RECOMBINANT AVIAN INFECTIOUS CORYZA VACCINE AND PROCESS FOR PREPARING SAME

Abstract

A recombinant avian infectious coryza vaccine and a process for preparing the same are provided. A process for preparing a recombinant avian infectious coryza vaccine which comprises step of constructing E. coli that may produce as an inclusion body a fusion peptide consisting of peptides derived from outer-membrane protein of Avibacterium paragarinarum serotype A and serotype C, step of culturing said E. coli and colleting and purifying inclusion body from culture, and step of preparing a preparation comprising said purified inclusion body, and an avian infectious coryza vaccine comprising as an active ingredient the fusion peptide. A linker sequence may be inserted between the respective peptides comprising the fusion peptide. For the peptide derived from the serotypes A and C, an amino acid sequence region of Region 2 or its vicinity responsible for protection from infection may be used.

Description

TECHNICAL FIELD

The present invention relates to a recombinant avian infectious coryza vaccine and a process for preparing the same. More particularly, the present invention relates to a recombinant avian infectious coryza vaccine comprising as an active ingredient a fusion peptide consisting of a part of an outer-membrane protein of Avibacterium paragallinarum (hereinafter also referred to as “A.pg”) serotype A and a part of an outer-membrane protein of A.pg serotype C and process for preparing the same.

BACKGROUND ART

Avian infectious coryza is one of the most important respiratory diseases caused by infection with A.pg. Chicken suffering from avian infectious coryza shows cardinal symptoms of a running nose, swelling of the face and epiphora. Avian infectious coryza brings about a great economical damage since it leads to decrease in the breeding rate of chicken, retarding of egg laying, decrease in egg production or failure of egg laying.

Page et al. classified A.pg into three serotypes A, B and C (see e.g. Non-patent reference 1) and Sawata et al. classified A.pg into two serotypes 1 and 2 (see e.g. Non-patent reference 2). Thereafter, Kume et al. reported that serotype A by Page et al. corresponds to serotype 1 by Sawata et al. and serotype C by Page et al. corresponds to serotype 2 by Sawata et al. (see e.g. Non-patent references and 4). Today, it is established that main causative agents of avian infectious coryza are A.pg serotype A (hereinafter also referred to as “A.pg-A”) and A.pg serotype C (hereinafter also referred to as “A.pg-C”).

For prevention of avian infectious coryza, an inactivated vaccine has hitherto been used widely which is obtained by inactivating the cells of A.pg-A or A.pg-C with formalin, thimerosal and the like. However, adverse side effects caused by such an inactivated vaccine have been an issue as it has been reported that local necrotic lesions are formed in the inoculated chicken when the vaccine is administered (see e.g. Non-patent reference 5). Under the circumstances, attempting to develop a safe vaccine, a recombinant vaccine has been investigated comprising a protective antigen against infection prepared by genetic recombination technique.

For instance, Tokunaga et al. isolated and identified a gene coding for an outer-membrane protein of A.pg-A (outer-membrane protein gene) and found that a peptide obtained by expressing a part of said gene (HPG3.5 kbp, HPG4.1 kbp) in E. coli is useful as a protective antigen against infection for avian infectious coryza. Furthermore, using said DNA fragment as a probe, they obtained an outer-membrane protein gene from A.pg-C and compared nucleotide sequences of open reading frame of the outer-membrane protein gene from A.pg-A and A.pg-C. As a result, they revealed that both nucleotide sequences had homology of about 80% as a whole, that a region of 3.4 kbp at the 5′- end (hereinafter also referred to as “Region 1”) and a region of about 1.2 kbp at the 3′- end (hereinafter also referred to as “Region 3”) had extremely high homology and that a region of about 1.5 kbp flanked by Region 1 and Region 3 (hereinafter also referred to as “Region 2”) had low homology (see Patent reference 1).

It is also reported by Noro et al. that the outer-membrane protein discovered by Tokunaga et al. is important as a protective antigen for avian infectious coryza. Noro et al. immunized chicken with peptides coded by DNA fragments of 4,801 by and 5,157 bp, which are parts of the outer-membrane protein gene from A.pg-A, to show that said peptides may induce HI antibody to A.pg-A and may have a vaccine effect (see e.g. Patent reference 2) and further reported that peptides coded by DNA fragments of about 5.1 kbp and 5.5 kbp, which are parts of the outer-membrane protein gene from A.pg-C, had similar function and effect (see e.g. Patent reference 3).

On the other hand, Yamamoto et al. employed a polypeptide coded by a DNA fragment of 2,016 bp, which comprises most of the outer-membrane protein gene from A.pg-A to show usefulness of said polypeptide (see e.g. Patent reference 4) but the nucleotide sequence of about 300 by at the 3′ end of the DNA fragment reported by them was extremely different from those shown by Tokunaga et al. and Noro et al.

• Patent reference 1: WO98/12331
• Patent reference 2: Japanese patent No. 4001117
• Patent reference 3: JP 2008-156317
• Patent reference 4: JP 2004-57078
• Non-patent reference 1: Am. J. Vet. Res., 23:85-95, 1962
• Non-patent reference 2: Jpn. J. Vet. Sci., 40:645-652, 1978
• Non-patent reference 3: m. J. Vet. Res., 41:757-760, 1980
• Non-patent reference 4: Am. J. Vet.Res., 41:1901-1904, 1980
• Non-patent reference 5: Avian Dis., 15:109-117, 1971

DISCLOSURE OF THE INVENTION

Technical Problem to be Solved by the Invention

As described above, it has been revealed that the outer-membrane protein or its partial peptide from A.pg-A and A.pg-C, the main causative agent of avian infectious coryza, is useful as a protective antigen against avian infectious coryza. Thus, by mixing these protective antigens against infection, immunization to avian infectious coryza may efficiently be done. However, an approach by simple mixing necessitates separate production of the two infectious protective antigens and thus is costly. In general, a vaccine for use in an animal, unlike a vaccine for use in human, would not be accepted by a stock farmer unless the vaccine is not only in high quality but also is available at a low cost. Therefore, for a vaccine for use in an animal, a process for the production with less cost for production is desired.

Means for Solving the Problems

The present inventors have assiduously investigated in order to attain the object as described above, and as a result, have revealed that peptide fragments coded by the sequence of about 1.6 kbp comprising Region 2 (the nucleotide sequence of 3,639 bp to 5,162 bp for A.pg-A and the nucleotide sequence of 4,247 bp to 5,758 bp for A.pg-C: see FIGS. 1 and 2) of the outer-membrane protein gene from A.pg-A and A.pg-C (peptides coded by a DNA sequence of from 3,558 bp to 5,192 bp for A.pg-A and by a DNA sequence of from 4,166 bp to 5,788 bp for A.pg-C: hereinafter also referred to as “AΔ5-1” and “CΔ5-1”, respectively: see FIGS. 1 and 2) are useful as a protective antigen for avian infectious coryza. The present inventors have found that a fusion peptide (hereinafter also referred to as “ACΔ5-1”), which is obtained by linking together a DNA fragment coding for AΔ5-1 and a DNA fragment coding for CΔ5-1 and expressing the resultant DNA fragment, maintained immunogenicity of the respective antigens even after fusion and that the fusion peptide exhibited infection protective effect to avian infectious coryza equivalent to or more than that of AΔ5-1 or CΔ5-1, each expressed alone. Furthermore, the present inventors have found that CΔ5-1 is expressed in a soluble fraction when expressed alone whereas AΔ5-1 is expressed in an insoluble fraction by forming an inclusion body to thereby complete the present invention.

Accordingly, an object of the present invention is to provide a vaccine for avian infectious coryza comprising as an active ingredient a fusion peptide, obtained by linking to each other a peptide fragment comprising a specific region of the outer-membrane protein from A.pg-A and a peptide fragment comprising a specific region of the outer-membrane protein from A.pg-C, and a process for preparing the same.

As used herein, the outer-membrane proteins from A.pg-A and A.pg-C as isolated and identified by Tokunaga et al. (Patent reference 1) are also collectively referred to as “HMTp210 protein” and peptide fragments derived from HMTp210 protein of A.pg-A and A.pg-C are also referred to as “Peptide A” and “Peptide C”, respectively.

