyzes the chemical reaction L-lysine cadaverine and CO2, and is classified as EC 4.1.1.18. Generally speaking, a lysine decarboxylase useful in the present invention will have activity similar to CadA (e.g. protect a cell from low pH). Suitable examples of lysine decarboxylase are known in the art, and may include the following enzymes (referenced by UNIPROT identifiers, available at www.uniprot.org): P0A1Z1, Q8X8X4, P0A9H4, or C5A1C4.

In some embodiments, a lysine decarboxylase of the invention is from a Salmonella species. In particular embodiments, a glutamate decarboxylase of the invention is from Salmonella Typhi. In other embodiments a lysine decarboxylase of the invention is from an Escherichia coli strain. In an exemplary embodiment, a lysine decarboxylase of the invention has the amino acid sequence of P0A1Z1.

vii) A Nucleic Acid Encoding a Lysine/Cadaverine Antiporter

A regulatable cassette of the invention comprises lysine/cadaverine antiporter. A lysine/cadaverine antiporter exchanges extracellular lysine for its intracellular decarboxylation product cadaverine thereby expelling intracellular protons. Generally speaking, a lysine/cadaverine antiporter useful in the present invention will have activity similar to CadB (e.g. protect a cell from low pH). Suitable examples of a lysine/cadaverine antiporter are known in the art, and may include the following enzymes (referenced by UNIPROT identifiers, available at www.uniprot.org): Q8Z4M1, P0AAF0, P0AAE8, J9ZST9, K0AT87, K0BD30, D3QL54, Q5PIH7, or B5QTS6.

In some embodiments, a lysine/cadaverine antiporter of the invention is from Salmonella species. In particular embodiments, a lysine/cadaverine antiporter of the invention is from Salmonella Typhi. In other embodiments a lysine/cadaverine antiporter of the invention is from Escherichia coll. In an exemplary embodiment, a lysine/cadaverine antiporter of the invention has the amino acid sequence of Q8Z4M1.

viii) A Nucleic Acid Encoding a Chloride Channel

In some embodiments, a regulatable cassette of the invention comprises a chloride channel protein. A chloride channel prevents membrane hyperpolarization at low pH. Generally speaking, a chloride channel protein useful in the present invention will have activity similar to ClcA from E. coll. Suitable examples of a chloride channel are known in the art, and may include the following (referenced by UNIPROT identifiers, available at www.uniprot.org): P37019, Q3Z5K2, Q8ZBM0, Q1 RG33, B7LWB6, B5Y1 L4, Q325Y4, Q32JV3, Q0T851, P59639, A5F0D5, Q9KM62, C3LVE3, Q87GZ9, Q7MDF0, A7FM08, Q1C3X2, A9R1 E4, Q1CLU6, B1IQI5, A6T4V9, B2U300, A7N6K9, Q8D6J0, B2K549, A4TPW7, B1JK21.

In some embodiments, a chloride channel of the invention is from Escherichia species. In particular embodiments, a chloride channel of the invention is from E coli. In other embodiments, a chloride channel of the invention is has significant homology with the E. coli chloride channel, ClcA. A skilled artisan would be able to identify those proteins with significant homology to an E. coli chloride channel. In an exemplary embodiment, the chloride channel of the invention has the amino acid sequence of P37019.

ix) Nucleic Acids Encoding a Urease System

In some embodiments, a regulatable cassette of the invention comprises all or some of a Ni-dependent urease system. A Ni-dependent urease system enables survival in extremely low pH by acid acclimation. Generally speaking, a Ni-dependent urease system useful in the present invention has activity similar to the Helicobacter pylori Ni-dependent urease system. The regulatable cassette may comprise urease proteins, such as UreA and UreB, and a carbonic anhydrase, such as HP1186. Additional components of the urease system, such as a proton-gated urea channel (UreI) and a chaperone complex necessary to incorporate Ni ions into the urease apoenzyme (UreE, UreF, UreG, UreH) may be under control of a constitutive promoter. Constitutive promoters are known in the art and may include PIpp.

In some embodiments, a Ni-dependent urease system of the invention is from Helicobacter species. In an exemplary embodiment, the Ni-dependent urease system of the invention is from H. pylori.

x) Transcription Termination Sequence

In some embodiments, the regulatable cassette further comprises a transcription termination sequence. A transcription termination sequence may be included to prevent inappropriate expression of nucleic acid sequences adjacent to the cassette.

(b) Acid Sensitive/Increase in Acid Resistance

In some embodiments, a recombinant bacterium of the invention is acid sensitive. As used herein, “acid sensitive” means that when cells are cultured under aerobic conditions in minimal media and in the absence of induction of the regulatable cassette, less than 1% of the bacteria are viable after 4 hours at pH3.

In some embodiments, the bacterium may be acid sensitive due to a loss of function of the acid tolerance response. In other embodiments, the bacterium may be acid sensitive due to loss of function of an acid resistance system such as the arginine decarboxylase or lysine decarboxylase system. Such “loss of function” may be caused by one or more mutations in the acid tolerance response, the arginine decarboxylase acid resistance system, the lysine decarboxylase system, or related systems that result in acid sensitivity. In an alternative embodiment, the bacterium may contain no mutation, but be acid sensitive due to exposure to environmental conditions that repress or fail to induce the acid tolerance or acid resistance systems.

In one embodiment, the bacterium may be acid sensitive, at least in part, because of an rpoS mutation. In another embodiment, the bacterium may be acid sensitive, at least in part, because of a phoPQ mutation. In still another embodiment, the bacterium may be acid sensitive, at least in part, because of a fur mutation. In still yet another embodiment, the bacterium may be acid sensitive, at least in part, because of a guaBA mutation.

Advantageously, an acid sensitive bacterium of the invention increases its acid resistance when the regulatable promoter is induced. As used herein “an increase in acid resistance” means that after induction of the regulatable cassette, when cells are cultured under aerobic conditions in minimal media and challenged at pH 3.0 for 4 hours, the number of viable bacteria after 4 hours is increased >10-fold compared to the parent strain lacking the acid resistance system. In some embodiments, induction of the regulatable promoter results in the same degree of acid resistance as the wild-type strain (e.g. without a mutation(s) that confers acid sensitivity). In other embodiments, induction of the regulatable promoter results in a greater degree of acid resistance than the wild-type strain.

(c) Other Mutations

A bacterium of the invention may comprise one or more mutations desirable in a bacterium used to evoke an immune response, such as in a vaccine. In particular, a bacterium may comprise one or more mutations to increase invasiveness, one or more mutations to allow endosomal escape, one or more mutations to reduce bacterium-induced host programmed cell death, one or more mutations to induce lysis of the bacterium, one or more mutations to express a nucleic acid encoding an antigen, one or more mutations to attenuate the bacterium, and/or other mutations to enhance the performance of the bacterium as a vaccine.

(d) Exemplary Embodiments

In exemplary embodiments of the present invention, the recombinant bacterium is a Salmonella Typhi bacterium adapted for use as a live attenuated vaccine. In further exemplary embodiments, the arginine decarboxylase and the arginine agmatine antiporter comprising the regulatable cassette are derived from a Salmonella bacterium. In still further exemplary embodiments, the arginine decarboxylase and the arginine agmatine antiporter comprising the regulatable cassette are adiA and adiC from Salmonella Typhi. In some embodiments, the cicA gene from E. coli is present in the chromosome and transcribed from its own native promoter, a heterologous constitutive promoter or a heterologous regulatable promoter.

In still another embodiment, a recombinant bacterium of the invention may comprise a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ. In some embodiments, the regulatable acid resistance cassette is regulated by a sugar-inducible promoter. The recombinant bacterium is acid sensitive in the absence of inducer for the regulatable acid resistance cassette. In particular embodiments, the regulatory promoter is responsive to the presence of rhamnose or arabinose. In some embodiments, the acid resistance mechanism comprises a ΔPcadBA:TT rhaSR PrhaBAD cadBA or ΔPcadBA::TT araC ParaBAD cadBA mutation.

In further exemplary embodiments, the lysine decarboxylase and the lysine: cadaverine antiporter comprising the regulatable cassette are derived from a member of the y-proteobacteria class. In other exemplary embodiments, the lysine decarboxylase and the lysine: cadaverine antiporter are cadA and cadB from Salmonella. In still further exemplary embodiments, cadA and cadB are derived from Salmonella Typhi. In some embodiments, the cicA gene from E. coli is present in the chromosome and transcribed from its own native promoter, a heterologous constitutive promoter or a heterologous regulatable promoter.

In a different exemplary embodiment, the regulatable acid resistance cassette is regulated by a sugar-inducible promoter. The recombinant bacterium is acid sensitive in the absence of inducer for the regulateable acid resistance cassette. In particular embodiments, the promoter is responsive to the presence of rhamnose or arabinose. In further exemplary embodiments, the glutamate decarboxylase and the glutamate/γ-aminobutyric acid antiporter comprising the regulatable cassette are derived from a bacterium of the y-proteobacteria class. In still further exemplary embodiments, the glutamate decarboxylase and the glutamate/γ-aminobutyric acid antiporter comprising the regulatable cassette are from Escherichia coli. In particular embodiments, a glutamate decarboxylase of the invention is from an Escherichia coli O157:H7 strain. In still other embodiments, a glutamate decarboxylase of the invention is from a Shigella species. In some embodiments, two glutamate decarboxylases may be present in the same strain (GadA and GadB). In some embodiments, the clcA gene from E. coli is present in the chromosome and transcribed from its own native promoter, a heterologous constitutive promoter or a heterologous regulatable promoter.

In a different embodiment, a recombinant bacterium of the invention comprises a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ. In some embodiments, the regulatable acid resistance cassette is regulated by a sugar-inducible promoter. The recombinant bacterium is acid sensitive in the absence of inducer for the regulateable acid resistance cassette. In particular embodiments, the promoter is responsive to the presence of rhamnose or arabinose. In some exemplary embodiments, the acid resistance mechanism is composed of a urease enzyme. In further embodiments, accessory proteins such as a proton-gated urea channel, carbonic anhydrase or enzyme chaperones will comprise additional components of the acid resistance mechanism. In particular embodiments, the urease, urease channel, carbonic anhydrase and apoenzyme chaperones are derived from a Helicobacter species. In other specific embodiments, the components that comprise the acid resistance mechanism are UreA, UreB, UreI, UreE, UreF, UreG, UreH and HP1186 from Helicobacter pylori.

In several exemplary embodiments, a recombinant bacterium of the invention is acid sensitive, is a Salmonella Typhi bacterium adapted for use as a live attenuated vaccine, and the arginine decarboxylase and the arginine agmatine antiporter comprising the regulatable cassette are adiA and adiC from Salmonella Typhi.

In one exemplary embodiment, a recombinant bacterium of the invention comprises a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ that renders the bacterium acid sensitive in the absence of rhamnose, and comprises a ΔPadiA::TT rhaSR PrhaBAD adiAC mutation.

In another exemplary embodiment, a recombinant bacterium of the invention comprises a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ that renders the bacterium acid sensitive in the absence of arabinose, and comprises a ΔPadiA::TT araC ParaBAD adiAC mutation.

In several exemplary embodiments, a recombinant bacterium of the invention is acid sensitive, is a Salmonella Typhi bacterium adapted for use as a live attenuated vaccine, and the glutamate decarboxylase and a glutamate/γ-aminobutyric acid antiporter comprising the regulatable cassette are gadB and gadC from Escherichia coli.

In one exemplary embodiment, a recombinant bacterium of the invention comprises a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ that renders the bacterium acid sensitive in the absence of rhamnose, and comprises a ΔPgadB:: TT rhaSR PrhaBAD gadBC mutation.

In another exemplary embodiment, a recombinant bacterium of the invention is a S. Typhi strain comprising a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ that renders the bacterium acid sensitive in the absence of arabinose, and comprises a ΔcysG::TT araC PBAD gadBC mutation.

In still another exemplary embodiment, a recombinant bacterium of the invention comprises a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ that renders the bacterium acid sensitive in the absence of arabinose, and comprises a APgadB::TT araC PBAD gadBC mutation.

In several exemplary embodiments, a recombinant bacterium of the invention is acid sensitive, is a Salmonella Typhi bacterium adapted for use as a live attenuated vaccine, and the lysine decarboxylase and a lysine/cadaverine antiporter comprising the regulatable cassette are cadB and cadA from Salmonella Typhi.

In one exemplary embodiment, a recombinant bacterium of the invention comprises a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ that renders the bacterium acid sensitive in the absence of rhamnose, and comprises a ΔPcadB:: TT rhaSR PrhaBAD cadBA mutation.

In another exemplary embodiment, a recombinant bacterium of the invention comprises a mutation in at least one of aroD, guaBA, rpoS, fur, or phoPQ that renders the bacterium acid sensitive in the absence of arabinose, and comprises a ΔPcadB::TT araC PBAD cadBA mutation.

In still another exemplary embodiment, a recombination bacterium of the invention is a Salmonella enterica serovar Gallinarum (S. Gallinarum) comprising a mutation in at least one of pmi or fur that renders the bacterium sensitive in the absence of arabinose, and comprises a ΔcysG::TT araC PBAD gadBC mutation.

In other exemplary embodiments, a recombinant bacterium of the invention is a Salmonella enterica serovar Dublin (S. Dublin) comprising a ΔPadiA::TT rhaSR RrhaBAD adiA Δ(PadiY::-adiY-PadiC) adiC mutation or a ΔcysG::TT araC PBAD gadBC mutation.

II. Vaccine Compositions and Administration

A recombinant bacterium of the invention may be administered to a host as a vaccine composition. As used herein, a vaccine composition is a composition designed to elicit an immune response to the recombinant bacterium, including any antigens that may be expressed by the bacterium. In an exemplary embodiment, the immune response is protective, as described above. Immune responses to antigens are well studied and widely reported. A survey of immunology is given by Paul, W E, Stites D et.al. and Ogra P L. et.al. Mucosal immunity is also described by Ogra P L et.al.

Vaccine compositions of the present invention may be administered to any host capable of mounting an immune response. Such hosts may include all vertebrates, for example, mammals, including domestic animals, agricultural animals, laboratory animals, and humans, and various species of birds, including domestic birds and birds of agricultural importance. Preferably, the host is a warm-blooded animal. The vaccine can be administered as a prophylactic or for treatment purposes.

In exemplary embodiments, the recombinant bacterium is alive when administered to a host in a vaccine composition of the invention. In further exemplary embodiments, a recombinant bacterium comprising a vaccine of the invention is derived from Salmonella Typhi. In still further exemplary embodiments, a recombinant bacterium comprising a vaccine of the invention is derived from Salmonella Typhi Ty2. Suitable vaccine composition formulations and methods of administration are detailed below.

