Literature DB >> 12182816

A micro-scale process for high-throughput expression of cDNAs in the yeast Saccharomyces cerevisiae.

Caterina Holz1, Oliver Hesse, Natalia Bolotina, Ulf Stahl, Christine Lang.   

Abstract

Methods have been developed aimed at applying at high-throughput technology for expression of cloned cDNAs in yeast. Yeast is a eukaryotic host, which produces soluble recombinant proteins and is capable of introducing post-translational modifications of protein. It is, thus, an appropriate expression system both for the routine expression of various cDNAs or protein domains and for the expression of proteins, which are not correctly expressed in Escherichia coli. Here, we describe a standard system in Saccharomyces cerevisiae, based on a vector for intracellular protein expression, where the gene products are fused to specific peptide sequences (tags). These epitope tags, the N-terminal His(6) tag and the C-terminal StrepII tag, allow subsequent immunological identification and purification of the gene products by a two-step affinity chromatography. This method of dual-tagged recombinant protein purification eliminates contamination by degraded protein products. A miniaturization of the procedures for cloning, expression, and detection was performed to allow all steps to be carried out in 96-well microtiter plates. The system is, thus, suitable for automation. We were able to analyze the simultaneous protein expression of a large number of cDNA clones due to the highly parallel approach of protein production and purification. The microtiter plate technology format was extended to quantitative analysis. An ELISA-based assay was developed that detects StrepII-tagged proteins. The application of this high-throughput expression system for protein production will be a useful tool for functional and structural analyses of novel genes, identified by the Human Genome Project and other large-scale sequencing projects.

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Year:  2002        PMID: 12182816     DOI: 10.1016/s1046-5928(02)00029-3

Source DB:  PubMed          Journal:  Protein Expr Purif        ISSN: 1046-5928            Impact factor:   1.650


  15 in total

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Review 2.  Protein production and purification.

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Journal:  Nat Methods       Date:  2008-02       Impact factor: 28.547

3.  Purification by Strep-Tactin affinity chromatography of a delete envelope gp51 protein of Bovine Leukaemia virus expressed in Sf21 insect cells.

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4.  Rapid one-step protein purification from plant material using the eight-amino acid StrepII epitope.

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Authors:  Gavin C Barnard; Angela R Kull; Nathan S Sharkey; Seemab S Shaikh; Alissa M Rittenhour; Irina Burnina; Youwei Jiang; Fang Li; Heather Lynaugh; Teresa Mitchell; Juergen H Nett; Adam Nylen; Thomas I Potgieter; Bianka Prinz; Sandra E Rios; Dongxing Zha; Natarajan Sethuraman; Terrance A Stadheim; Piotr Bobrowicz
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Authors:  Andrew P Turnbull; Daniel Kümmel; Bianka Prinz; Caterina Holz; Jeffrey Schultchen; Christine Lang; Frank H Niesen; Klaus-Peter Hofmann; Heinrich Delbrück; Joachim Behlke; Eva-Christina Müller; Ernst Jarosch; Thomas Sommer; Udo Heinemann
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9.  Establishing a versatile fermentation and purification procedure for human proteins expressed in the yeasts Saccharomyces cerevisiae and Pichia pastoris for structural genomics.

Authors:  Bianka Prinz; Jeffrey Schultchen; Ralf Rydzewski; Caterina Holz; Mewes Boettner; Ulf Stahl; Christine Lang
Journal:  J Struct Funct Genomics       Date:  2004

10.  Establishing the yeast Saccharomyces cerevisiae as a system for expression of human proteins on a proteome-scale.

Authors:  Caterina Holz; Bianka Prinz; Natalia Bolotina; Volker Sievert; Konrad Büssow; Bernd Simon; Ulf Stahl; Christine Lang
Journal:  J Struct Funct Genomics       Date:  2003
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