Thus, the present invention includes the followings:

• [1] A process for preparing a recombinant avian infectious coryza vaccine which comprises step of constructing a host that may produce as an inclusion body a fusion peptide consisting of a peptide fragment (Peptide A) derived from HMTp210 protein of A.pg-A and a peptide fragment (Peptide C) derived from HMTp210 protein of A.pg-C, step of culturing said host and colleting and purifying a fraction of inclusion body from culture, and step of preparing a preparation comprising said purified fraction of inclusion body.
• [2] The process of [1] wherein Peptide A and Peptide C consist of 600 or less amino acid residues.
• [3] The process of [1] wherein Peptide A has an amino acid sequence selected from the group consisting of SEQ ID NOs: 1, 27, 28, 29, 30, 31, 32, 33, 34 and 35 whereas Peptide C has an amino acid sequence selected from the group consisting of SEQ ID NOs: 2, 3, 4, 50, 51, 52, 53, 54, 55 and 56.
• [4] The process of [3] wherein Peptide A comprises an amino acid sequence shown by SEQ ID NO: 35 whereas Peptide C comprises an amino acid sequence shown by SEQ ID NO: 56.
• [5] The process of [3] or [4] wherein Peptide A or Peptide C comprises an amino acid sequence where one or several amino acids are deleted, added or replaced.
• [6] The process of any one of [1] to [5] wherein a ratio of Peptide A and Peptide C in the fusion peptide is 1 to 3 of Peptide C to 1 of Peptide A.
• [7] The process of any one of [1] to [6] wherein the fusion peptide comprises at least a structure where Peptide C is linked to the C-terminal of Peptide A.
• [8] The process of any one of [1] to [7] wherein the fusion peptide has a linker between Peptide A and Peptide A, Peptide C and Peptide C, or Peptide A and Peptide C.
• [9] The process of [3] wherein the fusion peptide has an amino acid sequence selected from the group consisting of SEQ ID NOs: 8, 9, 10, 11, 12, 13, 41, 42, 43, 44, 45, 46, 47, 48, 49, 61, 62, 63, 64, 65, 66 and 67.
• [10] A recombinant avian infectious coryza vaccine comprising as an active ingredient a fusion peptide consisting of a peptide fragment (Peptide A) derived from HMTp210 protein of A.pg-A and a peptide fragment (Peptide C) derived from HMTp210 protein of A.pg-C.
• [11] The vaccine of [10] wherein the fusion peptide has a property of forming an inclusion body when produced by the host.
• [12] The vaccine of [10] wherein Peptide A and Peptide C consist of 600 or less amino acid residues.
• [13] The vaccine of [10] wherein Peptide A has an amino acid sequence selected from the group consisting of SEQ ID NOs: 1, 27, 28, 29, 30, 31, 32, 33, 34 and 35 whereas Peptide C has an amino acid sequence selected from the group consisting of SEQ ID NOs: 2, 3, 4, 50, 51, 52, 53, 54, 55 and 56.
• [14] The vaccine of [13] wherein Peptide A comprises an amino acid sequence shown by SEQ ID NO: 35 whereas Peptide C comprises an amino acid sequence shown by SEQ ID NO: 56.
• [15] The vaccine of [13] or [14] wherein Peptide A or Peptide C comprises an amino acid sequence where one or several amino acids are deleted, added or replaced.
• [16] The vaccine of any one of [10] to [15] wherein a ratio of Peptide A and Peptide C in the fusion peptide is 1 to 3 of Peptide C to 1 of :Peptide A.
• [17] The vaccine of any one of [10] to [16] wherein the fusion peptide comprises at least a structure where Peptide C is linked to the C-terminal of Peptide.
• [18] The vaccine of any one of [10] to [17] wherein the fusion peptide has a linker between Peptide A and Peptide A, Peptide C and Peptide C, or Peptide A and Peptide C.
• [19] The vaccine of [13] wherein the fusion peptide has an amino acid sequence selected from the group consisting of SEQ ID NOs: 8, 9, 10, 11, 12, 13, 41, 42, 43, 44, 45, 46, 47, 48, 49, 61, 62, 63, 64, 65, 66 and 67.
• [20] A recombinant avian infectious coryza vaccine comprising as an active ingredient a peptide consisting of a sequence comprising the amino acid sequence shown by SEQ ID NO: 35, said sequence being within the amino acid sequence shown by SEQ ID NO: 1 with addition of 1 to 200 amino acid residues at the N-terminal and/or C-terminal thereof.
• [21] The vaccine of [20] wherein said vaccine comprises as an active ingredient a peptide consisting of the amino acid sequence shown by SEQ ID NO: 1.

[22] A recombinant avian infectious coryza vaccine comprising as an active ingredient a peptide consisting of a sequence comprising the amino acid sequence shown by SEQ ID NO: 56, said sequence being within the amino acid sequence shown by SEQ ID NO: 3 with addition of 1 to 200 amino acid residues at the N-terminal and/or C-terminal thereof.

• [23] The vaccine of [22] wherein said vaccine comprises as an active ingredient a peptide consisting of the amino acid sequence shown by SEQ ID NO: 3 or 52.
• [24] The vaccine of [21] or [23] wherein said peptide comprises an amino acid sequence where one or several amino acids are deleted, added or replaced.

Effects of the Invention

In accordance with the present invention, provided are an avian infectious coryza vaccine comprising as an active ingredient a fusion peptide consisting of a peptide fragment derived from HMTp210 protein of A.pg-A and a peptide fragment derived from HMTp210 protein of A.pg-C linked to each other and a process for preparing the same. The avian infectious coryza vaccine of the present invention may simultaneously provide immunization for protection from avian infectious coryza caused by A.pg-A and A.pg-C .

In accordance with the process of the present invention, it becomes possible to let CΔ5-1, which is expressed in a soluble fraction when expressed alone, form an inclusion body so as to be expressed in an insoluble fraction via expression of its fusion peptide with AΔ5-1. As a result, not only purification of said fusion peptide is facilitated but also production cost is reduced since infection protective antigens to A.pg-A and A.pg-C may be prepared with a single culture.

BRIEF DESCRIPTION OF DRAWINGS

FIG. 1 shows a position of AΔ5-1 fragment in HMTp210 gene of A.pg-A (HMTp210A gene) where the indicated nucleotide numbers correspond to those disclosed in Patent reference 1 (Tokunaga et al.).

FIG. 2 shows position of CΔ4c-1, CΔ5-1 and CΔ6b-1b fragments in HMTp210 gene of A.pg-C (HMTp210C gene) where the indicated nucleotide numbers correspond to those disclosed in Patent reference 1 (Tokunaga et al.).

FIG. 3 is a photograph showing results of SDS-PAGE performed on supernatant and precipitate fractions after centrifugation of cell debris of fusion peptide-producing E. coli. M: marker, Lane 1: AΔ5-1/CΔ4c-1 (precipitate fraction), Lane 2: AΔ5-1/CΔ4c-1 (supernatant fraction), Lane 3: ACΔ5-1 (precipitate fraction), Lane 4: ACΔ5-1 (supernatant fraction), Lane 5: AΔ5-1/CΔ6b-1b (precipitate fraction), Lane 6: AΔ5-1/CΔ6b-1b (supernatant fraction). Arrows show fusion peptides as expressed.

FIG. 4 shows a position of AΔ5-1, AΔ5-2, AΔ5-3, AΔ5-4, AΔ9-2, AΔ9-3, AΔ9-4, CΔ6-2, CΔ6-3 and CΔ6-4 fragments in HMTp210 gene of A.pg-A (HMTp210A gene) where the indicated nucleotide numbers correspond to those disclosed in Patent reference 1 (Tokunaga et al.).

FIG. 5 shows a position of CΔ5-1, CΔ5-2, CΔ5-4, CΔ9-0, CΔ9-2, CΔ9-4, CΔ6-2 and CΔ6-4 fragments in HMTp210 gene of A.pg-C (HMTp210C gene) where the indicated nucleotide numbers correspond to those disclosed in Patent reference 1 (Tokunaga et al.).

FIG. 6 is a photograph showing results of SDS-PAGE performed on precipitate fractions after centrifugation of cell debris of fusion peptide-producing E. coli. M: marker, Lane 1: ACΔ5-1 (precipitate fraction), Lane 2: AΔ5-2/CΔ5-1 (precipitate fraction), Lane 3: AΔ5-3/CΔ5-1 (precipitate fraction), Lane 4: AΔ5-4/CΔ5-1 (precipitate fraction), Lane 5: AΔ9-2/CΔ5-1 (precipitate fraction), Lane 6: AΔ9-3/CΔ5-1 (precipitate fraction), Lane 7: AΔ9-4/CΔ5-1 (precipitate fraction), Lane 8: AΔ6-2/CΔ5-1 (precipitate fraction), Lane 9: AΔ6-3/CΔ5-1 (precipitate fraction), Lane 10: AΔ6-4/CΔ5-1 (precipitate fraction), Arrows show fusion peptides as expressed.

FIG. 7 is a photograph showing results of SDS-PAGE performed on precipitate fractions after centrifugation of cell debris of fusion peptide-producing E. coli. M: marker, Lane 1: ACΔ5-1 (precipitate fraction), Lane 2: AΔ5-1/CΔ5-2 (precipitate fraction), Lane 3: AΔ5-1/CΔ5-4 (precipitate fraction), Lane 4: AΔ5-1/CΔ9-0 (precipitate fraction), Lane 5: AΔ5-1/CΔ9-2 (precipitate fraction), Lane 6: AΔ5-1/CΔ9-4 (precipitate fraction), Lane 7: AΔ5-1/CΔ6-2 (precipitate fraction), Lane 8: AΔ5-1/CΔ6-4 (precipitate fraction), Arrows show fusion peptides as expressed.