(a) Vaccine Composition

A vaccine composition comprising a recombinant bacterium of the invention may optionally comprise one or more possible additives, such as carriers, preservatives, stabilizers, adjuvants, and other substances.

In one embodiment, the vaccine comprises an adjuvant. Adjuvants, such as aluminum hydroxide or aluminum phosphate, are optionally added to increase the ability of the vaccine to trigger, enhance, or prolong an immune response. In exemplary embodiments, the use of a live attenuated recombinant bacterium may act as a natural adjuvant. The vaccine compositions may further comprise additional components known in the art to improve the immune response to a vaccine, such as T cell co-stimulatory molecules or antibodies, such as anti-CTLA4. Additional materials, such as cytokines, chemokines, and bacterial nucleic acid sequences naturally found in bacteria, like CpG, are also potential vaccine adjuvants.

In another embodiment, the vaccine may comprise a pharmaceutical carrier (or excipient) used to resuspend the lyophilized RASV. Live RASVs are generally lyophilized in the presence of various types of protectants, very often sugars, than enhance thermal stability and are reconstituted at time of use. Such a carrier may be any solvent or solid material for encapsulation that is non-toxic to the inoculated host and compatible with the recombinant bacterium. A carrier may give form or consistency, or act as a diluent. Suitable pharmaceutical carriers may include liquid carriers, such as normal saline and other non-toxic salts at or near physiological concentrations, and solid carriers not used for humans, such as talc or sucrose, or animal feed. Carriers may also include stabilizing agents, wetting and emulsifying agents, salts for varying osmolarity, encapsulating agents, buffers, and skin penetration enhancers. Carriers and excipients as well as formulations for parenteral and nonparenteral drug delivery are set forth in Remington's Pharmaceutical Sciences 19th Ed. Mack Publishing (1995). When used for administering via the bronchial tubes, the vaccine is preferably presented in the form of an aerosol.

Care should be taken when using additives so that the live recombinant bacterium is not killed, or have its ability to effectively colonize lymphoid tissues such as the GALT, NALT and BALT compromised by the use of additives. Stabilizers, such as lactose or monosodium glutamate (MSG), may be added to stabilize the vaccine formulation against a variety of conditions, such as temperature variations or a freeze-drying process.

The dosages of a vaccine composition of the invention can and will vary depending on the recombinant bacterium, the regulated antigen, and the intended host, as will be appreciated by one of skill in the art. Generally speaking, the dosage need only be sufficient to elicit a protective immune response in a majority of hosts. Routine experimentation may readily establish the required dosage. Typical initial dosages of vaccine for oral administration could be about 1×107 to 1×1010 CFU depending upon the age of the host to be immunized. Administering multiple dosages may also be used as needed to provide the desired level of protective immunity.

In an embodiment, a vaccine composition of the invention may be administered in combination with a compound to reduce the pH of the gastric components. The compound may be used to buffer the stomach pH of a subject. Buffering the pH of the stomach may further enhance the immune response elicited in response to a vaccine composition. In an exemplary embodiment, Ensure® may be administered in combination with a vaccine composition. In another exemplary embodiment, sodium bicarbonate may be administered in combination with a vaccine composition.

(b) Methods of Administration

In order to stimulate a preferred response of the GALT, NALT or BALT cells, administration of the vaccine composition directly into the gut, nasopharynx, or bronchus is preferred, such as by oral administration, intranasal administration, gastric intubation or in the form of aerosols, although other methods of administering the recombinant bacterium, such as intravenous, intramuscular, subcutaneous injection or intramammary, intrapenial, intrarectal, vaginal administration, or other parenteral routes, are possible.

In some embodiments, these compositions are formulated for administration by injection (e.g., intraperitoneally, intravenously, subcutaneously, intramuscularly, etc.). Accordingly, these compositions are preferably combined with pharmaceutically acceptable vehicles such as saline, Ringer's solution, dextrose solution, and the like.

III. Kits

The invention also encompasses kits comprising any one of the compositions above in a suitable aliquot for vaccinating a host in need thereof. In one embodiment, the kit further comprises instructions for use. In other embodiments, the composition is lyophilized such that addition of a hydrating agent (e.g., buffered saline) reconstitutes the composition to generate a vaccine composition ready to administer, preferably orally.

IV. Methods of Use

A further aspect of the invention encompasses methods of using a recombinant bacterium of the invention. For instance, in one embodiment the invention provides a method for modulating a host's immune system. The method comprises administering to the host an effective amount of a composition comprising a recombinant bacterium of the invention. One of skill in the art will appreciate that an effective amount of a composition is an amount that will generate the desired immune response (e.g., mucosal, humoral or cellular). Methods of monitoring a host's immune response are well-known to physicians and other skilled practitioners. For instance, assays such as ELISA, and ELISPOT may be used. Effectiveness may be determined by monitoring the amount of the antigen of interest remaining in the host, or by measuring a decrease in disease incidence caused by a given pathogen in a host. For certain pathogens, cultures or swabs taken as biological samples from a host may be used to monitor the existence or amount of pathogen in the individual.

In another embodiment, the invention provides a method for eliciting an immune response against an antigen in a host. The method comprises administering to the host an effective amount of a composition comprising a recombinant bacterium of the invention.

In still another embodiment, a recombinant bacterium of the invention may be used in a method for eliciting an immune response against a pathogen in an individual in need thereof. The method comprises administrating to the host an effective amount of a composition comprising a recombinant bacterium as described herein. In a further embodiment, a recombinant bacterium described herein may be used in a method for ameliorating one or more symptoms of an infectious disease in a host in need thereof. The method comprises administering an effective amount of a composition comprising a recombinant bacterium as described herein.

In a further embodiment, the present invention encompasses a method for increasing the acid resistance of an acid sensitive bacterium. The method comprises introducing into the acid sensitive bacterium a cassette comprising a regulatable promoter operable linked to an arginine decarboxylase and an arginine agmatine antiporter as described in Section I above. Alternatively, the method comprises introducing into the acid sensitive bacterium a cassette comprising a regulatable promoter operable linked to a glutamate decarboxylase and a glutamate/γ-aminobutyric acid antiporter as described in Section I above. In another embodiment, the method comprises introducing into the acid sensitive bacterium a cassette comprising a regulatable promoter operable linked to a lysine decarboxylase and a lysine/cadaverine antiporter as described in Section I above. Upon induction of the regulatable promoter, the recombinant bacterium experiences an increase in acid resistance. In some variations of these embodiments, the regulatable promoter may be induced by a sugar, such as rhamnose or arabinose. In other variations of these embodiments, the recombinant bacterium comprises a mutation in at least one nucleic acid sequence selected from the group consisting of aroD, guaBA, rpoS, fur, and phoPQ.

In yet still another embodiment, the present invention encompasses a method of increasing the survival of probiotic bacteria during passage throught the stomach. The method comprises introducing into the probiotic bacterium a cassette comprising a regulatable promoter operable linked to an arginine decarboxylase and an arginine agmatine antiporter as described in Section I above. Alternatively, the method comprises introducing into the probiotic bacterium a cassette comprising a regulatable promoter operable linked to a glutamate decarboxylase and a glutamate/γ-aminobutyric acid antiporter as described in Section I above. In another embodiment, the method comprises introducing into the probiotic bacterium a cassette comprising a regulatable promoter operable linked to a lysine decarboxylase and a lysine/cadaverine antiporter as described in Section I above. Upon induction of the regulatable promoter, the recombinant bacterium experiences an increase in acid resistance. In some variations of these embodiments, the regulatable promoter may be induced by a sugar, such as rhamnose or arabinose. According to this method, the probiotic bacterium survives the low pH stomach environment and effectively colonizes the subject.

The following examples are included to demonstrate preferred embodiments of the invention. It should be appreciated by those of skill in the art that the techniques disclosed in the examples that follow represent techniques discovered by the inventors to function well in the practice of the invention. Those of skill in the art should, however, in light of the present disclosure, appreciate that may changes can be made in the specific embodiments that are disclosed and still obtain a like or similar result without departing from the spirit and scope of the invention, therefore all matter set forth or shown in the accompanying drawings is to be interpreted as illustrative and not in a limiting sense.

EXAMPLES

The following examples are simply intended to further illustrate and explain the present invention. The invention, therefore, should not be limited to any of the details in these examples.

Introduction

Before orally ingested enteric pathogens such as Salmonella can reach their target host cells, they must first survive their encounter with the low pH of the human stomach; approximately 2.0 following a fast (1). This is an extremely hostile environment for wild-type Salmonella, thus Salmonella contains multiple regulatable systems to aid in survival at low pH (2, 3). The best studied of these systems is the acid tolerance response (ATR). Cells exposed to moderately low pH synthesize numerous acid shock proteins. Although the specific functions of these proteins are largely unknown, jointly they mitigate the proton damage experienced by the cell during low pH challenge (pH 3.0) (4, 5). The acid tolerance response is a complex multi-component system coordinated by a number of global regulatory proteins. In stationary phase, RpoS is a key regulator of the acid tolerance response. Not only does the acid tolerance response of an rpoS mutant fail to provide the same level of protection as in a wild-type strain, but rpoS mutants are unable to sustain the acid tolerance response, resulting in rapid cell death upon pH 3.0 challenge (4, 6). In log phase cells, the Salmonella virulence proteins PhoP/PhoQ and Fur regulate the acid tolerance response. Fur controls a subset of acid shock proteins essential for protecting the cell against organic acid challenge while PhoP/PhoQ coordinates protection against inorganic acid challenge (7, 8).

The vast majority of live attenuated Salmonella vaccines for humans are constructed from Salmonella Typhi strain Ty2, an rpoS mutant (9). To create a vaccine, additional attenuating mutations are necessary in virulence genes. However, these mutations can affect more than just virulence. In addition to the rpoS mutation derived from its parent strain Ty2, the licensed typhoid vaccine strain Ty21a carries galE and tvi mutations as well as a number of other, less well-characterized, mutations (10-12). The strain is sensitive to low pH, due at least in part to its inability to mount a functional acid tolerance response (13). Another vaccine strain, Ty800, contains a deletion of the phoPQ locus. This strain is safe and reasonably immunogenic in humans (14), but one would expect that the combination of the phoPQ deletion and rpoS mutation would render this strain exquisitely sensitive to acidic pH (6, 8). A similar situation occurs for the vaccine strains χ9639(pYA4088) and χ9640(pYA4088) (15). These strains are also safe and immunogenic in humans (69), but the mutation in their fur locus leaves them vulnerable to low pH.

Most vaccine researchers avoid the problem low gastric pH poses by coating their vaccine in a protective enteric capsule (e.g. Ty21a) or by co-administering an antacid (usually sodium bicarbonate) at the time of immunization (16-21). Preventing vaccine exposure to low pH increases the number of viable cells that reach the intestine and improves vaccine immunogenicity (21, 22).The disadvantage of bypassing the acidic environment of the stomach is that the low pH encounter serves as an important signal to Salmonella, allowing it to recognize entry into a host environment. Exposure to acid stimulates up-regulation of the genes that confer resistance to the short chain fatty acids (23), antimicrobial peptides (24) and osmotic stress (6) found in the intestine. Also, induction of the acid tolerance response has been linked to upregulation of SPI-1 and SPI-2 and an increase in epithelial cell invasion in the intestine (25-27). Thus, transient exposure to low pH prepares the invading bacteria for the stresses of the intestine and for host-cell interactions. Therefore, it is possible that if we can enhance the survival rate of live attenuated Salmonella vaccine strains at low pH, we can not only eliminate the need for low pH bypass strategies but also improve the ability of the vaccine strain to interact with host tissues to enhance immunogenicity.

As a first step toward this goal, we explored methods to increase the low pH survival of S. Typhi strains containing rpoS, phoPQ or fur mutations, because each renders strains acid sensitive and each has been incorporated into live attenuated vaccine strains. One robust means used by Salmonella to resist low pH challenge is the arginine decarboxylase acid resistance system (AR3) (28). This system consists of arginine decarboxylase (AdiA) and an arginine-agmatine antiporter (AdiC) (29). Acid resistance is conferred by the activity of AdiA, which consumes one proton from the intracellular environment with each reaction cycle and causes a rapid rise in intracellular pH (30, 31). AdiC then exchanges the agmatine reaction product to the periplasm in exchange for another arginine substrate molecule(29, 32).The combined activities of AdiA and AdiC allow Salmonella to resist pH 2.5 for greater than two hours(3).

Because the arginine decarboxylase system functions independently of the acid tolerance response, we hypothesized that synthesis of AdiA and AdiC would confer high levels of acid resistance on strains containing mutations that affect acid tolerance such as rpoS, phoPQ and fur. However, the arginine decarboxylase system is tightly regulated and is not normally available to cells grown under standard vaccine culture conditions (33). Therefore, we replaced the native promoter of arginine decarboxylase with the araBAD or rhaBAD promoter and compared the level of arginine decarboxylase activity when cells were cultured in the presence of arabinose and rhamnose, respectively. Once we selected the promoter with optimal sugar-dependent expression and activity of the arginine decarboxylase system (PrhaBAD), our objectives were two-fold. First, we determined if the rhamnose-regulated arginine decarboxylase system could rescue rpoS, phoPQ and fur mutants during low pH challenge if cells were cultured in the presence of rhamnose but without any other environmental signals that would induce either decarboxylase activity or the acid tolerance response. Second, to determine whether the rhamnose-regulated system functioned equivalently to the native arginine decarboxylase system, we compared the level of acid resistance afforded by the rhamnose-dependent arginine decarboxylase system with the acid resistance of rpoS, phoPQ and fur mutants cultured under decarboxylase- and acid tolerance-inducing conditions.

Materials and Methods

DNA manipulation and plasmid construction. Chromosomal DNA from S. Typhi Ty2 was isolated using the Wizard Genomic DNA Purification kit (Promega, Madison, Wis., USA). Plasmid DNA was isolated using QIAprep Spin Miniprep kit (QIAGEN, Valencia, Calif., USA) or the Wizard Plus Midiprep DNA Purification system (Promega). DNA inserts were amplified by PCR using the Phusion DNA polymerase (New England Biolabs, lspwich, Mass., USA) or the Easy-A high-fidelity PCR cloning enzyme (Agilent, Santa Clara, Calif., USA). Restriction and modification enzymes for cloning (New England Biolabs) were used in accordance with the manufacturer's instructions.

