Literature DB >> 12070324

High-throughput screening of soluble recombinant proteins.

Yan-Ping Shih1, Wen-Mei Kung, Jui-Chuan Chen, Chia-Hui Yeh, Andrew H-J Wang, Ting-Fang Wang.   

Abstract

The aims of high-throughput (HTP) protein production systems are to obtain well-expressed and highly soluble proteins, which are preferred candidates for use in structure-function studies. Here, we describe the development of an efficient and inexpensive method for parallel cloning, induction, and cell lysis to produce multiple fusion proteins in Escherichia coli using a 96-well format. Molecular cloning procedures, used in this HTP system, require no restriction digestion of the PCR products. All target genes can be directionally cloned into eight different fusion protein expression vectors using two universal restriction sites and with high efficiency (>95%). To screen for well-expressed soluble fusion protein, total cell lysates of bacteria culture ( approximately 1.5 mL) were subjected to high-speed centrifugation in a 96-tube format and analyzed by multiwell denaturing SDS-PAGE. Our results thus far show that 80% of the genes screened show high levels of expression of soluble products in at least one of the eight fusion protein constructs. The method is well suited for automation and is applicable for the production of large numbers of proteins for genome-wide analysis.

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Year:  2002        PMID: 12070324      PMCID: PMC2373646          DOI: 10.1110/ps.0205202

Source DB:  PubMed          Journal:  Protein Sci        ISSN: 0961-8368            Impact factor:   6.725


  11 in total

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Journal:  Nat Struct Biol       Date:  2000-10

6.  Sticky-end PCR: new method for subcloning.

Authors:  G Zeng
Journal:  Biotechniques       Date:  1998-08       Impact factor: 1.993

7.  The univector plasmid-fusion system, a method for rapid construction of recombinant DNA without restriction enzymes.

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Review 8.  Gene fusions for purpose of expression: an introduction.

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10.  Immunocytochemical demonstration of human proinsulin chimeric polypeptide within cytoplasmic inclusion bodies of Escherichia coli.

Authors:  D C Paul; R M Van Frank; W L Muth; J W Ross; D C Williams
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  57 in total

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Authors:  Yan-Ping Shih; Hui-Chung Wu; Su-Ming Hu; Ting-Fang Wang; Andrew H-J Wang
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Journal:  J Biomol NMR       Date:  2005-02       Impact factor: 2.835

4.  Effect of N-terminal solubility enhancing fusion proteins on yield of purified target protein.

Authors:  Martin Hammarström; Esmeralda A Woestenenk; Niklas Hellgren; Torleif Härd; Helena Berglund
Journal:  J Struct Funct Genomics       Date:  2006-07-19

5.  Fine-tuning of protein domain boundary by minimizing potential coiled coil regions.

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6.  Expression of membrane proteins from Mycobacterium tuberculosis in Escherichia coli as fusions with maltose binding protein.

Authors:  A Korepanova; J D Moore; H B Nguyen; Y Hua; T A Cross; F Gao
Journal:  Protein Expr Purif       Date:  2006-12-24       Impact factor: 1.650

7.  Enzyme free cloning for high throughput gene cloning and expression.

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8.  Gateway vectors for the production of combinatorially-tagged His6-MBP fusion proteins in the cytoplasm and periplasm of Escherichia coli.

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Journal:  Protein Sci       Date:  2005-12       Impact factor: 6.725

9.  High-throughput expression of C. elegans proteins.

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10.  Design, expression, and purification of a Flaviviridae polymerase using a high-throughput approach to facilitate crystal structure determination.

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Journal:  Protein Sci       Date:  2004-10       Impact factor: 6.725

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