FIG. 8 is a photograph showing results of SDS-PAGE performed on supernatant and precipitate fractions after centrifugation of cell debris of peptide C-producing E. coli. M: marker, Lane 1: CΔ5-1-pQE (supernatant fraction), Lane 2: CΔ5-2-pQE (supernatant fraction), Lane 3: CΔ5-4-pQE (supernatant fraction), Lane CΔ9-0-pQE (supernatant fraction), Lane 5: CΔ9-2-pQE (supernatant fraction), Lane 6: CΔ9-4-pQE (supernatant fraction), Lane 7: CΔ6-2-pQE (precipitate fraction), Lane 8: CΔ6-4-pQE (supernatant fraction). Arrows show fusion peptides as expressed.

BEST MODE FOR CARRYING OUT THE INVENTION

The present invention is characterized by a process for preparing a recombinant avian infectious coryza vaccine comprising step of preparing an inclusion body-forming fusion peptide consisting of Peptide A derived from HMTp210 protein of Avibacterium paragarinarum (hereinafter referred to as “A.pg”) serotype A and Peptide C derived from HMTp210 protein of A.pg-C. More specifically, the present invention is characterized by a process for preparing an avian infectious coryza vaccine which comprises step of constructing a host that may produce as an inclusion body a fusion peptide consisting of a peptide fragment derived from HMTp210 protein of A.pg-A and a peptide fragment derived from HMTp210 protein of A.pg-C, step of culturing said host and colleting and purifying a fraction of inclusion body from culture, and step of preparing a preparation comprising said purified fraction of inclusion body, and an avian infectious coryza vaccine comprising as an active ingredient said fusion peptide.

A DNA fragment may be obtained as described below that consists of a part of a gene (hereinafter also referred to as “HMTp210A gene”) coding for an amino acid sequence of HMTp210 protein (SEQ ID NO: 25) of A.pg-A and a gene (hereinafter also referred to as “HMTp210C gene”) coding for an amino acid sequence of HMTp210 protein (SEQ ID NO: 26) of A.pg-C

There are several isolated strains of A.pg-A and A.pg-C and any of these strains may be used in the present invention without limitation. Hitherto, there have been isolated, for instance, 221, O83 and W strains etc. for A.pg-A and 53-47, Modesto and HK-1 strains etc. for A.pg-C wherein mutations of substitution, deletion or addition of one or several amino acids are noted. For the present invention, any of these strains or mutants may be used.

For growth of A.pg-A and A.pg-C, a culture medium may be used that suitably contains polypeptone, glucose, casamino acid, sodium glutamate, yeast extract, sodium chloride, chicken meat infusion, nicotineamide adenine dinucleotide (β-NAD), chicken sera, and the like. A chicken broth supplemented with chicken sera was used herein, containing polypeptone S 5 g, casamino acid 1 g, sodium chloride 5 g, sodium L-glutamate 5 g, glucose 1 g, yeast extract 10 g, chicken meat infusion 175 mL, chicken sera 25 mL, β-NAD 0.025% in 1,000 mL of culture medium, for growth in a small/medium scale. Culture condition may be usually set at the temperature of 37° C. for 16 to 24 hours, which condition may suitably vary depending on purpose of use, a mode of culture, an amount of bacteria inoculated, a scale of culture, and the like.

Cells in culture may be collected by centrifugation (5,800 g, 20 min.) in a precipitate fraction. HMTp210A gene and HMTp210C gene (hereinafter also referred to collectively as “HMTp210 gene” in case that the two genes are not separately referred to) may be prepared from a genomic: DNAs extracted from the cells by genetic recombination technique according to Sambrook et al. (Molecular Cloning, A Laboratory Manual Second Edition. Cold Spring Harbor Laboratory Press, N.Y., 1989). A commercially available kit may also be used. For instance, for extraction of chromosomal DNAs, PureGene kit (Gentra Systems), SepaGene kit (Sanko Junyaku Co., Ltd.), ISOPLANT (Wako Pure Chemical Industries, Ltd.), and the like may be used.

More specifically, chromosomal DNAs may be extracted from the cells collected by centrifugation using PureGene kit: (Gentra Systems) and the like, and a genome DNA library of the cells may be prepared in accordance with Tokunaga et al. (Patent reference 1). Using the obtained DNA fragments as a template, PCR may be performed to amplify DNA fragments in desired sizes using Prime STAR HS DNA Polymerase (TAKARA BIO Inc.) in accordance with protocol attached thereto. Primers for use in PCR may be designed based on the nucleotide sequences of A.pg-A- and A.pg-C-derived HMT p210 genes as Tokunaga et al. disclosed (Patent reference 1). Primers for PCR may be readily available if asked to DNA synthesis contractor services (e.g. Sigma Genosys Japan K.K.). When designed, nucleotide sequences of appropriate restriction enzyme cleavage sites may be added at the 5′-end of upstream Primer and at the 5′-end of downstream Primer.

A DNA fragment coding for the fusion peptide of the present invention may be obtained by linking together the DNA fragment coding for HMTp210A gene and the DNA fragment coding for HMTp210C gene, as obtained above, using a DNA synthase directly or after cleavage with a restriction enzyme. A DNA fragment coding for a linker consisting of an amino acid sequence of a suitable size may optionally be added between the DNA fragment coding for HMTp210A gene and the DNA fragment coding for HMTp210C gene. For a linker, an amino acid with a lot of flexibility such as a neutral amino acid, e.g. glycine, serine, and the like may preferably be used. A linker consisting of a single sort of amino acids or two or more sorts of amino acids may be used. A linker may be in general in a size of 5 to 20 amino acids, preferably, in a size of 10 to 15 amino acids.

In accordance with the present invention, a DNA fragment of the HMTp210A gene and the HMTp210C gene coding for a fusion peptide may be used that may protect from infection of A.pg-A and A.pg-C and form an inclusion body. Such a DNA fragment includes, for instance, a DNA fragment coding for a peptide of Region 2 of an outer-membrane protein, a DNA fragment coding for a peptide of Region 2 with addition of an amino acid sequence at N-terminal and/or C-terminal thereof, DNA fragment coding for a peptide of Region 2 with addition of an amino acid sequence at N-terminal or C-terminal thereof and with deletion of an amino acid sequence at the remaining N-terminal or C-terminal thereof, and a DNA fragment coding for a peptide of Region 2 with deletion of an amino acid sequence at N-terminal and/or C-terminal thereof. The amino acid sequence to be added or deleted may be of 1 to 200, preferably 30 to 150 amino acids in length. Preferable is a DNA fragment coding for a peptide derived from HMTp210 protein of A.pg-A having an amino acid sequence selected from the group consisting of SEQ ID NOs: 1, 27, 28, 29, 30, 31, 32, 33, 34 and 35 and a peptide derived from HMTp210 protein of A.pg-C having an amino acid sequence selected from the group consisting of SEQ ID NOs: 2, 3, 4, 5, 6, 7, 50, 51, 52, 53, 54, 55 and 56. A DNA fragment coding for a mutant of the above peptide may also be used wherein one or several amino acids are deleted, added or replaced. A “mutant of the above peptide wherein one or several amino acids are deleted, added or replaced” as used herein refers to a mutant of the above peptide wherein 1, 2, 3, 4 or 5 amino acids are deleted, added or replaced. A DNA fragment coding for such a mutant peptide may be obtained by hybridization with a DNA fragment having a nucleotide sequence complementary to the nucleotide sequence of the DNA fragment coding for the above peptide under stringent condition or a method for introducing mutation such as site directed mutagenesis. These may be done by using kits commercially available.

Any combination of a DNA fragment derived from the HMTp210A gene and a DNA fragment derived from the HMTp210C gene may be used as far as a resulting peptide may form an inclusion body. For instance, a DNA fragment coding for a fusion peptide may be a DNA fragment derived from the HMTp210A gene downstream of which a DNA fragment derived from the HMTp210C gene is bound or vice versa. DNA fragments coding for a fusion peptide may also be combined to each other in tandem. Also, two or more DNA fragments derived from the HMTp210A gene may be bound to each other and downstream thereof two or more DNA fragments derived from the HMTp210C gene may further be bound. A DNA coding for fusion peptide may consists of a DNA fragment derived from the HMTp210A gene and a DNA fragment derived from the HMTp210C gene at a ratio of 1 of the former to 1 to 3 of the latter. Preferably, said ratio is 1:1. A nucleotide sequence of the obtained DNA fragment, after cloning into pBluescript II SK+ (Stratagne) or pCR2.1-TOPO (Invitrogen), may be determined with a DNA sequencer (ABI Prism 377 Applied Biosystems).