Construction of S. Typhi mutants. The bacterial strains and plasmids used in this study are listed in Table 1. Primers used during the construction of plasmids are listed in Table 2. To construct the ΔaroD mutation, two DNA fragments adjacent to the aroD gene were amplified from the chromosome of Ty2. Primers Aro-1 and -2 were used for the upstream fragment, while primers Aro-3 and -4 were used for the downstream fragment. These fragments were digested with BamHl, ligated using T4 DNA ligase, re-amplified by PCR with primers Aro-1 and -4 and cloned into the Ahdl sites of pYA4278 via TA overhangs to generate the suicide vector pYA4895. The ΔaroD deletion was introduced into Ty2 by conjugation as described by Kaniga (34). The resulting strain (χ11548) exhibits aromatic amino acid auxotrophy and carries a deletion of the complete coding sequence of aroD that spans 759 bp.

An arabinose-regulated fur mutant was constructed via P22 HT int transduction (35) using a lysate grown on χ9269 containing a chromosomally integrated copy of pYA4181 (36) to create the S. Typhi strain χ11118. The presence of the ΔPfur::TT araC PBAD fur mutation in S. Typhi was confirmed by PCR using the primers Fur-1 and -2. Arabinose-dependent synthesis of Fur was verified by western blot.

To remove the entire adi locus (A(adiA-adiC)), the upstream and downstream flanking regions in Ty2 were amplified using PCR primers Adi-1 and -2 and primers Adi-3 and -4, respectively. The flanking regions were digested with BamHl and ligated together with T4 DNA ligase. The resulting product was re-amplified by PCR using primers Adi-1 and -4 and cloned into the Ahdl sites of pYA4278 to generate the suicide vector pYA5066. The A(adiA-adiC) mutation (hereafter (ΔadiA-adiC) encoded by pYA5066 was moved into Ty2 to create χ11500. This strain carries a 4806-bp deletion of the adi locus (complete coding sequences of adiA, adiY and adiC along with the adiY and adiC promoters) (FIG. 1). The absence of the adi locus was confirmed by PCR and by arginine decarboxylase assay.

Two mutations were constructed that placed adiA under the control of sugar-responsive promoters—A66 PadiA::TT araC ParaBAD adiA (regulated by arabinose) and ΔPadiA::TT rhaSR PrhaBAD adiA (regulated by rhamnose). For simplicity, these mutations will be referred to as ParaBAD adiA and PrhaBAD adiA, respectively. For the arabinose-regulated construct, the DNA regions flanking the adiA promoter were amplified by PCR from Ty2 using primers Adi-5 and-6 for the upstream region and primers Adi-7 and -8 for the downstream region. Both flanking regions were cloned into pYA3700 (using SphI and BgIII for the upstream region and KpnI and SacI for the downstream region) to generate pYA5075. The DNA segment containing the flanking regions and arabinose promoter was amplified by PCR using Adi-5 and -8 and the PCR product was cloned into the Ahdl sites of pYA4278 to create the suicide vector pYA5089. To generate the rhamnose-regulated construct, the araC ParaBAD promoter of pYA5089 was removed by XhoI and XbaI double digestion. The rhaSR PrhaBAD promoter from pYA5081 was amplified by PCR with the Rha-1 and -2 primers and cloned into pYA5089 using XhoI and XbaI to produce the suicide vector pYA5093. pYA5089 and pYA5093 were introduced into χ11548 by conjugation to produce χ11552 and χ11564, respectively. The juxtaposition of adiA with the appropriate promoter was verified by PCR with the Ara-1 and Adi-9 primers (χ11552) or Rha-3 and Adi-9 primers (χ11564) and by arginine decarboxylase assay. In both strains, 203 bp of the intergenic region between melR and adiA (including the -10 and -35 sites of the adiA promoter) were deleted and replaced with either TT araC ParaBAD (χ11552) or TT rhaRS PrhaBAD (χ11564). The strong transcription terminator T4 ip III was placed between the upstream melR gene and araC or rhaSR to prevent expression of anti-sense RNA. A strong Shine-Dalgarno site (AGGA) was inserted 10 bp upstream of the ATG start codon of adiA (FIG. 1).

The adiC gene was fused into an operon with adiA resulting in the Δ(PadiY-adiY-PadiC) adiC mutation (hereafter adiAC). The DNA regions flanking adiY were amplified by PCR from Ty2 using primers Adi-10 and -11 for the upstream region and primers Adi-12 and -13 for the downstream region. The two DNA segments were joined by overlap PCR and re-amplification with Adi-10 and -13. The final PCR product was ligated into pYA4278 at the Ahdl sites to produce the suicide vector pYA5072. The suicide vector was introduced into χ11564 and χ11548 by conjugation to produce χ11568 (ΔaroD PrhaBAD adiAC) and χ11636 (ΔaroD adiAC), respectively. The presence of the adiAC operon was confirmed by PCR using Adi-14 and -15. Both strains harbor a 1078-bp deletion that spans the transcription terminator following adiA, adiY and the promoter of adiC. The adiA and adiC genes are separated by a 119-bp intergenic sequence expected to decrease expression of adiC from the promoter upstream of adiA (FIG. 1).

Growth conditions and culture media. Experiments testing the regulation of arabinose- and rhamnose-controlled genes were conducted in the carbohydrate-free medium purple broth (BD Biosciences, Franklin Lakes, N.J., USA). For acid resistance experiments, strains were propagated in tryptic soy broth (TSB) (BD Biosciences) with 0.4% glucose, or in minimal E medium, pH 7.0 with 0.4% glucose (EG medium) (37). For our experiments, 22 μg/ml L-cysteine, 20 μg/ml L-tryptophan and 0.1% casamino acids were added to EG medium in order to supplement the growth of all strains (EGA medium). For strains with the ΔaroD mutation, 20 μg/ml L-tryptophan, 2 μg/ml p-aminobenzoic acid and 2.5 μg/ml 2, 3-dihydroxybenzoate were added to all media. EGA medium was additionally supplemented with 50 μg/ml L-phenylalanine and 20 μg/ml L-tyrosine. Rhamnose was added to 0.1% or to 0.4% in the case of strain χ11623, as indicated. Strains containing the ΔPfur::TT araC ParaBAD fur mutation were supplied with 0.2% arabinose unless otherwise indicated. All chemicals were purchased from Sigma-Aldrich (St. Louis, Mo., USA) or Thermo Fisher Scientific (Pittsburgh, Pa., USA) unless otherwise indicated.

Measurement of adiA expression by semi-quantitative PCR. Strains were grown in purple broth with varying concentrations of rhamnose or arabinose to an optical density at 600 nm (OD600) of 0.6. Total cellular RNA was isolated using the RNeasy Mini Kit (QIAGEN) and was treated with RNase-free DNase (QIAGEN). cDNA was generated via reverse transcription-PCR (RT-PCR) using 1 μg of cellular RNA with the TaqMan Reverse Transcriptase kit (Life Technologies, Grand Island, N.Y.) under the following conditions: 10 minutes at 25° C. for optimal random hexamer primer binding, then 45 minutes at 48° C. for extension followed by 5 minutes at 95° C. to heat inactivate the transcriptase. Semi-quantitative PCR of the adiA and gapA transcripts was performed using the GoTaq DNA Polymerase system (Promega) using primers SQ-1 and SQ-2 for gapA and SQ-3 and SQ-4 for adiA under the following conditions: 2.5 minutes at 95° C. for template denaturation, followed by 28 cycles of 40s at 95° C., 30 s at 48° C. for primer annealing and 1 minute at 72° C. for primer extension. The semi-quantitative PCR primer sequences are listed in Table 2 (SQ1-SQ4). PCR products were electrophoresed on a 2% agarose gel in the presence of ethidium bromide and visualized with the Chemi Doc XRS System (Bio-Rad Laboratories, Hercules, Calif., USA). Images were analyzed in Adobe PhotoshopCS4 (Adobe Systems Incorporated, San Jose, Calif., USA) in order to establish histogram values for the fluorescence signal intensity of the PCR products. Signal intensity values for adiA were normalized to the value obtained with the single gene expression control gapA for each culture.

Preparation of antiserum against arginine decarboxylase protein. E. coli BL21(DE3) harboring pYA5085 was used for the synthesis of His-tagged AdiA protein. Cells were grown in LB at 37° C. to mid-log phase (an optical density value at 600 nm [OD600] of 0.6). The growth medium was supplemented with 0.2 g/L pyridoxine to augment protein folding and enzyme activity (38). Protein synthesis was induced with 1 mM IPTG (isopropyl β-D-1-thiogalactopyranoside) (Amresco, Solon, Ohio, USA) for 4 hours at 37° C. Cells were collected by centrifugation and disrupted using lysozyme (3 mg/g cells) and deoxycholic acid (120 mg/g cells) (39). His-tagged AdiA protein from the soluble fraction was purified over TALON™ metal affinity resin (BD Biosciences) in accordance with the manufacturer's instructions except that 10% ethanol was added to the elution buffer. Purified protein was stored in 20 mM HEPES, 50 mM NaCl, pH 8.0 (30).

One juvenile New Zealand white rabbit (Charles River Laboratories, Wilmington, Mass., USA) was immunized with 200 μg of AdiA emulsified in Freund's complete adjuvant, and boosted with an additional 200 μg of AdiA emulsified in Freund's incomplete adjuvant 4 weeks and 8 weeks after the initial injection. Serum was collected 3 weeks following the final immunization.

Western blot procedure. Strains were grown overnight at 37° C. in purple broth containing various concentrations of rhamnose or arabinose. The amount of total cellular protein in each sample was normalized by absorbance at 280 nm using the NanoDrop ND-1000 (Thermo Scientific, Wilmington, De., USA). Equal amounts of cellular protein (100 μg for AdiA; 150 μg for Fur) were mixed with 2× SDS-PAGE buffer, boiled, and electrophoresed on a 10% acrylamide gel (40). Separated proteins were transferred to a PVDF membrane (Bio-Rad) using Towbin's wet transfer method (41), blocked in 5% skim milk, then probed with rabbit antiserum (final dilution 1:10,000) for the presence of AdiA or Fur (36). Bound primary antibody was detected by the addition of goat anti-rabbit IgG conjugated to alkaline phosphatase (Sigma-Aldrich). Blots were developed with NBT/BCIP (Amresco) and photographed using the ChemiDocXRS System.

Arginine decarboxylase assays. Arginine decarboxylase enzyme activity was measured using a modified version of the rapid glutamate decarboxylase assay previously described (42). Strains were grown overnight (18 h) to stationary phase in purple broth, washed once in phosphate buffered saline (PBS) (39)and normalized to an OD600 value of 0.7. Five ml of normalized cells were pelleted, resuspended in 2.5 ml arginine decarboxylase assay medium [1 g L-arginine, 0.05 g bromocresol green, 90 g NaCl, and 3 ml Triton X-100 per liter of distilled water (adjusted to pH 3.4)] and vortexed for 30 s. Assay tubes were incubated at 37° C. for 5-30 minutes, scored and photographed.

Acid resistance assays. Acid resistance was determined essentially as described previously (43, 44) with the following modifications. Strains were grown overnight to stationary phase in minimal EGA medium at pH 7.0 (37) or in TSB with 0.4% glucose. Cultures were normalized to the same OD600, then pelleted and washed once in EGA medium, pH 7.0 containing no growth supplements. Cells were pelleted a second time and resuspended at a density of 1×109 CFU/ml in EGA medium containing 1 mM L-arginine at pH 3.0, 2.5 or 2.0. Low pH challenge was conducted at 37° C. and samples were collected immediately after resuspension (t=0) and hourly for 4 h. Samples were serially diluted and plated onto LB agar to assess viability during challenge.

Statistical analyses. All statistical analyses were performed using GraphPad Prism version 5.04 for Windows(GraphPad Software, San Diego, Calif. USA, www.graphpad.com). Survival curves for 4-hour acid resistance assays were compared using two-way repeated measures (mixed model) ANOVA with Bonferroni's post-test. Data from 1 h acid resistance challenges were compared using the paired t test.

RESULTS Example 1 Comparison of adiA Regulation from Arabinose- and Rhamnose-Regulated Promoters

Genes encoding the arginine decarboxylase system are normally expressed in Salmonella only under anaerobic conditions (3, 33). To allow expression during aerobic growth, we constructed two conditional adiA mutants that resulted in strains in which adiA expression was regulated by either the araBAD or rhaBAD promoter. For safety, the sugar-regulated adiA constructions were introduced into S. Typhi strain χ11548, which carries an attenuating ΔaroD mutation (17, 45).Thus, in strains χ11552 (ΔaroD ParaBAD adiA) and χ11564 (ΔaroD PrhaBAD adiA), adiA expression should be responsive to the levels of exogenous arabinose or rhamnose, respectively. In the absence of the regulating sugar, both strains expressed low levels of adiA transcript consistent with background levels observed in Ty2 cultured under non-inducing conditions for adiA (FIG. 2A). Both strains increased production of the adiA mRNA transcript when 0.1% (10−1%) of the appropriate sugar was added. However, at lower sugar concentrations, the two strains behaved differently. Strain χ11552 (ParaBAD adiA) continued to express elevated amounts of adiA mRNA at arabinose concentrations as low as 0.0015 (10−3%). Only when the arabinose concentration fell below 0.001% (10−3%) did the amount of adiA transcript return to background levels. In contrast, strain χ11564 (PrhaBAD adiA) expressed adiA transcript only in the presence of 0.1% (10−1%) rhamnose and produced background levels of adiA mRNA at lower rhamnose concentrations.

AdiA protein synthesis and enzyme activity levels presented a pattern similar to the mRNA. χ11552 (ParaBAD adiA) synthesized AdiA over a wide range of arabinose concentrations (10−1-10−4% arabinose), while in χ11564 (PrhaBAD adiA) AdiA was detected over a narrower range of rhamnose concentrations (10−1-10−2% rhamnose) (FIG. 2B). While the highest amounts of AdiA in both strains were observed at the arabinose and rhamnose concentrations that increased levels of adiA transcript, small amounts of AdiA were also detected at sugar concentrations that did not produce a measurable increase in the amount of adiA transcript present (10−4% arabinose for χ11552 and 10−2% rhamnose for χ11564), which could reflect differences in the sensitivity of the two assays or to differences in the stability of the adiA mRNA transcript and AdiA protein.

