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N(pro) fusion technology to produce proteins with authentic N termini in E. coli.

N(pro) fusion technology to produce proteins with authentic N termini in E. coli. Research Abstract Details 

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  • N(pro) fusion technology to produce proteins with authentic N termini in E. coli. Abstract Text:

    clemens Clemens ,waltraud kaarWaltraud Kaar,karin ahrerKarin Ahrer,philipp wechnerPhilipp Wechner,rainer hahnRainer Hahn,florian wertherFlorian Werther,hannes schmidingerHannes Schmidinger,monika cserjan-puschmannMonika Cserjan-Puschmann,franz clementschitschFranz Clementschitsch,gerald striednerGerald Striedner,karl bayerKarl Bayer,alois jungbauerAlois Jungbauer,bernhard auerBernhard Auer,clemens Clemens ,waltraud kaarWaltraud Kaar,karin ahrerKarin Ahrer,philipp wechnerPhilipp Wechner,rainer hahnRainer Hahn,florian wertherFlorian Werther,hannes schmidingerHannes Schmidinger,monika cserjan-puschmannMonika Cserjan-Puschmann,franz clementschitschFranz Clementschitsch,gerald striednerGerald Striedner,karl bayerKarl Bayer,alois jungbauerAlois Jungbauer,bernhard auerBernhard Auer,

    We describe a prokaryotic expression system using the autoproteolytic function of N(pro) from classical swine fever virus. Proteins or peptides expressed as N(pro) fusions are deposited as inclusion bodies. On in vitro refolding by switching from chaotropic to kosmotropic conditions, the fusion partner is released from the C-terminal end of the autoprotease by self-cleavage, leaving the target protein with an authentic N terminus. A tailor-made N(pro) mutant called EDDIE, with increased in vitro and decreased in vivo cleavage rates, has enabled us to express proinsulin, domain-D of staphylococcal protein A, hepcidin, interferon-alpha1, keratin-associated protein 10-4, green fluorescent protein, inhibitorial peptide of senescence-evasion-factor, monocyte chemoattractant protein-1 and toxic gyrase inhibitor, among others. This N(pro) expression system can be used as a generic tool for the high-level production of recombinant toxic peptides and proteins (up to 12 g/l) in Escherichia coli without the need for chemical or enzymatic removal of the fusion tag.

    N(pro) fusion technology to produce proteins with authentic N termini in E. coli. Publishing Authors By Initials

    c C ,w kaarW Kaar,k ahrerK Ahrer,p wechnerP Wechner,r hahnR Hahn,f wertherF Werther,h schmidingerH Schmidinger,m cserjan-puschmannM Cserjan-Puschmann,f clementschitschF Clementschitsch,g striednerG Striedner,k bayerK Bayer,a jungbauerA Jungbauer,b auerB Auer,c C ,w kaarW Kaar,k ahrerK Ahrer,p wechnerP Wechner,r hahnR Hahn,f wertherF Werther,h schmidingerH Schmidinger,m cserjan-puschmannM Cserjan-Puschmann,f clementschitschF Clementschitsch,g striednerG Striedner,k bayerK Bayer,a jungbauerA Jungbauer,b auerB Auer,

    For similar abstracts research abstracts see: abstracts research

    PUBMED ID PMID:

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    N(pro) fusion technology to produce proteins with authentic N termini in E. coli. Journal Published:

    PUBLICATION TYPE: Research Support, Non-U.S. Gov

    Journal: Nature methods

    VOLUME: 4

    Page Numbers: 1037-43

    Journal Abbreviation: Nat. Methods

    ISSN: 1548-7105

    DAY: 18

    MONTH: 11

    YEAR: 2007

    N(pro) fusion technology to produce proteins with authentic N termini in E. coli. Information

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    LANGUAGE: eng

    NlmUniqueID: 101215604

    N(pro) fusion technology to produce proteins with authentic N termini in E. coli. Keywords Mesh Terms:

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    Grant and Affiliation Information for N(pro) fusion technology to produce proteins with authentic N termini in E. coli.

    AFFILIATION: Austrian Center of Biopharmaceutical Technology, Muthgasse 18, A-1190 Vienna, Austria.

    Country: United States

    United States Research PublicationUnited States Research Publication

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    MEDLINETA: Nat Methods

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