The thus obtained DNA fragments of A.pg-A and A.pg-C or the DNA fragment coding for a fusion peptide may be incorporated into an appropriate expression vector, which may then be introduced into a host for expression of each of the DNA fragments. For expression of a heterologous protein or peptide, bacteria, yeasts, animal cells, plant cells, insect cells, and the like may ordinarily be used, among which any host may be used as far as an inclusion body may be produced. For transformation of a host cell, methods known in the art may be used. For instance, calcium phosphate, DEAE dextran, approach using liposome such as lipofectin, polyethylene glycol fusion of protoplast, electroporation, heat shock, and the like may be used, as appropriately selected depending on a host cell as used. Preferably, E. coli may be used which allows for expression in a large amount.

For expression in E. coli, various expression vectors having trp promoter, T7 promoter, cspA promoter, and the like have been developed and commercially available and may be used as appropriate. Such an expression vector includes, for instance, pET-11d (Merck) and pQE30 (Quiagen). Depending on an expression vector, suitable E. coli such as BL21, HMS174, DH5a, HB101, JM109, and the like may be selected as a host. Transformation of E. coli may be conducted using commercially available competent cells in accordance with protocol attached thereto. Thus, recombinant E. coli producing the desired polypeptide may be obtained. For culture medium (e.g. LB, SOC, SOB, and the like) used for culture of E. coli, reagents used for selection of transformant (e.g. ampicillin) and reagents used for induced expression (e.g. indole acetic acid (IAA), isopropylthio-β-D-galactoside (IPTG), and the like), commercially available ones may be used. A pH of a culture medium may be within a range suitable for growth of E. coli (pH 6 to 8).

Screening of recombinant E. coli expressing a desired peptide (the object) may be carried out as described below. Cells cultured and grown in the presence of an expression inducer (IPTG was used in an expression system in the present invention) are collected by centrifugation (9,100 g, 5 minutes), suspended in a fixed volume of distilled water or PBS, disrupted by sonication or a homogenizer such as French press or Manton Golin and subject to centrifugation (e.g. 17,800 g, 15 minutes) for separation and recovery in precipitate and supernatant. To distilled water may appropriately be added a surfactant (e.g. Triton X-100), a chelating agent (e.g. EDTA), lisozyme, and the like. A fixed amount of supernatant and precipitate recovered may be subject to SDS-polyacrylamide gel electrophoresis, and after staining with Coomassie Brilliant Blue, expression of the object may be confirmed by a molecular size and stained image. For confirmation (or detection) of the object, approach based on an antigen-antibody reaction such as ELISA, Western blot, dot blot, and the like may also be used other than approach based on a molecular size as described above. All of these approaches are commonly used for detecting a heterologous protein or polypeptide expressed in E. coli and may be selected as appropriate. Thus, clones recovered in the precipitate, i.e. clones producing a fusion peptide that may form an inclusion body, may be selected.

Recovery of an inclusion body from the clones producing a fusion peptide may be carried out as described below. First, cells may be collected using centrifugation or MF membrane of a suitable size (Asahi Kasei Corporation). The collected cells may be disrupted in an appropriate manner so as to release inclusion bodies consisting of a fusion peptide out of the cells. Disruption of cells may be done by any known methods including, for instance, dissolution with a chemical substance, a surfactant, an enzyme, or physical treatment such as French press or sonication. By combining several of these, cells may be disrupted more effectively.

For instance, after the cells collected with MF membrane were diluted and concentrated with deionized water to remove the remaining culture components and the cellular metabolites, an appropriate buffer and lysozyme may be added and the resulting mixture may be left at a low temperature (4 to 15° C.) overnight to thereby dissolve the cellular membrane of the cells. The treated solution of the cells may be subject to French press (or Manton Golin) at 500 to 600 kg/cm² to disrupt the cells. A buffer may be of any kind as far as it has a buffering ability at a pH range of 7.5 to 9 at which lysozyme is active, such as Tris buffer. The buffer may be used at a concentration as commonly used as a buffer (10 to 50 mM). Lysozyme may be used at a concentration of 0.3 to 1.0 g/L. For instance, 20 mM Tris buffer at pH 8.5 may be added, lysozyme (0.6 g/L) may be added and the mixture may be left to stand at 4° C. overnight to dissolve the cell wall of the cells. After disrupting the cells with French press, dilution and concentration with a buffer or deionized water and MF membrane may be repeated to remove most of cellular components. Optionally, a surfactant such as Triton-X100 may be added. Inclusion bodies may be recovered by centrifugation of a concentrated solution containing inclusion bodies as precipitate.

The recovered inclusion bodies may be dissolved in a solution containing a denaturing agent. A denaturing agent to be used includes urea, guanidine hydrochloride, and the like with urea being preferable. Such urea and guanidine hydrochloride may be used in a range of concentration of 4 to 8 M and 2 to 6 M, respectively. For the present invention, 8M urea may preferably be used. For dissolving a denaturing agent and a reducing agent, a buffer at pH 6 to 9, preferably at pH 7 to 8, may be used. Any buffer that has a buffering ability at the above pH range may be used such as phosphate buffer, Tris buffer, glycine buffer, carbonate buffer, and the like. Dissolution may be performed at a temperature of 40° C. or less. Dissolution time may be set while observing dissolution of inclusion bodies, and usually 30 minutes to 1 hour.

Next, refolding, i.e. reconstruction of a normal steric structure, of a fusion peptide may be carried out by adding 10 to 20-fold volume of a buffer to the solution of inclusion bodies or by dialyzing the solution against a buffer. For refolding, the same kind, temperature and pH of a buffer as those used for dissolution of inclusion bodies may be employed. Refolding may be carried out at room temperature or less and by being left to stand for 1 to 7 days, preferably, for 3 to 4 days.

The solution containing fusion peptide may further be subject to purification procedure as occasion demands. For such purification procedure, a combination of the methods commonly used in the field of protein chemistry may be used such as e.g. centrifugation, salting-out, ultrafiltration, isoelectric focusing, electrophoresis, ion exchange chromatography, gel filtration chromatography, affinity chromatography, hydrophobic chromatography, hydroxyapatite chromatography, and the like. An amount of the obtained protein or polypeptide may be measured with a reagent for protein measurement such as BCA Protein Assay Reagent Kit (Pierce Biotechnology, Inc), Protein Assay Kit (BIO-RAD, Inc), and the like.

Usefulness of the fusion peptide of present invention as an avian infectious coryza vaccine may be demonstrated by immunizing chicken with a solution containing said fusion peptide and determining an antibody titer to A.pg-A and A.pg-C in sera obtained from the chicken or by challenging said immunized chicken with virulent bacteria and observing survival of the chicken and clinical symptoms such as a running nose, swelling of the face and epiphora. For immunization of chicken, an immune enhancing agent (adjuvant), as used for ordinary pharmaceutical preparation, may optionally be added. A mode of administration is not particularly restricted and administration may be done, for instance, subcutaneously, intradermally, intraperitoneally, or intranasally, oridinarily once to thrice every 2 to 4 weeks.

For preparing a pharmaceutical preparation containing the fusion peptide of the present invention as a vaccine, a solution containing said fusion peptide may be sterile filtered through membrane filter and to the filtrate may be added, as occasion demands, an immune enhancing agent (adjuvant) such as aluminum hydroxide, aluminum phosphate, mineral oil or non-mineral oil, a stabilizing agent such as Polysorbate 80, amino acids, and sugars, e.g. lactose and sucrose, and a preservative agent such as formalin, thimerosal, 2-phenoxyethanol, benzyl alcohol, benzethonium chloride and benzalkonium chloride. Also, by adding sugars effective as an excipient such as lactose or sucrose, a lyophilized preparation may be prepared. Thus, a vaccine comprising as an active ingredient the fusion peptide of the present invention may be prepared.

The obtained vaccine may be used alone as an avian infectious coryza vaccine or alternatively used as a mixed vaccine in combination with at least one vaccine selected from the group consisting of vaccines against other viruses such as avian infectious bronchitis virus, avian infectious bursal disease virus, avian encephalomyelitis virus, and egg drop syndrome virus, vaccinesropagainst bacteria such as Salmonella typhimurium, Salmonella enteritidis, and Salmonella pollorum and vaccines against protozoa such as Leucocytozoon cauleryi, Eimeria tenera, and Eimeria maxima.

The present invention is explained in more detail by means of the following Examples but is not construed to be limited thereto.