AdiA activity was evaluated by decarboxylase assay, in which active enzyme raises the assay medium pH above 5.0, resulting in a color change from yellow-green (negative) to blue (positive). Arginine decarboxylase activity (FIG. 2C) correlated with detection of AdiA on the western blot (FIG. 2B) and could be detected in χ11552 (ParaBAD adiA) cultures grown in the presence of arabinose concentrations as low as 10−3%. An intermediate reaction suggestive of low levels of enzyme activity was observed at 10−4% arabinose. In contrast, arginine decarboxylase activity was observed in χ11564 (PrhaBAD adiA) only at rhamnose concentrations greater than 10−2%. Because the rhamnose-regulated PrhaBAD promoter provided tighter control over AdiA synthesis and activity than the arabinose-regulated ParaBAD promoter, we selected the ΔPadiA:TT rhaSR PrhaBAD adiA mutation for further studies.

Example 2 Co-Regulation of adiA and adiC is Necessary for Survival During pH 3.0 Challenge

Our goal in introducing the PrhaBAD adiA construct into S. Typhi was to provide arginine-dependent acid resistance when cells were grown under conditions when this system is not normally induced (non-inducing conditions). To test this, we performed low pH challenges on cells grown aerobically in minimal EGA medium.

However, while χ11564 (ΔaroD PrhaBAD adiA) exhibited rhamnose-regulatable arginine decarboxylase activity under these conditions (data not shown), the survival profile of χ11564 (ΔaroD PrhaBAD adiA) at pH 3.0 did not differ from that of Ty2 or its parent strain χ11548 (ΔaroD) (FIG. 3). This is likely due to the fact that arginine-dependent acid resistance requires substrate::product exchange by AdiC in addition to proton consumption by AdiA (29). Based on this, we reasoned that the PrhaBAD promoter in strain χ11564 (ΔaroD PrhaBAD adiA) does not drive adiC expression due to the presence of a transcriptional terminator downstream of adiA and the intervening adiY gene. Thus, it is likely that adiC expression remains under the control of its native promoter and is not induced by rhamnose (FIG. 1). To co-regulate expression of both adiA and adiC, the intergenic region between the two genes, including the regulatory gene adiYand the adiC promoter, was deleted, resulting in the fusion of adiA and adiC into a single operon under the control of the native adiA promoter, resulting in strain χ11636 (adiAC) (FIG. 1). The sensitivity of χ11636 to pH 3.0 challenge was not significantly different from Ty2 and χ11548 (ΔaroD)(p=0.327) (FIG. 3). The adiAC operon fusion was then placed under transcriptional control of PrhaBAD adiA resulting in strain χ11568 (ΔaroD PrhaBAD adiAC). When grown with 0.1% rhamnose, strain χ11568 was highly resistant to pH 3.0 challenge (FIG. 3), displaying a 1,000 to10,000-fold increase over Ty2 in the number of viable cells present at all time points during challenge (p<0.0001).

Example 3 Survival of Strain χ11568 During pH 3 Challenge is Rhamnose- and Arginine-Dependent

A number of acid resistance and acid tolerance mechanisms have been described in stationary phase Salmonella. To confirm that the acid-resistant phenotype of χ11568 (ΔaroD PrhaBAD adiAC) was attributable to the rhamnose-regulated arginine decarboxylase system the strain was tested for survival at pH 3.0 in the absence of rhamnose and arginine. When cultured in minimal EGA medium without rhamnose, χ11568 (ΔaroD PrhaBAD adiAC) displayed a survival profile indistinguishable from the wild-type Ty2 and parent strain χ11548 (ΔaroD) during pH 3.0 challenge (FIG. 4A). Adding rhamnose to the EGA culture medium restored the acid resistance of χ11568 (ΔaroD PrhaBAD adiAC), resulting in a 1,000- to 10,000-fold higher survival rate when rhamnose was provided (p=0.001).

The acid resistance of χ11568 (ΔaroD PrhaBAD adiAC) also depended on the presence of arginine in the challenge medium (FIG. 4B). The percentage of viable χ11568 (ΔaroD PrhaBAD adiAC) cells during challenge rapidly declined over 4 hours in the absence of arginine, with few survivors detected after the first two hours. However, cells that were challenged in the presence of 1 mM arginine showed a marked increase in survival (p=0.003). Interestingly, removing arginine from the challenge medium also impaired survival of Ty2 (p=0.022), even though arginine decarboxylase activity was not detected under these culture conditions (data not shown).

The rhamnose-regulated arginine decarboxylase system provided a substantial benefit to S. Typhi survival during pH 2.5 challenge (FIG. 5). After 1 hour at pH 2.5, χ11568 (ΔaroD PrhaBAD adiAC) survived not only significantly better than its ΔaroD parent (χ11548) (ΔaroD)(p=0.010), but also significantly better than the wild type (p=0.010) and arginine decarboxylase knockout χ11500 (p=0.035). Of the 109 CFU that were challenged, over 105 CFU of χ11568(ΔaroD PrhaBAD adiAC) remained viable after one hour. Despite this high level of survival and although previous reports indicated that the arginine decarboxylase system could protect Salmonella Typhimurium for greater than two hours at pH 2.5 (3), we did not detect any S. Typhi survivors after the first hour of challenge (data not shown).

Example 4 Rescue of ΔphoPQ and ΔPfur::TT araC ParaBAD fur Mutants at pH 3 and 2.5

Because the rhamnose-regulated arginine decarboxylase system conferred such a high degree of acid resistance on χ11568(ΔaroD PrhaBAD adiAC) when grown aerobically in minimal media (non-inducing conditions) (FIG. 3), we tested the ability of this system to rescue two acid sensitive strains of S. Typhi—a phoPQ mutant (χ8444) and a conditional fur mutant (χ11118). These mutations result in well-characterized acid sensitivities. Introducing the PrhaBAD adiAC construct into strains χ8444 (ΔphoPQ) and χ11118 (ParaBAD fur) resulted in strains χ11622 and χ11623, respectively, that exhibited rhamnose-dependent arginine decarboxylase synthesis as described for χ11568 (ΔaroD PrhaBAD adiAC) (FIG. 2C and data not shown).

To evaluate the ability of the rhamnose-regulated arginine decarboxylase system to rescue ΔphoPQ, strain χ11622 (ΔphoPQ PrhaBAD adiAC) was grown in minimal EGA medium to stationary phase at pH 7.0 in the presence of 0.1% rhamnose and then were challenged at either pH 3.0 or pH 2.5. Under these growth conditions, the ΔphoPQ mutant χ8444 displayed a similar survival profile as the wild-type Ty2 (p=0.996) (FIG. 6A). In contrast, the survival of strainχ11622 (ΔphoPQ PrhaBAD adiAC) was significantly greater than its parent strain χ8444 (ΔphoPQ) or the wild-type Ty2 (p=0.034). Further, strain χ11622 (ΔphoPQ PrhaBAD adiAC) was significantly more resistant to a 1 h challenge at pH 2.5 than any of the other S. Typhi strains (p=0.009 for χ8444; 0.010 for Ty2 and 0.0232 for χ11500—ΔadiA-adiC) (FIG. 6B).

We next examined the impact of the arginine decarboxylase system on a fur mutant (χ11623 (ParaBAD fur PrhaBAD adiAC)). For this analysis, we utilized the conditional fur mutant χ11118 (ParaBAD fur) in which fur expression can be induced by addition of arabinose to the culture medium (36). However, western blot analysis indicated that, while Fur synthesis was induced by arabinose, the level of Fur produced in strain χ11118 (ParaBAD fur) was much less than the amount produced by Ty2 (FIG. 7A). Consistent with the low level of arabinose-induced Fur production, the survival of pH 3.0-challenged cells grown in the presence of 0.2% arabinose did not differ from that of cells grown in the absence of arabinose (p=0.934) (FIG. 7B). Since χ11118 fur) (ParaBAD had the phenotype of a fur knockout in the acid resistance assay irrespective of the arabinose concentration, we decided to work with it and the rhamnose-regulated arginine decarboxylase daughter strain (χ11623—ParaBAD fur PrhaBAD adiAC) only in the absence of arabinose. We observed no difference in survival at pH 3.0 between the wild-type Ty2, the arginine decarboxylase knockout χ11500 (ΔadiA-adiC) and χ11118 (ParaBAD fur) in our assay (p=0.392) (FIG. 7C). Strain χ11623 (ParaBAD fur PrhaBAD adiAC) displayed greater survival than its parent χ11118 (ParaBAD fur) for the first hour of challenge at pH 3.0 (p=0.010) indicating that the arginine decarboxylase system could rescue this fur mutant to some degree. However, there was no difference between χ11623 (ParaBAD fur PrhaBAD adiAC)and χ11118 (ParaBAD fur) for the later time points (p=0.337). A similar trend was observed at pH 2.5 (FIG. 7D). χ11623 (ParaBAD fur PrhaBAD adiAC) survived significantly better after 1 hour at pH 2.5 than its acid-sensitive parent χ11118 (ParaBAD fur) (p=0.013), but it was not significantly different from the wild-type Ty2 (p=0.242) or the arginine decarboxylase mutant χ11500 (ΔadiA-adiC) (p=0.122).

Example 5 Rhamnose-Dependent Acid Resistance is Equivalent to Acid Resistance in Cells grown Under Decarboxylase-Inducing Conditions

We next compared the level of acid resistance afforded by the rhamnose-regulated system to the acid resistance provided by the native system. Strains were grown anaerobically in unbuffered rich medium where the pH was allowed to fall below pH 5.0 during growth (native inducing conditions). Strains were supplied with 0.1% (or 0.4%, see below) rhamnose during growth. Cells were then challenged in EGA medium with 1 mM arginine at pH 3.0 or 2.5. The arginine decarboxylase deletion mutant χ11500 (ΔadiA-adiC) rapidly succumbed to challenge at both pH 3.0 and 2.5 (FIG. 8A, 8B). Ty2 and χ11548 (ΔaroD) displayed a high degree of acid resistance at pH 3.0 (greater than 104 CFU/ml were viable after 4 hours), but succumbed to pH 2.5 after 2 hours. In contrast, the highly acid resistant Shigella flexneri strain 2457T exhibited >70% viability for 4 hours at pH 3.0 and viability only decreased by one log after 4 hours at pH 2.5. Strain χ11568 (ΔaroD PrhaBAD adiAC) was not able to match the acid resistance profile of Shigella, although it displayed a survival profile equivalent to the S. Typhi Ty2 and χ11548(ΔaroD) grown under these conditions (p=0.210). These results indicate that the rhamnose-regulated system provides a level of acid resistance equivalent to the acid resistance afforded by the native system.

Under the native ad/A-inducing conditions, both phoPQ mutants, χ8444 (ΔphoPQ) andχ11622 (ΔphoPQ PrhaBAD adiAC), behaved similarly to Ty2 during pH 3.0 challenge (p=0.498) (FIG. 8C). This was in contrast to the arginine decarboxylase deletion strain χ11500 (ΔadiA-adiC), which survived significantly less well than the phoPQ strains at pH 3.0 (p=0.018). No difference was observed in survival at pH 3.0 between χ8444 (ΔphoPQ) (which utilized the native arginine decarboxylase system) and χ11622 (ΔphoPQ PrhaBAD adiAC) (which utilized the rhamnose-regulated system) (p=0.628). A similar pattern was observed at pH 2.5 (FIG. 8D). No difference was observed between the native arginine decarboxylase system in χ8444 (ΔphoPQ) and the rhamnose-regulated system in χ11622 (ΔphoPQ PrhaBAD adiAC) (p=0.702).

Unlike χ11568 (ΔaroD PrhaBAD adiAC) and χ11622 (ΔphoPQ PrhaBAD adiAC), the conditional fur mutant χ11623(ParaBAD fur PrhaBAD adiAC) did not produce detectable arginine decarboxylase activity in the presence of 0.1% rhamnose when cultured in anaerobic rich medium. Arginine decarboxylase activity was detectable only when the rhamnose concentration was increased to 0.4% (data not shown). Therefore, the concentration of rhamnose present in this assay was raised to 0.4% for χ11623(ParaBAD fur PrhaBAD adiAC). In contrast to the phoPQ mutants, the fur mutants χ11118 (ParaBAD fur) and χ11623 (ParaBAD fur PrhaBAD adiAC) were significantly more sensitive to pH 3.0 than the wild-type Ty2 (FIG. 8E). χ11118 (ParaBAD fur) and χ11623 (ParaBAD fur PrhaBAD adiAC) displayed a survival profile more similar to that of χ11500 (ΔadiA-adiC) (p=0.392) than Ty2 (p=0.0006). However, there was no observable difference in survival between χ11118 (ParaBAD fur) and χ11623 (ParaBAD fur PrhaBAD adiAC) at either pH 3.0 (p=0.332) or pH2.5 (p=0.882) (FIG. 8F). These results indicate that for both the ΔphoPQ and ParaBAD fur mutants, the rhamnose-regulated arginine decarboxylase system and the native system provided equivalent levels of acid resistance.

Discussion of Examples 1 to 5

In this work, we constructed an acid resistance system whose expression and activity responded to the presence of a single sugar, either arabinose or rhamnose. Both adiA and adiC expression were required for acid resistance (FIG. 3) and the rhamnose-regulated PrhaBAD promoter provided tighter control over adiA expression than the arabinose-regulated ParaBAD promoter (FIG. 2). The level of acid resistance provided by PrhaBAD adiAC grown with rhamnose under decarboxylase-inducing conditions was equivalent to the level of acid resistance observed with the native arginine decarboxylase system grown under the same conditions. However, the rhamnose-regulated adiAC system was regulatable in cells otherwise unprepared for low pH challenge, thus our rhamnose-regulated system significantly improved the survival of acid-unadapted aroD, phoPQ and fur mutants at pH 3 and 2.5 (FIGS. 3, 6 and 7).

Comparison of the arabinose-regulated ParaBAD and rhamnose-regulated PrhaBAD promoters indicated that PrhaBAD was less sensitive to its regulatory sugar than ParaBAD. At high concentrations of arabinose or rhamnose (0.1%), both promoters were active. The two promoters drove production of essentially equivalent amounts of adiA transcript at this concentration, consistent with previous results (46). As the amount of regulatory sugar present in the culture was decreased, the activity of the two promoters decreased differentially. While background levels of transcription were detected from PrhaBAD at rhamnose concentrations below 0.01% (10−2%), ParaBAD continued to function until the arabinose concentration fell below 0.0001° /o (10−4%). Some of this difference may be attributable to the “leakiness” of the ParaBAD promoter (47, 48). However, we used a modified sequence for ParaBAD, which exhibits tightly controlled arabinose-dependent transcription(49). Since rhamnose is transported into Salmonella more efficiently than arabinose, differences in sugar uptake are unlikely to be the cause of this discrepancy (50, 51). It is possible that rhamnose is converted to a non-inducing state following transport, because while neither arabinose nor rhamnose can be fermented by S. Typhi (52), the rhaB and rhaA genes are intact and their gene products may be able to act on the transported rhamnose. Another explanation is the previously observed slow rate of transcription from the PrhaBAD promoter (53) resulting from the cascade of regulation by RhaR and RhaS on PrhaBAD (51, 54) The reduced sensitivity of the PrhaBAD promoter makes it an ideal choice to regulate the arginine decarboxylase system since it allows tight control of gene expression even in media containing trace amounts of rhamnose, such as LB and TSB.

