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A novel PCR-based method for high throughput prokaryotic expression of antimicrobial peptide genes
BACKGROUND: To facilitate the screening of large quantities of new antimicrobial peptides (AMPs), we describe a cost-effective method for high throughput prokaryotic expression of AMPs. EDDIE, an autoproteolytic mutant of the N-terminal autoprotease, Npro, from classical swine fever virus, was selec...
| Autores principales: | , , , , , , , , , , |
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| Formato: | Online Artículo Texto |
| Lenguaje: | English |
| Publicado: |
BioMed Central
2012
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| Materias: | |
| Acceso en línea: | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3350388/ https://www.ncbi.nlm.nih.gov/pubmed/22439858 http://dx.doi.org/10.1186/1472-6750-12-10 |
| _version_ | 1782232652318769152 |
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| author | Ke, Tao Liang, Su Huang, Jin Mao, Han Chen, Jibao Dong, Caihua Huang, Junyan Liu, Shengyi Kang, Jianxiong Liu, Dongqi Ma, Xiangdong |
| author_facet | Ke, Tao Liang, Su Huang, Jin Mao, Han Chen, Jibao Dong, Caihua Huang, Junyan Liu, Shengyi Kang, Jianxiong Liu, Dongqi Ma, Xiangdong |
| author_sort | Ke, Tao |
| collection | PubMed |
| description | BACKGROUND: To facilitate the screening of large quantities of new antimicrobial peptides (AMPs), we describe a cost-effective method for high throughput prokaryotic expression of AMPs. EDDIE, an autoproteolytic mutant of the N-terminal autoprotease, Npro, from classical swine fever virus, was selected as a fusion protein partner. The expression system was used for high-level expression of six antimicrobial peptides with different sizes: Bombinin-like peptide 7, Temporin G, hexapeptide, Combi-1, human Histatin 9, and human Histatin 6. These expressed AMPs were purified and evaluated for antimicrobial activity. RESULTS: Two or four primers were used to synthesize each AMP gene in a single step PCR. Each synthetic gene was then cloned into the pET30a/His-EDDIE-GFP vector via an in vivo recombination strategy. Each AMP was then expressed as an Npro fusion protein in Escherichia coli. The expressed fusion proteins existed as inclusion bodies in the cytoplasm and the expression levels of the six AMPs reached up to 40% of the total cell protein content. On in vitro refolding, the fusion AMPs was released from the C-terminal end of the autoprotease by self-cleavage, leaving AMPs with an authentic N terminus. The released fusion partner was easily purified by Ni-NTA chromatography. All recombinant AMPs displayed expected antimicrobial activity against E. coli, Micrococcus luteus and S. cerevisia. CONCLUSIONS: The method described in this report allows the fast synthesis of genes that are optimized for over-expression in E. coli and for the production of sufficiently large amounts of peptides for functional and structural characterization. The Npro partner system, without the need for chemical or enzymatic removal of the fusion tag, is a low-cost, efficient way of producing AMPs for characterization. The cloning method, combined with bioinformatic analyses from genome and EST sequence data, will also be useful for screening new AMPs. Plasmid pET30a/His-EDDIE-GFP also provides green/white colony selection for high-throughput recombinant AMP cloning. |
| format | Online Article Text |
| id | pubmed-3350388 |
| institution | National Center for Biotechnology Information |
| language | English |
| publishDate | 2012 |
| publisher | BioMed Central |
| record_format | MEDLINE/PubMed |
| spelling | pubmed-33503882012-05-12 A novel PCR-based method for high throughput prokaryotic expression of antimicrobial peptide genes Ke, Tao Liang, Su Huang, Jin Mao, Han Chen, Jibao Dong, Caihua Huang, Junyan Liu, Shengyi Kang, Jianxiong Liu, Dongqi Ma, Xiangdong BMC Biotechnol Methodology Article BACKGROUND: To facilitate the screening of large quantities of new antimicrobial peptides (AMPs), we describe a cost-effective method for high throughput prokaryotic expression of AMPs. EDDIE, an autoproteolytic mutant of the N-terminal autoprotease, Npro, from classical swine fever virus, was selected as a fusion protein partner. The expression system was used for high-level expression of six antimicrobial peptides with different sizes: Bombinin-like peptide 7, Temporin G, hexapeptide, Combi-1, human Histatin 9, and human Histatin 6. These expressed AMPs were purified and evaluated for antimicrobial activity. RESULTS: Two or four primers were used to synthesize each AMP gene in a single step PCR. Each synthetic gene was then cloned into the pET30a/His-EDDIE-GFP vector via an in vivo recombination strategy. Each AMP was then expressed as an Npro fusion protein in Escherichia coli. The expressed fusion proteins existed as inclusion bodies in the cytoplasm and the expression levels of the six AMPs reached up to 40% of the total cell protein content. On in vitro refolding, the fusion AMPs was released from the C-terminal end of the autoprotease by self-cleavage, leaving AMPs with an authentic N terminus. The released fusion partner was easily purified by Ni-NTA chromatography. All recombinant AMPs displayed expected antimicrobial activity against E. coli, Micrococcus luteus and S. cerevisia. CONCLUSIONS: The method described in this report allows the fast synthesis of genes that are optimized for over-expression in E. coli and for the production of sufficiently large amounts of peptides for functional and structural characterization. The Npro partner system, without the need for chemical or enzymatic removal of the fusion tag, is a low-cost, efficient way of producing AMPs for characterization. The cloning method, combined with bioinformatic analyses from genome and EST sequence data, will also be useful for screening new AMPs. Plasmid pET30a/His-EDDIE-GFP also provides green/white colony selection for high-throughput recombinant AMP cloning. BioMed Central 2012-03-23 /pmc/articles/PMC3350388/ /pubmed/22439858 http://dx.doi.org/10.1186/1472-6750-12-10 Text en Copyright ©2012 Ke et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. |
| spellingShingle | Methodology Article Ke, Tao Liang, Su Huang, Jin Mao, Han Chen, Jibao Dong, Caihua Huang, Junyan Liu, Shengyi Kang, Jianxiong Liu, Dongqi Ma, Xiangdong A novel PCR-based method for high throughput prokaryotic expression of antimicrobial peptide genes |
| title | A novel PCR-based method for high throughput prokaryotic expression of antimicrobial peptide genes |
| title_full | A novel PCR-based method for high throughput prokaryotic expression of antimicrobial peptide genes |
| title_fullStr | A novel PCR-based method for high throughput prokaryotic expression of antimicrobial peptide genes |
| title_full_unstemmed | A novel PCR-based method for high throughput prokaryotic expression of antimicrobial peptide genes |
| title_short | A novel PCR-based method for high throughput prokaryotic expression of antimicrobial peptide genes |
| title_sort | novel pcr-based method for high throughput prokaryotic expression of antimicrobial peptide genes |
| topic | Methodology Article |
| url | https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3350388/ https://www.ncbi.nlm.nih.gov/pubmed/22439858 http://dx.doi.org/10.1186/1472-6750-12-10 |
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