EXAMPLE 1

Construction of Plasmids for Expression of Fusion Peptides

Genome DNA libraries of A.pg-A 221 strain and A.pg-C 53-47 strain were prepared in accordance with Tokunaga et. al. (Patent reference 1). Briefly, genomic DNAs were extracted using PureGene kit (Gentra Systems) from cells collected by centrifugation (Tomy, RD-20PIV, 4,400 g, 20 min.). Using the obtained DNAs as a template, PCR was performed with Prime STAR HS DNA Polymerase (TAKARA BIO Inc.) to amplify DNA fragments of HMTp210 protein genes of A.pg-A and A.pg-C. PCR conditions were as follows: after reaction at 98° C. for 1 minute, denaturation (98° C. for seconds), annealing (55° C. for 15 seconds), and elongation reaction (72° C. for 120 seconds) for 15 cycles, followed by termination reaction (72° C. for 7 minutes).

Table 1 shows names and Sequence ID NOs of the respective DNA fragments and PCR primers used in the amplification reaction. NcoI recognition sequence was added to the 5′-primer and BamHI recognition sequence was added to the 3′-primer used for amplification of the DNA fragments of A.pg-A and BamHI recognition sequence was added to both the 5′-primer and the 3′-primer used for amplification of the DNA fragments of A.pg-C. FIGS. 1 and 2 show relative position of the respective DNA fragments. In Table, SEQ ID NOs indicated in the column of DNA fragments denote amino acid sequences coded by the respective DNA fragments.

	TABLE 1
	DNA fragment	5′-primer	3′-primer
	AΔ5-1	AΔ5-1-P5	AΔ5-1-P3
	(SEQ ID NO: 1)	(SEQ ID NO: 14)	(SEQ ID NO: 15)
	CΔ4c-1	CΔ4c-1-P5	CΔ4-5-P3
	(SEQ ID NO: 2)	(SEQ ID NO: 16)	(SEQ ID NO: 17)
	CΔ5-1	CΔ5-1-P5	CΔ4-5-P3
	(SEQ ID NO: 3)	(SEQ ID NO: 18)	(SEQ ID NO: 17)
	CΔ6b-1b	CΔ6b-1b-P5	CΔ6b-1b-P3
	(SEQ ID NO: 4)	(SEQ ID NO: 19)	(SEQ ID NO: 20)

Expression plasmids were prepared as described below. First, AΔ5-1 was digested with NcoI and BamHI and, after separation by 0.8% agarose gel electrophoresis, the DNA fragments were eluted and recovered using Wizard SV Gel and PCR Clean-Up System (Promega). The obtained fragments were linked to an expression vector pET-lid (Merck) digested previously with NcoI and BamHI and the resulting plasmid was used to transform E. coli BL21(DE3) strain (Merck). From this transformant, expression plasmid (pET-11d-AΔ5-1) was extracted using Wizard Plus SV Minipreps DNA Purification System (Promega).

Next, CΔ4c-1, CΔ5-1 and CΔ6b-1b were digested with BamHI and, after separation by 0.8% agarose gel electrophoresis, the DNA fragments were eluted and recovered using Wizard SV Gel and PCR Clean-Up System (Promega). The obtained fragments were linked in a forward orientation to pET-11d-AΔ5-1 digested previously with BamHI and the resulting plasmid was used to transform E. coli BL21(DE3) strain (Merck) to give expression plasmids pET-11d-AΔ5-1-CΔ4c-1, pET-11d-AΔ5-1-CΔ5-1 and pET-11d-AΔ5-1-CΔ6b-1b. In each of the constructed expression plasmids, CΔ4c-1, CΔ5-1 and CΔ6b-1b were inserted directly downstream of AΔ5-1 in a forward orientation which produce the fusion peptides as shown in Table 2.

TABLE 2
Plasmid               Fusion peptide
pET-11d-AΔ5-1-CΔ4c-1  AΔ5-1/CΔ4c-1 (SEQ ID NO: 8)
pET-11d-AΔ5-1-CΔ5-1   ACΔ5-1 (SEQ ID NO: 9)
pET-11d-AΔ5-1-CΔ6b-1b AΔ5-1/CΔ6b-1b (SEQ ID NO: 10)

EXAMPLE 2

Construction of Plasmids for Expression of Fusion Peptides With Addition of Linker

For addition of a linker sequence, DNA fragments of HMTp210 protein gene of A.pg were amplified as described in Example 1. Table 3 shows names and Sequence ID NOs of the respective DNA fragments and PCR primers used in the amplification reaction. The 5′-primer was added with XbaI recognition sequence and the 3′-primer was added with BamHI recognition sequence. In Table, SEQ ID NOs indicated in the column of DNA fragments denote amino acid sequences coded by the respective DNA fragments.

	TABLE 3
	DNA fragment	5′-primer	3′-primer
	AΔ5-1	AΔ5-1-P5	AΔ5-1-P3
	(SEQ ID NO: 1)	(SEQ ID NO: 14)	(SEQ ID NO: 15)
	L-CΔ4c-1	CΔ4c-1-L-P5	CΔ4-5-P3
	(SEQ ID NO: 5)	(SEQ ID NO: 21)	(SEQ ID NO: 17)
	L-CΔ5-1	CΔ5-1-L-P5	CΔ4-5-P3
	(SEQ ID NO: 6)	(SEQ ID NO: 22)	(SEQ ID NO: 17)
	L-CΔ6b-1b	CΔ6b-1b-L-P5	CΔ6b-1b-P3
	(SEQ ID NO: 7)	(SEQ ID NO: 23)	(SEQ ID NO: 20)

Expression plasmids where a linker is linked directly downstream of AΔ5-1 were prepared as described below. First, AΔ5-1 obtained in Example 1 was digested with NcoI and BamHI and, after separation by 0.8% agarose gel electrophoresis, the DNA fragments were eluted and recovered using Wizard SV Gel and PCR Clean-Up System (Promega). Next, to the C-terminal of the obtained fragments was added with a DNA synthetase a linker sequence consisting of a nucleotide sequence coding for ten glycine residues (Gly Linker: SEQ ID NO: 24) to give a DNA fragment (AΔ5-1-L). As a consequence of addition of the linker sequence, Bam HI recognition sequence at the C-terminal of AΔ5-1 is lost and instead thereof XbaI recognition sequence is generated.

Next, CΔ4c-1, CΔ5-1 and CΔ6b-1b were digested with XbaI and BamHI and, after separation by 0.8% agarose gel electrophoresis, the DNA fragments were eluted and recovered using Wizard SV Gel and PCR Clean-Up System (Promega). The obtained fragments were ligated with AΔ5-1 and then digested with BamHI. After separation by 0.8% agarose gel electrophoresis, the DNA fragments were eluted and recovered using Wizard SV Gel and PCR Clean-Up System (Promega). Further, the obtained fragments were inserted into an expression vector pET-lid (Merck) previously digested with NcoI and BamHI. The resulting expression plasmid was used to transform E. coli BL21(DE3) strain (Merck) to give expression plasmids pET-11d-AΔ5-1-L-CΔ4c-1, pET-11d-AΔ5-1-L-CΔ5-1 and pET-11d-AΔ5-1-L-CΔ6b-1b. In each of the constructed expression plasmids, CΔ4c-1, CΔ5-1 and CΔ6b-1b were inserted directly downstream of the linker sequence in a forward orientation which produce the fusion peptides via glycine derived from the linker sequence as shown in Table 4.

TABLE 4
Plasmid                 Fusion peptide
pET-11d-AΔ5-1-L-CΔ4c-1  AΔ5-1/L-CΔ4c-1 (SEQ ID NO: 11)
pET-11d-AΔ5-1-L-CΔ5-1   ACΔ5-1-L (SEQ ID NO: 12)
pET-11d-AΔ5-1-L-CΔ6b-1b AΔ5-1/L-CΔ6b-1b (SEQ ID NO: 13)

EXAMPLE 3

Construction of Plasmids for Expression of Shortened Fusion Peptides (1)

Genome DNA libraries of A.pg-A 221 strain were prepared as described in Example 1. PCR was performed to amplify the DNA fragments shown in Table 5. PCR conditions were as follows: after reaction at 98° C. for 1 minute, denaturation (98° C. for 10 seconds), annealing and elongation reactions (70° C. for 120 seconds) for 15 cycles, followed by termination reaction (72° C. for 7 minutes). Expression plasmids containing these fragments, pET-11d-AΔ5-1, pET-11d-AΔ5-2, pET-11d-AΔ5-3, pET-11d-AΔ5-4, pET-11d-AΔ9-2, pET-11d-AΔ9-3, pET-11d-AΔ9-4, pET-11d-AΔ6-2, pET-11d-AΔ6-3 and pET-11d-AΔ6-4, were extracted. Table 5 shows names and Sequence ID NOs of the respective DNA fragments and PCR primers used in the amplification reaction. The 5′-primer was added with NcoI recognition sequence and the 3′-primer was added with BamHI recognition sequence. FIG. 4 shows relative position of the respective DNA fragments. In Table, SEQ ID NOs indicated in the column of DNA fragments denote amino acid sequences coded by the respective DNA fragments.