Rhamnose-dependent acid resistance in S. Typhi depended on three things—the presence of rhamnose in the culture medium, the presence of arginine in the challenge medium, and the fusion of adiA and adiC into an operon under the control of PrhaBAD. The absence of any of these components resulted in rapid cell death at pH 3.0 (FIGS. 3 and 4). The requirement for co-regulation of adiA and adiC is consistent with the known mechanism of the arginine decarboxylase system. Although AdiA is the enzyme that consumes protons and is responsible for raising the intracellular pH during low pH challenge (55), AdiC is required to import a continuous supply of arginine substrate from the periplasm (29). Deletions of either adiA or adiC abolish arginine-dependent acid resistance (3). The arginine requirement for survival at low pH confirms that the acid resistance we observed was due to the Salmonella arginine decarboxylase system and not to the stationary phase acid tolerance response or the oxidative acid resistance response (AR1), as neither of these systems requires arginine (2, 43). Interestingly, even though cells were cultured in aerobic minimal medium to prevent induction of the native arginine decarboxylase system in wild-type S. Typhi strain Ty2 (3), we observed an arginine-dependent increase in resistance to pH 3 challenge (FIG. 4B). This suggests that arginine decarboxylase is expressed at low levels in S. Typhi during stationary phase culture—a conclusion consistent with the low, but detectable, levels of adiA transcript observed in Ty2.

Substituting the rhamnose promoter PrhaBAD for the native adiA promoter did not affect the degree of acid resistance afforded at low pH. Strains with rhamnose-dependent acid resistance survived low pH challenge as well as their respective parent strain cultured under native decarboxylase-inducing conditions. Cells remained viable for over 4 hours at pH 3.0 and for at least 2 hours at pH 2.5. No protection was afforded against pH 2.0 challenge (data not shown), consistent with previous reports for Salmonella (2, 56). By substituting the rhamnose promoter for the native arginine decarboxylase promoter, we were able to rescue χ11568 (ΔaroD PrhaBAD ad/AC), a derivative of the rpoS mutant strain Ty2, from low pH challenge via rhamnose induction of the arginine decarboxylase system (FIG. 3). χ11568 (ΔaroD PrhaBAD adiAC) cells grown under non-inducing conditions (aerobic minimal medium, pH 7) remained viable for over 4 hours at pH 3 when rhamnose was included in the growth medium. This indicates that the activity of the arginine decarboxylase system alone is sufficient for low pH survival in S. Typhi. However, χ11568 (ΔaroD PrhaBAD adiAC) cultured under decarboxylase-inducing conditions (anaerobic rich medium with 0.4% glucose) approximately 100-fold more cells survived pH 3 challenge than when it was cultured aerobically in minimal medium (compare FIG. 3 and FIG. 7A). This is because the growth conditions necessary to induce arginine decarboxylase production in wild-type Salmonella simultaneously induce the stationary phase acid tolerance response (3, 6, 57). The disparity in survival rates between cells cultured aerobically in minimal medium and cells cultured under fermentative conditions underscore the comprehensive nature of the acid response in Salmonella—maximum resistance to low pH is achieved by use of a variety of strategies to counter the effects of low pH.

The rhamnose regulated arginine decarboxylase system was also able to rescue a phoPQ mutant from low pH challenge (FIG. 6). The rhamnose-regulated arginine decarboxylase system in strain χ11622 (ΔphoPQ PrhaBAD adiAC) provided approximately a 1000-fold increase in viability at pH 3.0 over the parent phoPQ mutant (χ8444) when cells were grown aerobically in minimal medium (cells unprepared for low pH). At pH 2.5, the viability of χ11622 (ΔphoPQ PrhaBAD adiAC) after 1 hour exceeded not only that of the parent phoPQ mutant, but also that of the wild-type Ty2. The success of our system at rescuing the phoPQ mutant may be due to two reasons. First, the strains were challenged during stationary phase, when PhoP/PhoQ are less important for acid tolerance (58). Second, a mutation in the phoPQ locus causes a very well characterized sensitivity to inorganic acid (8). At low pH, inorganic acids exist almost exclusively in their dissociated state (free proton with conjugate base), which makes them ideal candidates for neutralization by arginine decarboxylase (it will consume the free protons in the decarboxylase reaction, which immediately raises the intracellular pH and stops further cytoplasmic damage by the free protons). Thus the arginine decarboxylase system is well-poised to compensate for the acid sensitivity imposed by a phoPQ mutation.

Survival of the ParaBAD fur mutant (χ11623) was enhanced by PrhaBAD adiAC, although the improvement was not as great as it was for the ΔaroD and ΔphoPQ mutants. The addition of the rhamnose-regulated arginine decarboxylase system improved viability during pH 3 and pH 2.5 challenges, but unlike the phoPQ mutant, the fur mutant only benefitted during the first hour of challenge (FIG. 7). The reason for the difficulty of rescue may be two-fold. First, unlike phoPQ mutants, fur mutants are sensitive to organic acids. Inorganic acids such as HCl and organic acids behave quite differently inside the cell, due to differences in their dissociation constants. Our EGA challenge medium contained not only the inorganic acid HCl, but also 10 mM citric acid (37). It is possible that the consumption of free protons by the arginine decarboxylase system is less effective at countering the effects of an organic acid such as citric acid than the strong inorganic acid HCl (8, 23, 37, 59). Second, because the APfur::TT araC ParaBAD fur mutation was introduced into Ty2, the strain also contains an rpoS mutation. RpoS and Fur jointly regulate a number of key effectors responsible for protection against organic acid. Thus, the combination of fur and rpoS mutations may have rendered χ11623 much more sensitive to acid than the rpoS mutation alone or the combination of phoPQ and rpoS (4, 6). Finally, the Pfur mutation may have altered the ability of χ11623 to transport rhamnose, as it required four times the concentration of rhamnose to induce arginine decarboxylase activity as the aroD and phoPQ mutants. Fur is known to regulate expression of a number of outer membrane proteins and other genes that may influence surface structure (60). Thus, it is possible that membrane perturbations due to the lack of Fur in the cell may have resulted in a reduction in rhamnose transport activity by RhaT.

The construction of the rhamnose-regulated arginine decarboxylase system allowed us to increase the acid resistance of S. Typhi (to pH 2.5) on demand. Importantly, aerobically grown vaccine strains were protected from pH 3 and pH 2.5. Since the low pH of the gastric environment poses a significant threat to the success of any live attenuated Salmonella vaccine, the rhamnose-regulated arginine decarboxylase system represents a novel means to augment survival in this in vivo compartment. Also, because low gastric pH is an important virulence signal, the ability to administer vaccines without stomach pH neutralization may also improve vaccine performance in the host.

TABLE 1 Strains and plasmids used in this study Strain or Derivation or plasmid Genotypea Source E. coli strains BL21 (DE3) F ompT hsdSB(rB mB) gal dcm (DE3) Novagen χ7213 thr-1 leuB6 fhuA21 lacY1 glnV44 recA1 ΔasdA4 Δ(zhf-2::Tn10) (61) thi-1 RP4-2-Tc::Mu [λpir] χ7573 Wild type O157:H7 strain 278F2 J. Giron S. Typhi strains χ3769(Ty2) Wild-type, cys trp rpoS (62) χ8444 ΔphoPQ (63) χ11118 ΔPfur::TT araC ParaBAD fur Ty2 χ11500 Δ(adiA-adiC) Ty2 χ11548 ΔaroD Ty2 χ11552 ΔaroD ΔPadiA::TT araC ParaBAD adiA χ11548 χ11564 ΔaroD ΔPadiA::TT rhaSR PrhaBADadiA χ11548 χ11568 ΔaroD ΔPadiA::TT rhaSR PrhaBAD adiA Δ(PadiY-adiY-PadiC) adiC χ11564 χ11622 ΔphoPQ ΔPadiA::TT rhaSR PrhaBAD adiA Δ(PadiY-adiY-PadiC) adiC χ8444 χ11623 ΔPfur::TT araC ParaBAD fur ΔPadiA::TT rhaSR PrhaBAD adiA Δ(PadiY-adiY- χ11118 PadiC) adiC χ11636 ΔaroD Δ(PadiY-adiY-PadiC) adiC χ11548 χ11742 Δfur Ty2 Shigella flexneri strains 2457T S. flexneri 2a, wild-type, Pcr+ Mal λr (64) Plasmids pET28a Protein synthesis vector, T7 promoter; Kanr Novagen pJET1.2 Commercial cloning vector, pMB1 ori, Apr Thermo Scientific pUC18 Commercial cloning vector, pMB1 ori, Apr Lab stock pYA3700 Vector encoding the tightly regulated TT araC ParaBAD cassette (65, 66) pYA4181 Suicide vector to generate the ΔPfur::TT araC ParaBAD fur mutation (36) pYA4278 Suicide vector, sacB mobRP4 oriR6K; Cmr (67) pYA4895 Suicide vector to generate the ΔaroD mutation pYA4278 pYA5066 Suicide vector to generate the Δ(adiA-adiC) mutation pYA4278 pYA5072 Suicide vector to generate the Δ(PadiY-adiY-PadiC) adiC mutation pYA4278 pYA5075 Intermediate vector for the creation of ΔPadiA::TT araC ParaBAD adiA pYA3700 pYA5081 Suicide vector specifying the tightly regulated rhaSR PrhaBAD (68) cassette pYA5085 Protein synthesis vector with N-terminal His-tag on AdiA pET28a pYA5089 Suicide vector to generate the ΔPadiA::TT araC ParaBAD adiA mutation pYA4278, pYA5075 pYA5093 Suicide vector to generate the ΔPadiA::TT rhaSR Prhabad adiA pYA5089, mutation pYA5081 pYA5116 Suicide vector to generate ΔendA pYA5103 pYA5119 Suicide vector to generate ΔendA::clcA pYA5116 pYA5120 Suicide vector to generate ΔcysG::TT araC PBAD gadBC pYA5115 aIn genotype descriptions, the subscripted number refers to a composite deletion and insertion of the indicated gene. P, promoter; TT, T4 ip III transcription terminator; Cmr, chloramphenicol resistance; Kanr, kanamycin resistance.

TABLE 2 PCR primers used in the study Name Sequence (5′-3′) Relevant mutation Adi-1 CCGGTACCGATGGGAATATTCCAGCG Δ(adiA-adiC) Adi-2 CCGGATCCCTTTTACCCGGTTGTG Δ(adiA-adiC) Adi-3 CCGGATCCCCACGTGTAGTTAATGTTATCGC Δ(adiA-adiC) Adi-4 CCAAGCTTGGCAATCACGGCTGCC Δ(adiA-adiC) Adi-5 CATGGCATGCCGAATGAGCAAATTC ΔPadiA::TT araC ParaBAD adiA Adi-6 CCGGAGATCTTGATAGTGGTATCCGGCTT ΔPadiA::TT araC ParaBAD adiA Adi-7 CATGGGTACCAGGAGGTAAAAGATGATGAAAG ΔPadiA::TT araC ParaBAD adiA Adi-8 CATGGAGCTCCGCCATAATAATCGTG ΔPadiA::TT araC ParaBAD adiA Adi-9 CATAGCCGTACCATGCTTCGTCG Regulated adiA constructs Adi-10 GCGCTCTAGACGCACCACCGACTTCCAG Δ(Padiy-adiY-PadiC) adiC Adi-11 GTATCATACCCCCTCAGAATGTTGCAGCAATACTCAG Δ(Padiy-adiY-PadiC) adiC Adi-12 TTCCCTGAGTATTGCTGCAACATTCTGAGGGGGTAT Δ(Padiy-adiY-PadiC) adiC G Adi-13 GCATGGATCCCCAGAACCAGCCGAAG Δ(Padiy-adiY-PadiC) adiC Adi-14 CCGGTACCCGAACTCCGTTATTCCTTAC Δ(Padiy-adiY-PadiC) adiC Adi-15 CCAAGCTTCAGATAGCCGACGCC Δ(Padiy-adiY-PadiC) adiC Ara-1 GATTAGCGGATCCTACCTGACGC araC ParaBAD Aro-1 CCCGGGTGCTGGCTGAACAGTTCCTCGAG ΔaroD Aro-2 CCGGATCCTCCGGCATTATGCAGGCGTCG ΔaroD Aro-3 CCGGATCCGCGTGTCCTGTCAGTTTTTTTTCTTCTC ΔaroD Aro-4 TCTAGATCTCCGCATGGGTACATGAAGTTCCGG ΔaroD Fur-1 ACATGCATGCTGTGACTGGGATGACTTCTTCCCG ΔPfur::TT araC PBAD fur Fur-2 TCCCCCGGGCACTTTTCCGCAATCAAGGCAG ΔPfur::TT araC PBAD fur Rha-1 GCACTCTAGATTAATCTTTCTGCGAATTG ΔPadiA::TT rhaSR PrhaBADadiA Rha-2 GCATCTCGAGGCTGAATTTCATTAC ΔPadiA::TT rhaSR PrhaBADadiA Rha-3 TCAGTAACGAGAAGGTCGCG rhaSR PrhaBAD SQ-1 GCTGAAATATGACTCCACTCAC gapA SQ-2 CGTCAACACCAACTTCGTC gapA SQ-3 ACCGACTTCCAGATTATGTTCC adiA SQ-4 CGTGTTGATCAGCGTTCCC adiA Gad-1 GGCCGAGCTCCTATCCTGCCGCAAACC ΔcysG::TT araC PBAD gadBC Gad-2 CAATTCTAGGATAGAATAATAAAGCGGCCGCGACATT ΔcysG::TT araC PBAD gadBC ACCCCTTAATGGTTG Gad-3 GTTTTTTTGGGCTAGCCTCGAGAGGAGTTTAAAATGG ΔcysG::TT araC PBAD gadBC ATAAGAAG Gad-4 GAATAACAGGGCTTTATTTTAAGATCTAAAAAGGGAG ΔcysG::TT araC PBAD gadBC CGATGAAT Gad-5 CATCGCTCCCTTTTTAGATCTGCCCTGTTATTCAGGG ΔcysG::TT araC PBAD gadBC CTTTA Gad-6 GCATGGTACCCGACCAATGCGGCAAC ΔcysG::TT araC PBAD gadBC Gad-7 CCCCCTCGAGGGTATGTTTAAAGCTGTTC ΔcysG::TT araC PBAD gadBC Gad-8 GGCACCGTTCGTCGCCCCGGATATCG gadBC seq Gad-9 CAGGTAAAGCTAAGCAGCTCACATTAC gadBC seq Gad-10 CGTTCTGATGTCCCATGTGGCACCGG gadBC seq Ara-1 CATTAAGGGGTAATGTCGCGGCCGCTTTATTATTCTA ΔcysG::TT araC PBAD gadBC TCCTAGAATTGTG Ara-2 CTTCTTATCCATTTTAAACTCCTCTCGAGGCTAGCCC ΔcysG::TT araC PBAD gadBC AAAAAAACG Ara-3 GATTAGCGGATCCTACCTGACGC ΔcysG::TT araC PBAD gadBC

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Example 6 Sugar-Inducible Amino Acid Decarboxylase Systems

Glutamate Decarboxylase.