	TABLE 5
	DNA fragment	5′-primer	3′-primer
	AΔ5-1	AΔ5-1-P5	AΔ5-1-P3
	(SEQ ID NO: 1)	(SEQ ID NO: 14)	(SEQ ID NO: 15)
	AΔ5-2	AΔ5-1-P5	AΔ2-P3
	(SEQ ID NO: 27)	(SEQ ID NO: 14)	(SEQ ID NO: 38)
	AΔ5-3	AΔ5-1-P5	AΔ3-P3
	(SEQ ID NO: 28)	(SEQ ID NO: 14)	(SEQ ID NO: 39)
	AΔ5-4	AΔ5-1-P5	AΔ4-P3
	(SEQ ID NO: 29)	(SEQ ID NO: 14)	(SEQ ID NO: 40)
	AΔ9-2	AΔ9-P5	AΔ2-P3
	(SEQ ID NO: 30)	(SEQ ID NO: 36)	(SEQ ID NO: 38)
	AΔ9-3	AΔ9-P5	AΔ3-P3
	(SEQ ID NO: 31)	(SEQ ID NO: 36)	(SEQ ID NO: 39)
	AΔ9-4	AΔ9-P5	AΔ4-P3
	(SEQ ID NO: 32)	(SEQ ID NO: 36)	(SEQ ID NO: 40)
	AΔ6-2	AΔ6-P5	AΔ2-P3
	(SEQ ID NO: 33)	(SEQ ID NO: 37)	(SEQ ID NO: 38)
	AΔ6-3	AΔ6-P5	AΔ3-P3
	(SEQ ID NO: 34)	(SEQ ID NO: 37)	(SEQ ID NO: 39)
	AΔ6-4	AΔ6-P5	AΔ4-P3
	(SEQ ID NO: 35)	(SEQ ID NO: 37)	(SEQ ID NO: 40)

Next, CΔ5-1 obtained in Example 1 was digested with BamHI and, after separation by 0.8% agarose gel electrophoresis, the DNA fragments were eluted and recovered using Wizard SV Gel and PCR Clean-Up System (Promega). Further, the obtained fragments were linked in a forward orientation to pET-11d-AΔ5-1, pET-11d-AΔ5-2, pET-11d-AΔ5-3, pET-11d-AΔ5-4, pET-11d-AΔ9-2, pET-11d-AΔ9-3, pET-11d-AΔ9-4, pET-11d-AΔ6-2, pET-11d-AΔ6-3 and pET-11d-AΔ6-4 previously digested with BamHI. The resulting expression plasmids were used to transform E. coli BL21(DE3) strain (Merck) to give expression plasmids pET-11d-AΔ5-1-CΔ5-1, pET-11d-AΔ5-2-CΔ5-1, pET-11d-AΔ5-3-CΔ5-1, pET-11d-AΔ5-4-CΔ5-1, pET-11d-AΔ9-2-CΔ5-1, pET-11d-AΔ9-3-CΔ5-1, pET-11d-AΔ9-4-CΔ5-1, pET-11d-AΔ6-2-CΔ5-1, pET-11d-AΔ6-3-CΔ5-1 and pET-11d-AΔ6-4-CΔ5-1. In each of the constructed expression plasmids, CΔ5-1 was inserted directly downstream of the Peptide A expression gene in a forward orientation which produce the fusion peptides as shown in Table 6.

TABLE 6
Plasmid             Fusion peptide
pET-11d-AΔ5-1-CΔ5-1 ACΔ5-1 (SEQ ID NO: 9)
pET-11d-AΔ5-2-CΔ5-1 AΔ5-2/CΔ5-1 (SEQ ID NO: 41)
pET-11d-AΔ5-3-CΔ5-1 AΔ5-3/CΔ5-1 (SEQ ID NO: 42)
pET-11d-AΔ5-4-CΔ5-1 AΔ5-4/CΔ5-1 (SEQ ID NO: 43)
pET-11d-AΔ9-2-CΔ5-1 AΔ9-2/CΔ5-1 (SEQ ID NO: 44)
pET-11d-AΔ9-3-CΔ5-1 AΔ9-3/CΔ5-1 (SEQ ID NO: 45)
pET-11d-AΔ9-4-CΔ5-1 AΔ9-4/CΔ5-1 (SEQ ID NO: 46)
pET-11d-AΔ6-2-CΔ5-1 AΔ6-2/CΔ5-1 (SEQ ID NO: 47)
pET-11d-AΔ6-3-CΔ5-1 AΔ6-3/CΔ5-1 (SEQ ID NO: 48)
pET-11d-AΔ6-4-CΔ5-1 AΔ6-4/CΔ5-1 (SEQ ID NO: 49)

EXAMPLE 4

Construction of Plasmids for Expression of Shortened Fusion Peptides (2)

Genome DNA libraries of A.pg-C 53-47 strain were prepared as described in Example 1 to give the DNA fragments shown in Table 7. PCR conditions were as described in Example 3. Table 7 shows names and Sequence ID NOs of the respective DNA fragments and PCR primers used in the amplification reaction. Both the 5′-primer and the 3′-primer were added with BamHI recognition sequence. FIG. 5 Shows relative position of the respective DNA fragments. In Table, SEQ ID NOs indicated in the column of DNA fragments denote amino acid sequences coded by the respective DNA fragments.

	TABLE 7
	DNA fragment	5′-primer	3′-primer
	CΔ5-1	CΔ5-1-P5	CΔ4-5-P3
	(SEQ ID NO: 3)	(SEQ ID NO: 18)	(SEQ ID NO: 17)
	CΔ5-2	CΔ5-1-P5	CΔ2-P3
	(SEQ ID NO: 50)	(SEQ ID NO: 18)	(SEQ ID NO: 58)
	CΔ5-4	CΔ5-1-P5	CΔ4-P3
	(SEQ ID NO: 51)	(SEQ ID NO: 18)	(SEQ ID NO: 59)
	CΔ9-0	CΔ9-P5	CΔ0-P3
	(SEQ ID NO: 52)	(SEQ ID NO: 57)	(SEQ ID NO: 60)
	CΔ9-2	CΔ9-P5	CΔ2-P3
	(SEQ ID NO: 53)	(SEQ ID NO: 57)	(SEQ ID NO: 58)
	CΔ9-4	CΔ9-P5	CΔ4-P3
	(SEQ ID NO: 54)	(SEQ ID NO: 57)	(SEQ ID NO: 59)
	CΔ6-2	CΔ6b-1b-P5	CΔ2-P3
	(SEQ ID NO: 55)	(SEQ ID NO: 19)	(SEQ ID NO: 58)
	CΔ6-4	CΔ6b-1b-P5	CΔ4-P3
	(SEQ ID NO: 56)	(SEQ ID NO: 19)	(SEQ ID NO: 59)

Next, as described in Example 1, CΔ5-1, CΔ5-4, CΔ9-0, CΔ9-2, C9-4, CΔ6-2 and CΔ6-4 were digested with BamHI and, after separation by 0.8% agarose gel electrophoresis, the DNA fragments were eluted and recovered using Wizard SV Gel and PCR Clean-Up System (Promega). The obtained fragments were linked in a forward orientation to pET-11d-A5-1 previously digested with BamHI to give expression plasmids pET-11d-AΔ5-1-CΔ5-1, pET-11d-AΔ5-1-CΔ5-2, pET-11d-AΔ5-1-CΔ5-4, pET-11d-AΔ5-1-CΔ9-0, pET-11d-AΔ5-1-CΔ9-2, pET-11d-AΔ5-1-CΔ9-4, pET-11d-AΔ5-1-CΔ6-2 and pET-11d-AΔ5-1-CΔ-4. In each of the constructed expression plasmids, CΔ5-1, CΔ5-2, CΔ5-4, CΔ9-0, CΔ9-2, CΔ9-4, CΔ6-2 and CΔ6-4 were inserted directly downstream of AΔ5-1 in a forward orientation which produce the fusion peptides as shown in Table 8.

TABLE 8
Plasmid             Fusion peptide
pET-11d-AΔ5-1-CΔ5-1 ACΔ5-1 (SEQ ID NO: 12)
pET-11d-AΔ5-1-CΔ5-2 AΔ5-1/CΔ5-2 (SEQ ID NO: 61)
pET-11d-AΔ5-1-CΔ5-4 AΔ5-1/CΔ5-4 (SEQ ID NO: 62)
pET-11d-AΔ5-1-CΔ9-0 AΔ5-1/CΔ9-0 (SEQ ID NO: 63)
pET-11d-AΔ5-1-CΔ9-2 AΔ5-1/CΔ9-2 (SEQ ID NO: 64)
pET-11d-AΔ5-1-CΔ9-4 AΔ5-1/CΔ9-4 (SEQ ID NO: 65)
pET-11d-AΔ5-1-CΔ6-2 AΔ5-1/CΔ6-2 (SEQ ID NO: 66)
pET-11d-AΔ5-1-CΔ6-4 AΔ5-1/CΔ6-4 (SEQ ID NO: 67)

EXAMPLE 5

Construction of Plasmids for Expression of Peptide C

Genome DNA libraries of A.pg-C 53-47 strain were prepared as described in Example 1 to give DNA fragments similar to those shown in Table 7. PCR conditions were as described in Example 3. Names and Sequence ID NOs of the respective DNA fragments and PCR primers used in the amplification reaction were the same as in Table 7 with exception that a restriction enzyme recognition sequence in the 3′-primer was changed from BamHI recognition sequence to HindIII recognition sequence so that the amplified fragments may be inserted into expression vector pQE30 (QIAGEN) more efficiently.

Next, CΔ5-1, CΔ5-2, CΔ5-4, CΔ9-0, CΔ9-2, CΔ9-4, CΔ6-2 and CΔ6-4 were digested with BamHI and HindIII and, after separation by 0.8% agarose gel electrophoresis, the DNA fragments were eluted and recovered using Wizard SV Gel and PCR Clean-Up System (Promega). The obtained fragments were linked to expression vector pQE30 digested with BamHI and HindIII. The resulting expression plasmids were used to transform E. coli JM109 strain (QIAGEN) to give plasmids expressing CΔ5-1, CΔ5-2, CΔ5-4, CΔ9-0, CΔ9-2, CΔ9-4, CΔ6-2 and CΔ6-4. The amino acid sequences of peptides obtained from these expression plasmids are those coded by the respective DNA fragments shown in Table 7 with addition at their N-terminal of histidine tag sequence (MRGSHHHHHHGS) derived from the vectors.

EXAMPLE 6

Expression of Fusion Peptide (1)

E. coli BL21 (DE3) strain (Merck) possessing the respective expression plasmids obtained in Examples 1 and 2 were inoculated to 1 to 5 mL of LB medium containing 50 μg/mL ampicillin and shake cultured while shaking at 30 to 37° C. until OD₆₀₀ of the culture fluid reached 0.5. IPTG was then added at a final concentration of 1 mM and culture was continued for 3 hours. After centrifugation (Torry, MX-300, 9,100 g, 5 minutes), supernatant was discarded, a washing buffer (PBS) was added at an amount equivalent to the amount of the initial culture fluid and the cells were suspended to uniformity. The suspension was subject to sonication under ice cooling using handy sonicater (Torry, UR-20P) at power 10 for 10 seconds for ten times and centrifuged at 17,800 g for 15 minutes. The supernatant was isolated and to the precipitate was added, a washing buffer at an amount equivalent to the amount of the sonicated solution before centrifugation and the precipitate was suspended to uniformity. To each of the isolated supernatant and the precipitate was added an equivalent amount of a sample buffer (2×SDS) and, after heating in boiled water for 5 minutes, SDS-PAGE and staining with Coomassie Brilliant Blue were performed in the conventional manner. When the fusion peptides were observed in the precipitate suspension, it was judged that said fusion peptides formed an inclusion body. FIG. 3 shows the respective expression patterns.

When expressed alone, CΔ4c-1 was expressed in a soluble fraction and fraction of CΔ5-1 expression was not constant whereas all the fusion peptides were stably expressed as an inclusion body. Regarding an expression level, it was somewhat low for AΔ5-1/CΔ4c-1 and was almost equal to each other for the remaining two fusion peptides ACΔ5-1 and AΔ5-1/CΔ6b-1b with good expression. The fusion peptides with addition of linker showed an expression level equivalent to that of the fusion peptides without addition of linker.

EXAMPLE 7

Immunogenicity of Fusion Peptide (1)

To confirm the vaccine efficacy of the fusion peptides, a challenge test was carried out using homologous virulent strain. The inclusion bodies in the precipitate suspension of ACΔ5-1 and ACΔ5-1-L obtained in Example 6 were solubilized with 8M urea and the buffer was replaced with PBS (pH 7.4) using a dialysis membrane. A vaccine prepared by emulsifying ACΔ5-1 at the amount of antigen shown in Table 9 in 0.5 mL per dose with oil adjuvant was once administered intramuscularly to the leg of SPF chickens of 8 weeks old for immunization. As a control, group administered with commercially available oil-adjuvanted vaccine with inactivated cells (OILVAX NB₂AC, Juridical Foundation The Chemo-Sero-Therapeutic Research Institute) and group with no administration were set. Four weeks after immunization, 0.2 mL of a solution containing A.pg-A 221 strain (1.0×10¹⁰ CFU/mL) or A.pg-C 53-47 strain (3.0×10⁹ CFU/mL) was administered intranasally and clinical symptoms of a running nose, swelling of the face and epiphora were observed for a week.

As a result, as shown in Table 9, chicken administered with the fusion peptides exhibited excellent protective efficacy against challenge from A.pg-A 221 strain and A.pg-C 53-47 strain and even at 0.06 μg/dose, the vaccine efficacy was more than that of 1/1,000 amount of the commercially available oil adjuvant vaccine. The peptides with addition of linker also exhibited the same protective efficacy. Thus, the fusion peptides proved to be useful as a vaccine.

	TABLE 9
		Protective rate to
	Amount of	challenging strain
Vaccine	antigen	A.pg-A 221	A.gp-C 53-47
ACΔ5-1	6	μg/dose	100%	100%
	0.6	μg/dose	100%	100%
	0.06	μg/dose	100%	100%
ACΔ5-1-L	6	μg/dose	100%	100%
(with linker	0.6	μg/dose	100%	100%
addition)	0.06	μg/dose	100%	100%
OILVAX	1/10-fold	100%	100%
NB2 AC	1/100-fold	100%	100%
	1/1,000-fold	40%	20%
No immunized	—	0%	0%
control

EXAMPLE 8

Efficacy of Fusion Peptide to Heterologous Strain

To confirm the vaccine efficacy of the fusion peptides to the other strains (heterologous strains) than A.pg-A 221 strain and A.pg-C 53-47 strain used for preparing the fusion peptide, the challenge test was carried out as in Example 7. The procedures of Example 7 were repeated except that a different amount of antigen for immunization and different virulent strains, i.e. A.pg-A 083 strain (1.0×10⁹ CFU/mL), A.pg-A W strain (4.1×10⁹ CFU/mL) and A.pg-C Modesto strain (2.8×10⁹ CFU/mL), for challenge were used.

As a result, as shown in Table 10, chicken administered with the fusion peptides exhibited excellent protective efficacy against challenge from all the strains of A.pg-A 083, A.pg-A W and A.pg-C Modesto. Thus, the fusion peptides proved to be useful as a vaccine to other virulent strains from which the fusion peptides were not derived.

	TABLE 10
		Challenging	Amount of	Protection
	Vaccine	strain	antigen	rate
	Peptide A	A.pg-A 083	3	μg/dose	100%
	(AΔ5-1)		0.3	μg/dose	100%
			0.03	μg/dose	40%
		A.pg-A W	3	μg/dose	100%
			0.3	μg/dose	100%
			0.03	μg/dose	40%
	Fusion	A.pg-C	6	μg/dose	100%
	peptide	Modesto	0.6	μg/dose	100%
	(ACΔ5-1)		0.06	μg/dose	100%
	OILVAX	A.pg-A 083	1/10-fold	100%
	NB2 AC		1/100-fold	100%
			1/1,000-fold	20%
		A.pg-A W	1/10-fold	100%
			1/100-fold	80%
			1/1,000-fold	0%
		A.pg-A C	1/10-fold	100%
		Modesto	1/100-fold	80%
			1/1,000-fold	20%
	No immunized	A.pg-A 083	—	0%
	control	A.pg-A W	—	0%
		A.pg-C	—	0%
		Modesto

The respective strains used in the challenge test were analyzed for their nucleotide sequence of region 2. As a result, for A.pg-A, complete identity between 083 strain and W strain and 1 nucleotide mutation (A/G: glutamic acid at No. 1227 of SEQ ID NO: 25 is replaced with glycine) between 221 strain and 083 strain and between 221 strain and W strain were observed. For A.pg-C, deletion of 3 nucleotides AAG (glutamic acid at No. 1144 of SEQ ID NO: 26) was observed in Modesto strain as compared to 53-47 strain.

EXAMPLE 9

Comparison of Efficacy Between Fusion Peptide ACΔ5-1 and Respective Peptides

To compare the vaccine efficacy between the fusion peptide ACΔ5-1 and Peptide A or Peptide C before fusion, an immunization test was carried out. The vaccines were prepared as described in Example 7. A vaccine prepared by emulsifying ACΔ5-1, Peptide A or Peptide C at the amount of antigen shown in Table 11 in 0.5 mL per dose with oil adjuvant was once administered intramuscularly to the leg of SPF chickens of 4 weeks old for immunization. As a control, group with no administration was set. Four weeks after immunization, an antibody titer was determined as described by Ushijima et al. (Japanese patent application No. 2008-29589). Specifically, antibody measurement was carried out by ELISA.