The glutamate decarboxylase (GAD) system of E. coli O157:H7 is composed of two homologous decarboxylases (GadA and GadB) and a glutamate/γ-aminobutyric acid antiporter (GadC) (15). GadA and GadB are biochemically indistinguishable and only one is required for survival at pH 2.5 in E. coli. However, both are required for survival at pH 2 (5, 6). In E. coli, this system maintains an internal pH between 4-5 (14). Based on our findings that the antiporter is required for acid resistance in the AdiA system, we took advantage of the fact that gadB and gadC are co-transcribed from a single operon (5) (gadA is located at a distant site on the chromosome (15)) by cloning the gadBC operon and placing it under transcriptional control of the araC PBAD promoter. To accomplish this, we engineered an operon substitution mutation into the cysG locus: ΔcysG::TT araC PBAD gadBC. We fused the arabinose-regulator cassette containing araC, the araC promoter, and the PBAD promoter to the flanking region upstream of the cysG locus in Salmonella Typhi Ty2 (FIG. 9). The upstream flanking region was amplified by PCR from Ty2 using primers Gad-1 and -2 (Table 2); the araC cassette was amplified by PCR from plasmid pYA3700 using primers Ara-1 and -2. The two DNA segments were joined by overlap PCR and re-amplified with primers Gad-1 and Ara-2. The overlap PCR product was ligated into pUC18 at the Sal I/XhoI and SacI sites to produce the intermediate vector pYA5105. The strong transcription terminator T4 ip III placed between the upstream nirC gene and araC prevents expression of antisense RNA as well as transcription due to the cysG promoter that remains within the coding sequence of nirC.

We fused the gadBC operon with the cysG downstream flanking region. Flanking DNA was amplified by PCR from Ty2 using primers Gad-3 and -4; the gadBC operon was amplified from enterohemorrhagic E. coli strain χ7573 using primers Gad-5 and -6. The two DNA segments were joined by overlap PCR and re-amplified with primers Gad-3 and -6. The overlap product was ligated into pCR2.1 TOPO to generate pYA5101. The upstream flanking region-araC fusion from pYA5105 and the gadBC operon-downstream flanking region fusion from pYA5101 were amplified using Gad-1/Ara-2 and Gad-3/ -6 respectively (see above) and joined by overlap PCR and re-amplified with primers Gad-1 and -6. This PCR product was ligated into pJET1.2 to produce intermediate vector, pYA5115. The intergenic region between the araC cassette and gadBC operon was confirmed by PCR primers, Ara-3 and Gad-7. We confirmed the sequence integrity of the gadBC operon using primers Gad-8, -9 and -10. The fusion product from pYA5115 was amplified with primers Gad-1 and -6 and ligated into pYA4278 at the AhdI sites, generating the suicide vector pYA5120. pYA5120 was introduced into Salmonella Typhi Ty2 phoPQ mutant, χ8444, by conjugation to produce χ11760. The generation and activity of E. coli decarboxylase within Salmonella was verified by Western blot, acid resistance survival and glutamate decarboxylase assay.

Using pYA5120, the araC PBAD gadBC construct (FIG. 9) was introduced into several S. Typhi strains, each carrying a mutation known to attenuate Salmonella, ΔguaBA (19), ΔphoPQ (9, 10) or Δfur (4, 20). Note that Salmonella strains with mutations in either phoPQ (8) or fur (7) are extremely acid sensitive. In addition, preliminary results indicate that our ΔguaBA S. Typhi mutant is also more sensitive to acid shock than its Ty2 parent (data not shown). Although this phenotype has not been documented in the literature, it is interesting to note that a previous study reported that in E. coli, GuaB synthesis is induced by exposure to low pH (21). The araC PBAD gadBC system confers sugar-inducible acid resistance to all three mutant strains when S. Typhi cells are grown aerobically at pH 7.0 (FIG. 10). In fact, the survival of strains carrying this system was greater than wild-type Ty2 grown under the same conditions.

Low gastric pH mouse model. While In vitro acid resistance assays provide good preliminary information, an animal model will give us a better idea of how our strains will behave in the clinic. As mentioned above, the gastric environment of a fasted mouse is around pH 4 (12) compared to a fasted human, whose stomach pH is around 2 (17). This difference can have a profound effect on Salmonella survival and could provide data that does not reflect what will happen in humans. To create a gastric pH closer to the human stomach, we took advantage of the observation that injecting mice with histamine transiently increases HCl secretion by parietal cells lining the stomach (3). Note that in this model, mice are injected with the H1 antagonist chlorpheniramine prior to injection with histamine to block an allergic reaction (3). This approach was also used in a study to establish the significance of low gastric pH as a barrier to infection (16). Based on these observations, we have adapted this model to evaluate the ability of attenuated Salmonella to transit the stomach (22). In preliminary studies, we monitored gastric pH in live mice as a function of time after histamine injection (FIG. 11). Our results indicated that the minimum pH was reached after one hour.

To validate the low gastric pH mouse model, we monitored survival of a variety of enteric pathogens in fasted mice with or without histamine injection. For these experiments, cells were grown in LB and either challenged at pH 3.0 in vitro (FIG. 12A) or used to inoculate fasted mice with or without histamine injection. In all cases, survival was less in the low pH mouse than in the fasted mouse (FIG. 12B). Not surprisingly, the Vibrio cholerae strain underwent the most killing, consistent with our in vitro results.

Survival of S. Typhi strains carrying sugar-inducible acid resistance systems in the low gastric pH mouse model. To evaluate the impact of these systems in low gastric pH mice, we set up a co-infection experiment in which strains with or without the rhamnose inducible adiAC genes carried plasmids with different antibiotic resistance markers. Strains were grown aerobically with 0.1% rhamnose and used to co-infect fasted, low gastric pH mice. Overall, induction of adiAC enhanced the survival of all strains (FIG. 13). The greatest increase in survival, 10-fold, was observed in the ΔphoPQ strain, consistent with our published in vitro results, which showed that the rhamnose-inducible adiAC system had the greatest impact on the ΔphoPQ mutant. A similar experiment was performed to evaluate strains carrying arabinose-inducible gadBC. Survival of all strains was enhanced about 10-fold (FIG. 14). Taken together, these results demonstrate that both systems are capable of increasing the survival of a variety of S. Typhi strains carrying mutations that can be used to attenuate virulence for use as human vaccines.

Lysine decarboxylase system. In addition to the adiAC and gadBC systems, resistance to acid shock can also be mediated by the AR4 system, lysine decarboxylase and lysine:cadaverine antiporter, encoded by cadA and cadB, respectively (13). In Salmonella, the cadAB genes are present as an operon and are induced by low pH and anaerobiosis, in a CadC-dependent manner when lysine is present (13). The cadAB system also plays a role in the acid tolerance response (13). This system greatly enhances the ability of Salmonella to survive an acid challenge at pH 2.3 after overnight anaerobic growth in a rich medium at pH 5 (18). Unlike adiAC or gadBC, this system can also enhance the growth of Salmonella at a moderately acidic pH of 4.5. Notably, this is observed under both aerobic and anaerobic growth conditions, which may be of additional benefit during vaccine preparation and transit through the stomach. In addition, this system lead to an increase the pH external to the cell, which may have benefits in the macrophage lysosome. To evaluate this system, we will construct S. Typhi vaccine strains (e.g ΔphoP, Δfur, ΔguaAB) in which cadAB expression is driven by a sugar-inducible promoter and characterize them in vitro, as we have done for adiAC and gadBC.

Construction of an S. Typhi vaccine strain with enhanced survival at pH 2.0. (i) Addition of gadA to strains carrying a sugar-regulated gadBC operon. In E. coli, GadA and GadB are nearly identical isoforms of glutamate decarboxylase located at different places on the chromosome (15). The gadBC operon alone is effective acid protection at pH 2.5, while both gadA and gadBC are required for maximum rates of survival at pH 2.0 (2). We observed similar results in that insertion of the gadBC into S. Typhi protects well against acid shock down to pH 2.5 (FIG. 10), but is ineffective against a pH 2.0 challenge (data not shown). Thus, it may be possible to enhance S. Typhi survival by introduction of an araC PBAD gadA construct into strains already carrying araC PBAD gadBC. The gadA gene will be inserted into the chromosome by substituting it for araE. Deletion of araE does not affect the virulence of S. Typhimurium (data not shown). The construction of the araC PBAD gadA cassette will be done essentially as we have described for araC PBAD adiA (1) and araC PBAD gadBC.

Addition of chloride channel protein ClcA from E. coli. Survival below pH 3 in E. coli is predicated on the reversal of the transmembrane potential (14). Currently no data are available to indicate whether this occurs in Salmonella, but it is likely that this will be the case. To test this, we will introduce the ClC chloride channel (eriC/clcA) from E. coli, using suicide plasmid pYA5119, as this has been shown to be an essential player in acid resistance by preventing membrane hyperpolarization at low pH (11, 14). Although S. Typhimurium and S. Typhi contain genes designated as ClC channels, alignment with the E. coli eriC reveals no significant homology and casts doubt on the ability of the Salmonella channels to serve as a substitute at low pH.

References Cited in Example 6

1. Brenneman, K. E., C. Willingham, W. Kong, R. Curtiss, 3rd, and K. L. Roland. 2013. Low pH Rescue of Acid-Sensitive Salmonella Typhi Strains by a Rhamnose-Regulated Arginine Decarboxylase System. J Bacteriol. 195:3062-3072.

2. Castanie-Cornet, M. P., T. A. Penfound, D. Smith, J. F. Elliott, and J. W. Foster. 1999. Control of acid resistance in Escherichia coli. J Bacteriol 181:3525-3535.

3. Chew, C. S., X. Chen, R. J. Bollag, C. Isales, K. H. Ding, and H. Zhang. 2008. Targeted disruption of the Lasp-1 gene is linked to increases in histamine-stimulated gastric HCl secretion. Am J Physiol Gastrointest Liver Physiol 295:G37-G44.

4. Curtiss, R., 3rd, S. Y. Wanda, B. M. Gunn, X. Zhang, S. A. Tinge, V. Ananthnarayan, H. Mo, S. Wang, and W. Kong. 2009. Salmonella strains with regulated delayed attenuation in vivo. Infect Immun.

5. De Biase, D., A. Tramonti, F. Bossa, and P. Visca. 1999. The response to stationary-phase stress conditions in Escherichia coli: role and regulation of the glutamic acid decarboxylase system. Mol Microbiol 32:1198-1211.

6. De Biase, D., A. Tramonti, R. A. John, and F. Bossa. 1996. Isolation, overexpression, and biochemical characterization of the two isoforms of glutamic acid decarboxylase from Escherichia coli. Protein Expr Purif 8:430-438.

7. Foster, J. W. 1991. Salmonella acid shock proteins are required for the adaptive acid tolerance response. J Bacteriol 173:6896-6902.

8. Foster, J. W., and H. K. Hall. 1990. Adaptive acidification tolerance response of Salmonella typhimurium. J Bacteriol 172:771-778.

9. Galan, J. E., and R. Curtiss, 3rd. 1989. Virulence and vaccine potential of phoP mutants of Salmonella Typhimurium. Microb Pathog 6:433-443.

10. Hohmann, E. L., C. A. Oletta, K. P. Killeen, and S. I. Miller. 1996. phoP/phoQ-deleted Salmonella typhi (Ty800) is a safe and immunogenic single-dose typhoid fever vaccine in volunteers. J Infect Dis 173:1408-1414.

11. Iyer, R., T. M. Iverson, A. Accardi, and C. Miller. 2002. A biological role for prokaryotic ClC chloride channels. Nature 419:715-718.

12. McConnell, E. L., A. W. Basit, and S. Murdan. 2008. Measurements of rat and mouse gastrointestinal pH, fluid and lymphoid tissue, and implications for in-vivo experiments. J Pharm Pharmacol 60:63-70.

13. Neely, M. N., and E. R. Olson. 1996. Kinetics of expression of the Escherichia coli cad operon as a function of pH and lysine. J Bacteriol 178:5522-5528.

14. Richard, H., and J. W. Foster. 2004. Escherichia coli glutamate- and arginine-dependent acid resistance systems increase internal pH and reverse transmembrane potential. J Bacteriol 186:6032-6041.

15. Smith, D. K., T. Kassam, B. Singh, and J. F. Elliott. 1992. Escherichia coli has two homologous glutamate decarboxylase genes that map to distinct loci. J Bacteriol 174:5820-5826.

16. Tennant, S. M., E. L. Hartland, T. Phumoonna, D. Lyras, J. I. Rood, R. M. Robins-Browne, and I. R. van Driel. 2008. Influence of gastric acid on susceptibility to infection with ingested bacterial pathogens. Infect Immun 76:639-645.

17. Verdu, E. F., R. Fraser, D. Armstrong, and A. L. Blum. 1994. Effects of omeprazole and lansoprazole on 24-hour intragastric pH in Helicobacter pylori-positive volunteers. Scand J Gastroenterol 29:1065-1069.

18. Viala, J. P., S. Meresse, B. Pocachard, A. A. Guilhon, L. Aussel, and F. Barras. 2011. Sensing and adaptation to low pH mediated by inducible amino acid decarboxylases in Salmonella. PLoS One 6:e22397.

19. Wang, J. Y., M. F. Pasetti, F. R. Noriega, R. J. Anderson, S. S. Wasserman, J. E. Galen, M. B. Sztein, and M. M. Levine. 2001. Construction, genotypic and phenotypic characterization, and immunogenicity of attenuated ΔguaBA Salmonella enterica serovar Typhi strain CVD 915. Infect Immun 69:4734-4741.

20. Wilmes-Riesenberg, M. R., B. Bearson, J. W. Foster, and R. Curtiss, 3rd. 1996. Role of the acid tolerance response in virulence of Salmonella typhimurium. Infect Immun 64:1085-1092.

21. Yohannes, E., D. M. Barnhart, and J. L. Slonczewski. 2004. pH-dependent catabolic protein expression during anaerobic growth of Escherichia coli K-12. J Bacteriol 186:192-199.

22. Brenneman, K. E., C. Willingham, J. Kilbourne, R. Curtiss III and K.L. Roland. 2014. A low gastric pH mouse model to evaluate live attenuated bacterial vaccines. PLoS One 9:e87411.

Example 7 Urease System

Another method to increase the acid resistance of Salmonella vaccine strains is to introduce the Ni-dependent urease system of Helicobacter pylori. The urease system is a unique acid resistance strategy, different from the others described herein. Helicobacter survives at extremely low pH not by acid resistance (temporary halt of all metabolic activities while protons are consumed and exported away from the cell), but by acid acclimation, where the cytoplasm is buffered to almost neutral pH (pH 5-7) and metabolic processes can still occur [1]. This system is more complex than the GAD or ADI systems and involves many more gene products. Urea from the gastric fluid is allowed to enter the cell at low pH by UreI (a proton-gated urea channel) [2]. The urea is then converted to ammonia by the urease (composed of UreA and UreB) [3]. The ammonia freely diffuses into the periplasm, where it is used in conjunction with H2CO3 generated by carbonic anhydrase (named HP1186) to establish a periplasmic reservoir of bicarbonate buffer [4]. This system consumes two protons per reaction cycle, as opposed to one proton per cycle in the GAD and ADI systems. The urease system has the additional advantage of consuming protons in the periplasm (as opposed to the cytoplasm), which further protects essential cytoplasmic molecules.

The urease system involves more genes than the decarboxylase systems, and for this system, it is unlikely that all of these genes must be under the control of a regulatable promoter, only the ones that directly contribute to proton consumption (ureAB and HP1186). These genes will be introduced into the Salmonella chromosome under the control of a sugar-regulatable promoter such as rhaRS-PrhaBAD

The additional components of this system, ureI—encoding the proton-gated urea channel—and ureEFGH—encoding a chaperone complex necessary to incorporate Ni ions into the urease apoenzyme [5]—will be introduced into the chromosome under the control of a constitutive promoter such as PIpp.

References Cited in Example 7

1. Sachs, G., et al., The gastric biology of Helicobacter pylori. Annu Rev

Physiol, 2003. 65: p. 349-69.

2. Rektorschek, M., et al., Acid resistance of Helicobacter pylori depends on the UreI membrane protein and an inner membrane proton barrier. Mol Microbiol, 2000. 36(1): p. 141-52.

3. Labigne, A., V. Cussac, and P. Courcoux, Shuttle cloning and nucleotide sequences of Helicobacter pylori genes responsible for urease activity. J Bacteriol, 1991. 173(6): p. 1920-31.

4. Marcus, E. A., et al., The periplasmic alpha-carbonic anhydrase activity of Helicobacter pylori is essential for acid acclimation. J Bacteriol, 2005. 187(2): p. 729-38.

5. Park, J. U., et al., Effect of the urease accessory genes on activation of the Helicobacter pylori urease apoprotein. Mol Cells, 2005. 20(3): p. 371-7.

Example 8 The Presence of Acid Resistance Systems Increases the Immunogenicity of a Live Attenuated Salmonella Vaccine

To investigate the effect of our system on immunogenicity, we constructed derivatives of S. Typhimurium ΔphoPQ strain χ8089 that carried either the ΔPadiA::TT araC PBAD adiAC or the ΔcysG::TT araC PBAD gadBC systems in which adiAC or gadBC expression is regulated by arabinose. Strains were grown in the presence of 0.1% arabinose and used to inoculate mice treated with histamine to induce a low gastric pH. Mice were given various doses of each strain, 1×104, 1×106 or 1×108 CFU. Mice were inoculated with the same dose of the same strains on days 0 and 28 (low gastric pH induced prior to both doses). Mice were challenged on day 49 with 1×108 CFU of wild-type S. Typhimurium strain χ3761 and observed for two weeks post challenge. The results (Table 3) indicated that only strains carrying the arabinose-inducible acid resistance system were protective when administered at doses of 1×106 CFU or 1×108 CFU. None were protective at the 1×104 dose. These results indicate that an acid-resistance system can enhance the immunogenicity of live attenuated Salmonella vaccines.

TABLE 3 Effect of arabinose-inducible acid resistance systems on protective efficacy of S. Typhimurium ΔphoPQ strains Immunizing Dose Post challenge Strain* (CFU) live/total χ8089 1 × 104 0/5 χ11808 1 × 104 0/5 χ11789 1 × 104 1/5 χ8089 1 × 106 0/5 χ11808 1 × 106 3/5 χ11789 1 × 106 2/5 χ8089 1 × 108 0/5 χ11808 1 × 108 5/5 χ11789 1 × 108 5/5 PBS 0/5 *genotypes - χ8089 = ΔphoPQ χ11808 = ΔphoPQ ΔPadiA::TT araC PBAD adiAC χ11789 = ΔphoPQ ΔcysG::TT araC PBAD gadBC

Mice were immunized day 0 and 28 (acid mice both times). Challenge on day 49 with 1×108 CFU wild-type S. Typhimurium χ3761. Mice observed for 21 days post challenge

Example 9 Use of Acid-Resistance Systems in Probiotic Bacteria

Probiotics are live microorganisms, which may provide beneficial effects when ingested. Although the mechanisms underlying still remain poorly understood, studies have demonstrated that the probiotics can efficiently inhibit the impact of pathogens in the gut either by directly by growth competition or indirectly via production of inhibitory substances such as bacteriocins [1]. Typical probiotics such as Lactic acid bacteria, bifidobacteria, certain yeasts and bacilli have been well studied for decades and show beneficial effects on treatment of antibiotic-associated diarrhea [2], lactose intolerance [3] and colon cancer [4]. The ability of probiotics to improve host immune function [5,6], modulate inflammatory and hypersensitivity responses [5] have also been documented. The Escherichia coli Nissle 1917 strain has been used as a probiotic agent in human and animal medicine to treat chronic inflammatory and infectious diseases of the human and animal intestine [7].

Similar to live bacterial vaccines, probiotic strains are administered orally a must survive the low pH stomach environment in order to be effective. The regulatable acid resistance systems may serve to increase the survival of probiotic bacteria during passage through the stomach.

References cited in Example 9

1. Sanders M E. Impact of probiotics on colonizing microbiota of the gut. J Clin Gastroenterol 45 Suppl, S115-119 (2011).

2. D'Souza A L, Rajkumar C, Cooke J, Bulpitt C J. Probiotics in prevention of antibiotic associated diarrhoea: meta-analysis. Bmj324(7350), 1361 (2002).

3. Sanders M E. Considerations for use of probiotic bacteria to modulate human health. The Journal of nutrition 130(2S Suppl), 384S-390S (2000).

4. Brady L J, Gallaher D D, Busta F F. The role of probiotic cultures in the prevention of colon cancer. The Journal of nutrition 130(2S Suppl), 410S-414S (2000).

5. Reid G, Jass J, Sebulsky M T, McCormick J K. Potential uses of probiotics in clinical practice. Clinical microbiology reviews 16(4), 658-672 (2003).

6. Ouwehand A C, Salminen S, Isolauri E. Probiotics: an overview of beneficial effects. Antonie van Leeuwenhoek 82(1-4), 279-289 (2002).

7. Kamada N, Inoue N, Hisamatsu T et aL Nonpathogenic Escherichia coli strain Nissle1917 prevents murine acute and chronic colitis. Inflammatory bowel diseases 11(5), 455-463 (2005).

Example 10 Use of Acid Resistance Systems in a Live Attenuated Salmonella enterica Serovar Gallinarum Vaccine for Poultry

Salmonella enterica serovar Gallinarum (S. Gallinarum) is a host-adapted pathogen that causes fowl typhoid—an important disease of poultry (1). Fowl typhoid is a septicemic disease with a typically short course and significant morbidity and mortality, which can reach as high as 100% (2). The disease occurs primarily in mature flocks, although birds of all ages may be infected. Certain mutations of S. Gallinarum, such as Δfur mutant χ11797 and Δfur Apmi mutant χ11798, are effective when delivered intramuscularly, but are only partially effective when delivered orally. This discrepancy can be explained by the acid sensitivity of these strains (FIG. 15).

Thus, it may be that because the double mutant is more sensitive to low pH than the Δfur strain (FIG. 15), it does not survive as well during passage through the low pH environment of the proventriculus. If this is the case, pH sensitivity may also help to explain our conflicting results with fur mutant χ11797, which was protective when orally administered to chicks (Table 4), but was less effective when orally administered to older layers. The proventricular pH in chickens changes during the first few weeks of life, ranging from a pH of about 5 at two days of age to about 3 to 3.5 by fifteen days of age (3). Thus, it is possible that survival of strain χ11797 was greater in chicks than in the older birds used in our study. When we bypassed the gastric compartment by intramuscular injection, the χ11797 was able to elicit a protective response (Table 4). The increased acid sensitivity of χ11798 could account for its lack of immunogenicity in chicks.

Introduction of an inducible acid resistance system can overcome this acid sensitivity. We introduced the arabinose-regulated gadBC system by introducing suicide plasmid pYA5120 (Table 1) into strains χ11797 and χ11798 by conjugation. Transconjugants are selected on LB plates with 20 μg/ml chloramphenicol. Loss of the integrated suicide plasmid is selected for on LB plates with 5% sucrose. The resulting strains derived from χ11797 and χ11798 are designated χ12040 and χ12041, respectively. When the strains are grown in the presence of 0.05% arabinose, the presence of the gadBC system increased the acid resistance of both strains to wild-type levels (FIG. 16). Thus, inclusion of the gadBC system can enhance acid resistance of S. Gallinarum vaccine strains.

TABLE 4 Efficacy of Δfur and Δfur Δpmi mutants as vaccines against S. Gallinarum challenge in chickens. Age of S. Gallinarum bird at Route of % vaccine vacci- vacci- sur- strain Genotype nation Breed nation vival χ11797 Δfur 5 days  Rhode oral 91% Island Red χ11798 Δpmi 5 days  Rhode oral 22% Δfur Island Red Buffer 5 days  Rhode oral 18% Island Red χ11797 Δfur 7 weeks Brown oral 50% layers χ11797 Δfur 7 weeks Brown intra- 100%  layers muscular χ11798 Δpmi 7 weeks Brown intra- 100%  Δfur layers muscular No 38% vaccine

References Cited in Example 10

1. Shivaprasad H L. 2000. Fowl typhoid and pullorum disease. Rev Sci Tech 19:405-424.

2. Barrow P A, Freitas Neto O C. 2011. Pullorum disease and fowl typhoid—new thoughts on old diseases: a review. Avian Pathol 40:1-13.

3. Rynsburger J M, Classen H L. 2007. Effect of age on intestinal pH of broiler chickens, International Poultry Scientific Forum, Atlanta, Ga., USA.

Example 11 Use of Acid Resistance Systems in Salmonella enterica Serovar Dublin Vaccines

Salmonella Dublin is host-adapted for cattle, causing systemic infections, enteritis and abortions (1). It can also cause human disease (1). As in non-ruminants, the gastrointestinal tract of cattle is composed of low pH compartments in which acid-sensitive bacteria are killed (2). During transit through the ruminant gastrointestinal tract, Salmonella encounters various acidic conditions. Volatile fatty acid (VFA) concentrations are high in the rumen of grain-fed animals, and the pH may vary from 5.0 to 6.5. In these conditions, VFAs are in the undissociated form and can freely enter the bacterial cells, dissociate, and acidify the cytosol. In hay-fed animals, less fermentation occurs in the rumen, and the pH remains between 6.5 and 7. In the abomasum, Salmonella can encounter strongly acidic conditions, regardless of the diet, due to the presence of mineral acids, resulting in a pH below 3. Then the pH increases from the proximal part to the distal part of the small intestine, cecum and colon. Inclusion of an inducible acid resistance system into live attenuated S. Dublin vaccines will enhance survival during low pH encounters in orally vaccinated cattle, leading to improved immunogenicity and efficacy. Introduction of an inducible acid resistance system can be accomplished by step-wise introduction of the ΔPadiA:TT AP rhaSR PrhaBAD adiA using plasmid pYA5093 followed by introduction of the Δ(PadiY-adiY-PadiC) adiC mutation using suicide plasmid pYA5072 to yield the rhamnose-regulated adiA system ΔPadiA::TT rhaSR PrhaBAD adiA Δ(PadiY-adiY-PadiC) adiC. Alternatively, the arabinose-regulated gadBC system can be introduced using plasmid pYA5120 (ΔcysG::TT araC PBAD gadBC).

References Cited in Example 11

1. Uzzau S, Brown D J, Wallis T, Rubino S, Leori G, Bernard S, Casadesus J, Platt D J, Olsen J E. 2000. Host adapted serotypes of Salmonella enterica. Epidemiol Infect 125:229-255.

2. Chaucheyras-Durand F, Faqir F, Ameilbonne A, Rozand C, Martin C. 2010. Fates of acid-resistant and non-acid-resistant Shiga toxin-producing Escherichia coli strains in ruminant digestive contents in the absence and presence of probiotics. Appl Environ Microbiol 76:640-647.

Example 12 Survival of Vaccine Strains in Low Gastric pH Mouse Model is Enhanced By Co-Administration of Ensure® Nutrition Shake

Methods. Strains used in this study are shown in Table 5. Plasmids are shown in Table 6. Six week old, female BALB/c mice (Charles River Laboratories, Wilmington, Mass., USA) were fasted without food or water for 6 h prior to the start of the experiment. Mice received the histamine H1-receptor antagonist chlorpheniramine (0.3 mg/kg) subcutaneously to prevent allergy/anaphylaxis symptoms. Prior to inoculation, low gastric pH was induced by subcutaneous injection of histamine dihydrochloride (10 mg/kg). Strains were grown to late log phase (optical density at 600 nm of 0.9), then pelleted and resuspended in PBS at a concentration of 5×1010 CFU/ml. Groups of 5 mice were orally inoculated 50 min after the administration of histamine (1). Low gastric pH was treated with sodium bicarbonate, Ensure, or nothing. Groups that were treated with bicarbonate received 40 μl of a 1.3% sodium bicarbonate solution orally 10 minutes prior to inoculation and an additional 10 μl 10 minutes after immunization. Groups that were treated with Ensure received 20 μl of Ensure® Nutrition shake (milk chocolate flavor) 10 minutes prior to inoculation and an additional 20 μl 10 minutes after immunization.