The different peptides within Region 2 of A.pg-A and A.pg-C were diluted with 50 mM bicarbonate buffer to 1 μg/mL and each 50 μL of the solution was added to 96-well plate for immobilization. After adsorption at 4° C. overnight, the solution was discarded, and the plate was washed with 300 μL of PBS-T (8.1 mM disodium hydrogenphosphate, 1.5 mM potassium dihydrogenphosphate, 137 mM sodium chloride, 2.7 mM potassium chloride, 0.1% Tween 20) and added with 300 μL of PBS-T supplemented with 5% skim milk for blocking. The blocking solution was discarded. Serum was diluted with PBS-T supplemented with 10% skim milk to 100-fold and each 50 μL of the solution was added for reaction at room temperature for 1 hour. After removing the reaction solution, the plate was washed with PBS-T three times. An anti-chicken IgG-HRP-labeled antibody was diluted with PBS-T supplemented with 5% skim milk to 20,000-fold and each 50 μL of the solution was added to each well for reaction at room temperature for 30 minutes in the dark. After removing the reaction solution, the plate was washed with PBS-T three times. Each 100 μL of a substrate solution (TMB+substrate-chromogen: DAKO) was added for reaction at room temperature for 15 minutes. Each 100 μL of 3M sulfuric acid was added to stop the reaction. Absorbance at the wavelength of 450 nm was measured with 96-well plate reader (Molecular Devices Japan).

As a result, as shown in Table 11, the chicken immunized with the fusion peptide ACΔ5-1 exhibited a high antibody titer at 0.6 μg/dose and 100% of a positive conversion rate for both A.pg-A and A.pg-C. At 0.06 μg/dose of the fusion peptide, 80% and 40% of a positive conversion rate were observed for both A.pg-A _and A.pg-C, respectively. However, at 0.03 μg/dose of Peptide A or Peptide C, a positive conversion rate was 60% and 0% for A.pg-A and A.pg-C, respectively. Thus, it proved that the fusion peptide ACΔ5-1 had higher efficacy than Peptide A or Peptide C before fusion.

	TABLE 11
		Mean antibody titer
	Amount of	(positive conversion rate)
Vaccine	antigen	A.pg-A	A.pg-C
Fusion	6	μg/dose	2.152	(100%)	1.649	(100%)
peptide	0.6	μg/dose	1.924	(100%)	1.177	(100%)
(ACΔ5-1)	0.06	μg/dose	1.175	(80%)	0.565	(40%)
	0.006	μg/dose	0.514	(60%)	0.112	(0%)
Peptide A	3	μg/dose	2.051	(100%)	0.163	(0%)
(AΔ5-1)	0.3	μg/dose	2.197	(100%)	0.146	(0%)
	0.03	μg/dose	1.209	(60%)	0.086	(0%)
	0.003	μg/dose	0.080	(0%)	0.127	(0%)
Peptide C	3	μg/dose	0.153	(0%)	1.749	(100%)
(CΔ5-1)	0.3	μg/dose	0.176	(0%)	1.865	(100%)
	0.03	μg/dose	0.072	(0%)	0.089	(0%)
	0.003	μg/dose	0.072	(0%)	0.084	(0%)
No immunized	—	0.092	(0%)	0.099	(0%)
control

EXAMPLE 10

Expression of Fusion Peptide (2)

E. coli BL21 (DE3) strain (Merck) possessing the respective expression plasmids obtained in Examples 3 and 4 were subject to expression as described in Example 6 and an expression level was determined. FIGS. 6 and 7 show the respective expression patterns. For Peptide A, AΔ5-4, AΔ9-2, AΔ9-4, AΔ6-2 and AΔ6-4, when expressed alone, were expressed in a soluble fraction but, upon fusion with CΔ5-1, the resulting fusion peptides stably formed an inclusion body except for AΔ6-4. AΔ6-4/CΔ5-1, though principally formed an inclusion body, may sometimes be expressed in a soluble fraction and hence its expression was instable. All the fusion peptides had the same and excellent expression level. On the other hand, Peptide C, when expressed alone, was expressed in a soluble fraction except for CΔ6-2 but, upon fusion with AΔ5-1, the resulting fusion peptides stably formed an inclusion body. All the fusion peptides had the same and excellent expression level.

EXAMPLE 11

Immunogenicity of Fusion Peptide (2)

To confirm the vaccine efficacy of the fusion peptides obtained in Example 10, a challenge test was carried out using homologous virulent strain (A.pg-A 221 strain) as described in Example 7. The procedures of Example 7 were repeated except that a different amount of antigen for immunization and different number of cells of virulent strain, i.e. A.pg-A 221 strain, 1.2×10⁹ CFU/mL, for challenge were used. As a result, as shown in Table 12, chicken immunized with the respective fusion peptides exhibited excellent protective effects against challenge from A.pg-A 221 strain where 80% protection for AΔ6-4/CΔ5-1 and 100% protection for the longer fusion peptides were confirmed.

	TABLE 12
		Amount of	Protection
	Vaccine	antigen	rate
	ACΔ5-1	6 μg/dose	100%
	AΔ5-2/CΔ5-1	6 μg/dose	100%
	AΔ5-3/CΔ5-1	6 μg/dose	100%
	AΔ5-4/CΔ5-1	6 μg/dose	100%
	AΔ9-2/CΔ5-1	6 μg/dose	100%
	AΔ9-3/CΔ5-1	6 μg/dose	100%
	AΔ9-4/CΔ5-1	6 μg/dose	100%
	AΔ6-2/CΔ5-1	6 μg/dose	100%
	AΔ6-3/CΔ5-1	6 μg/dose	100%
	AΔ6-4/CΔ5-1	6 μg/dose	80%
	No immunized	—	0%
	control

EXAMPLE 12

Expression of Peptide C

E. coli JM109 (QIAGEN) possessing the respective expression plasmids obtained in Example 5 were subject to expression as described in Example 6 and an expression level for the respective cells was determined by SDS-PAGE (FIG. 8). The thus obtained peptides were named as CΔ5-1-pQE, CΔ5-2-pQE, CΔ5-4-pQE, CΔ9-0-pQE, CΔ9-2-pQE, CΔ9-4-pQE, CΔ6-2-pQ and CΔ6-4-pQE. All the peptides except for CΔ6-2-pQE were expressed in a soluble fraction with an excellent expression level.

EXAMPLE 13

Confirmation of Protective Effect of Peptide C

To confirm the vaccine effect of Peptides C obtained in Example 12, a challenge test was carried out as described in Example 7. A vaccine prepared by emulsifying Peptide C at the amount of antigen shown in Table 13 with oil adjuvant was once administered intramuscularly to the leg of SPF chickens of 4 weeks old for immunization. Four weeks after immunization, 0.2 mL of a solution containing A.pg-C 53-47 strain (5.2×10⁹ CFU/mL) was administered intranasally and clinical symptoms of a running nose, swelling of the face and epiphora were observed for a week.

As a result, as shown in Table 13, chicken administered with CΔ5-1-pQE and CΔ9-0-pQE exhibited excellent protective effects at 3 μg/dose. The protective effect of 60% was observed for the shortest CΔ6-4-pQE. From these results, it is expected that, for the protective effects to A.pg-C, a sequence at the C-terminal of non-homologous region (Region 2) in relation to A.pg-A is important and it was proved that a comparatively high protective effects were exhibited if the peptide includes at least the region of CΔ6-4. Furthermore, as shown in Example 9, it is expected that immunogenicity may be improved upon expression in fusion than expressed alone.

	TABLE 13
		Amount of	Protection
	Vaccine	antigen	rate
	CΔ5-1-pQE	3 μg/dose	100%
	CΔ9-0-pQE	3 μg/dose	100%
	CΔ9-2-pQE	3 μg/dose	60%
	CΔ6-4-pQE	3 μg/dose	60%
	No immunized	—	0%
	control

INDUSTRIAL APPLICABILITY

By using the present invention, a vaccine of avian infectious coryza caused by Avibacterium paragarinarum serotypes A and C may be provided.

Claims

1-19. (canceled)

20. A recombinant avian infectious coryza vaccine comprising as an active ingredient a peptide consisting of a sequence comprising the amino acid sequence shown by SEQ ID NO: 35, said sequence being within the amino acid sequence shown by SEQ ID NO: 1 with addition of 1 to 200 amino acid residues at the N-terminal and/or C-terminal thereof.

21. The vaccine of claim 20 wherein said vaccine comprises as an active ingredient a peptide consisting of the amino acid sequence shown by SEQ ID NO: 1.

22-23. (canceled)

24. The vaccine of claim 21 or 23 wherein said peptide comprises an amino acid sequence where one or several amino acids are deleted, added or replaced.