Gastric transit assays. Mice were inoculated as described above. Strains used in the gastric transit assays contained the low copy number plasmid pWSK129 (Kanr) to allow for precise quantitation of strain numbers in the non-sterile environment of the gastrointestinal tract. Mice were euthanized 1 h after inoculation and the entire small intestine was removed, homogenized and serially diluted. Samples were plated onto LB agar containing 0.2% arabinose with kanamycin to determine the number of viable bacteria present following low pH gastric transit. The survival of the Ensure® and bicarbonate groups was compared to the control group using the Mann-Whitney test. Statistical analysis was performed by GraphPad Prism version 6.00 for Windows (Graph Pad Software, La Jolla Calif. USA).

Results. To examine the ability of bicarbonate and Ensure® to combat gastric pH, these were used to buffer the stomach pH of mice. Because the gastric pH of a fasted mouse is about pH 4.0 and the gastric pH of a fasted human is about pH 1-2 (3,5,7), gastric acid secretion was induced in mice prior to immunization to better mimic the situation in humans. Using this protocol, the pH in the mouse stomach is reduced to around 1.5. Mice received either bicarbonate or Ensure® prior to and immediately following inoculation. Control mice received no treatment. Vaccine viability was measured following gastric transit (FIG. 17). For two of the three S. Typhi vaccine strains and the S. Typhimurium model strain, administration of Ensure® significantly increased the number of viable cells that reached the small intestine (p=0.0019 for χ9633(pYA4088), p=0.0256 for χ9640(pY4088) and p=0.0006 for χ9558(pYA4088)). This was a 599-, 75.0- and 647-fold increase, respectively, in the geometric mean number of viable cells to reach the ileum. Administration of Ensure® prior to and following immunization did not significantly affect the ability of χ9639(pYA4088) to transit the gastric compartment (p=0.2317), quite possibly due to the mutation in the rpoS gene which confers acid sensitivity. Bicarbonate similarly improved the survival of χ9640(pYA4088) (p=0.0190) and χ9558(pYA4088) (p=0.0379) during gastric transit, resulting in a 41.0- and 8.79-fold increase in the geometric mean number of cells to reach the ileum, respectively. Administration of bicarbonate did not significantly impact the survival of χ9633(pYA4088) or χ9639(pYA4088) (p=0.2317 and 0.4945, respectively). Overall, Ensure® worked best to protect these strains from low gastric pH. We infer that inclusion of a sugar-inducible acid resistance system such as araC PBAD gadBC or ΔPadiA::TT rhaSR PrhaBAD adiA Δ(PadiY-adiY-PadiC)-adiC, will enhance survival of these vaccines further.

TABLE 5 Strains used in gastric transit assays demonstrating protective effect of Ensure ® Nutrition shake. Sal- Ref- monella er- Strain Serovar Genotype/Phenotypea ence χ9558 Typhi- Δpmi Δ(gmd-fcl) ΔPfur::TT araC PBAD fur (4) murium ΔPcrp::TT araC PBAD crp ΔasdA:TT araC PBAD c2 ΔaraE ΔaraBAD ΔrelA::araC PBAD lacI TT ΔsopB ΔagfBAC, RpoS+ χ9633 Typhi ΔPcrp::TT araC PBAD crp ΔPfur::TT araC PBAD (6) fur Δpmi Δ(gmd-fcl) ΔsopB ΔrelA::araC PBAD lacI TT ΔaraE ΔaraBAD ΔtviABCDE ΔagfBAC ΔasdA, RpoS+ χ9639 Typhi ΔPcrp::TT araC PBAD crp ΔPfur::TT araC PBAD (6) fur Δpmi Δ(gmd-fcl) ΔrelA::araC PBAD lacI TT ΔaraE ΔtviABCDE ΔagfBAC ΔsopB ΔasdA, RpoS χ9640 Typhi ΔPcrp::TT araC PBAD crp ΔPfur::TT araC PBAD (6) fur Δpmi Δ(gmd-fcl) ΔrelA::araC PBAD lacI TT ΔaraE ΔtviABCDE ΔagfBAC ΔsopB ΔasdA RpoS+ aIn genotype descriptions, the subscripted number refers to a composite deletion and insertion of the indicated gene. P, promoter; TT, T4 ip III transcription terminator.

TABLE 6 Plasmids used in this study Plasmid Descriptiona Reference pWSK129 pSC101 ori, Kanr (8) pYA3493 pBR ori, Asd+ vector with bla SS-based (2) periplasmic antigen secretion pYA4088 Encodes the α-helical region of PspA (9) (aa 3-285) in pYA3493 aori, replication of origin; SS, secretion signal; Kanr, kanamycin resistance

References Cited for Example 12

1. Brenneman, K. E., C. Willingham, J. A. Kilbourne, R. Curtiss, 3rd and K. L. Roland. A low gastric pH mouse model to evaluate live attenuated bacterial vaccines. PLoS One 9: e87411.2014

2. Kang, H. Y., J. Srinivasan and R. Curtiss, 3rd. Immune responses to recombinant pneumococcal PspA antigen delivered by live attenuated Salmonella enterica serovar Typhimurium vaccine. Infect Immun 70: 1739-1749.2002

3. Kararli, T. T. Comparison of the gastrointestinal anatomy, physiology, and biochemistry of humans and commonly used laboratory animals. Biopharm Drug Dispos 16: 351-380.1995

4. Li, Y., S. Wang, G. Scarpellini, B. Gunn, W. Xin, S. Y. Wanda, K. L. Roland and R. Curtiss, 3rd. Evaluation of new generation Salmonella enterica serovar Typhimurium vaccines with regulated delayed attenuation to induce immune responses against PspA. Proc Natl Acad Sci USA 106: 593-598.2009

5. McConnell, E. L., A. W. Basit and S. Murdan. Measurements of rat and mouse gastrointestinal pH, fluid and lymphoid tissue, and implications for in-vivo experiments. J Pharm Pharmacol 60: 63-70.2008

6. Shi, H., J. Santander, K. E. Brenneman, S. Y. Wanda, S. Wang, P. Senechal, W. Sun, K. L. Roland and R. Curtiss. Live recombinant Salmonella Typhi vaccines constructed to investigate the role of rpoS in eliciting immunity to a heterologous antigen. PLoS One 5: e11142.2010

7. Verdu, E., F. Viani, D. Armstrong, R. Fraser, H. H. Siegrist, B. Pignatelli, J. P. Idstrom, C. Cederberg, A. L. Blum and M. Fried. Effect of omeprazole on intragastric bacterial counts, nitrates, nitrites, and N-nitroso compounds. Gut 35: 455-460.1994

8. Wang, R. F. and S. R. Kushner. Construction of versatile low-copy-number vectors for cloning, sequencing and gene expression in Escherichia coli. Gene 100: 195-199.1991

9. Xin, W., S. Y. Wanda, Y. Li, S. Wang, H. Mo and R. Curtiss, 3rd. Analysis of type II secretion of recombinant pneumococcal PspA and PspC in a Salmonella enterica serovar Typhimurium vaccine with regulated delayed antigen synthesis. Infect Immun 76: 3241-3254.2008

Claims

1. A recombinant attenuated derivative of a pathogenic enteric bacterium comprising at least one of the following:

a) a regulatable promoter operably linked to a nucleic acid encoding an arginine decarboxylase and a nucleic acid encoding an arginine agmatine antiporter;
b) a regulatable promoter operably linked to a nucleic acid encoding a glutamate decarboxylase and a nucleic acid encoding a glutamate/γ-aminobutyric acid antiporter; or
c) a regulatable promoter operably linked to a nucleic acid encoding a lysine decarboxylase and a nucleic acid encoding a lysine/cadaverine antiporter.

2. The recombinant bacterium of claim 1, wherein the enteric bacterium is either naturally acid sensitive or becomes more acid sensitive because of attenuating mutations, such that in the absence of induction of the regulatable promoter, the recombinant bacterium is acid sensitive, but upon induction of the regulatable promoter, the recombinant bacterium displays an increase in acid resistance.

3. The recombinant bacterium of claim 2, wherein the bacterium is acid sensitive because of a mutation in a nucleic acid sequence selected from the group consisting of rpoS, fur, phoPQ and guaBA.

4. The recombinant bacterium of claim 1, wherein the regulatable promoter is induced by a sugar.

5. The recombinant bacterium of claim 4, wherein the sugar is selected from the group consisting of arabinose and rhamnose.

6. The recombinant bacterium of claim 1, wherein the bacterium comprises at least one mutation selected from the group consisting of:

a) ΔPadiA::TT araC ParaBAD ad/AC mutation;
b) ΔPadiA::TT rhaSR PrhaBAD adiAC mutation;
c) rhaSR PrhaBAD gadBC mutation;
d) araC ParaBAD gadBC mutation;
e) ΔPcadB::TT rhaSR PrhaBAD cadBA mutation; and
f) ΔPcadB::TT araC ParaBAD cadBA mutation.

7. The recombinant bacterium of claim 6, wherein the bacterium further comprises at least one element selected from the group consisting of:

a) a regulatable promoter operably linked to gadA;
b) the cicA gene from E. coli transcribed from its own native promoter, a heterologous constitutive promoter or a heterologous regulatable promoter; and
c) a Ni-dependent urease system from H. pylori.

8. The recombinant bacterium of claim 1, wherein the bacterium is a Salmonella bacterium and:

a) the nucleic acid encoding the arginine decarboxylase is a Salmonella adiA sequence and the nucleic acid encoding the arginine agmatine antiporter is a Salmonella adiC sequence; or
b) the nucleic acid encoding the glutamate decarboxylase is an E. coli gadB and/or an E. coli gadA sequence and the nucleic acid encoding the glutamate γ-aminobutyric acid antiporter is an E. coli gadC sequence; or
c) the nucleic acid encoding the lysine decarboxylase is a Salmonella cadA sequence and the nucleic acid encoding the lysine/cadaverine antiporter is a cadB sequence.

9. A vaccine composition, the composition comprising a bacterium of claim 1.

10. A method for increasing the acid resistance of an acid sensitive bacterium, the method comprising introducing into the acid sensitive bacterium a cassette comprising at least one of the following: such that in the absence of induction of the regulatable promoter, the recombinant bacterium is acid sensitive, but upon induction of the regulatable promoter, the recombinant bacterium displays an increase in acid resistance.

a) a regulatable promoter operably linked to a nucleic acid encoding an arginine decarboxylase and a nucleic acid encoding an arginine agmatine antiporter;
b) a regulatable promoter operably linked to a nucleic acid encoding a glutamate decarboxylase and a nucleic acid encoding a glutamate/γ-aminobutyric acid antiporter; or
c) a regulatable promoter operably linked to a nucleic acid encoding a lysine decarboxylase and a nucleic acid encoding a lysine/cadaverine antiporter,

11. The method of claim 9, wherein the bacterium comprises a mutation in at least one nucleic acid sequence selected from the group consisting of rpoS, fur, phoPQ and guaBA.

12. The method of claim 9, wherein the regulatable promoter is induced by a sugar.

13. The method of claim 11, wherein the sugar is selected from the group consisting of arabinose and rhamnose.

14. The method of claim 9, wherein the bacterium comprises at least one mutation selected from the group consisting of:

a) ΔPadiA::TT araC ParaBAD adiAC mutation;
b) APadiA::TT rhaSR PrhaBADadiAC mutation;
c) rhaSR PrhaBAD gadBC mutation;
d) araC ParaBAD gadBC mutation;
e) APcadB::TT rhaSR PrhaBAD cadBA mutation; and
f) APcadB::TT araC ParaBAD cadBA mutation.

15. The recombinant bacterium of claim 14, wherein the bacterium further comprises at least one element selected from the group consisting of:

a) a regulatable promoter operably linked to gadA;
b) the cicA gene from E. coli transcribed from its own native promoter, a heterologous constitutive promoter or a heterologous regulatable promoter; and
c) a Ni-dependent urease system from H. pylori.

16. The method of claim 9, wherein the bacterium is a Salmonella bacterium and:

a) the nucleic acid encoding the arginine decarboxylase is a Salmonella adiA sequence and the nucleic acid encoding the arginine agmatine antiporter is a Salmonella adiC sequence; or
b) the nucleic acid encoding the glutamate decarboxylase is an E. coli gadB and/or an E. coli gadA sequence and the nucleic acid encoding the glutamate γ-aminobutyric acid antiporter is an E. coli gadC sequence; or
c) the nucleic acid encoding the lysine decarboxylase is a Salmonella cadA sequence and the nucleic acid encoding the lysine/cadaverine antiporter is a cadB sequence.

17. A recombinant Salmonella bacterium, the bacterium comprising a regulatable promoter operably linked to at least one nucleic acid selected from the group consisting of:

a) adiA and adiC;
b) gadB and gadC; and
c) cadB and cadA.

18. The recombinant Salmonella bacterium of claim 17, wherein the bacterium further comprises a mutation in at least one nucleic acid sequence selected from the group consisting of rpoS, fur, phoPQ and guaBA that renders the bacterium acid sensitive.

19. The recombinant Salmonella bacterium of claim 17, wherein the bacterium further comprises at least one element selected from the group consisting of:

a) a regulatable promoter operably linked to gadA;
b) the clcA gene from E. coli transcribed from its own native promoter, a heterologous constitutive promoter or a heterologous regulatable promoter; and
c) a Ni-dependent urease system from H. pylori.

20. A vaccine composition, the composition comprising a bacterium of claim 17.

Patent History
Publication number: 20170327830
Type: Application
Filed: Dec 28, 2016
Publication Date: Nov 16, 2017
Inventors: Roy Curtiss, III (Paradise Valley, AZ), Karen Brenneman (Leland, NC), Kenneth Roland (Mesa, AZ)
Application Number: 15/392,024
Classifications
International Classification: C12N 15/74 (20060101); A61K 39/00 (20060101); A61K 39/112 (20060101); A61K 39/00 (20060101); A61K 39/00 (20060101); C12N 9/88 (20060101); A61K 39/00 (20060101);