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Elimination of truncated recombinant protein expressed in E. coli by removing cryptic translation initiation site.

Protein Expr Purif.. 2016-05; 
MJ Jennings, AF Barrios, S Tan.
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Catalog Antibody ... Western blotting was performed using anti-Gcn5 antibodies (custom antibodies by Cocalico Biologicals, Reamstown, PA) or anti-HIS antibodies (GenScript, Piscataway, NJ). Acknowledgements. We thank David Garboczi (NIH) for sharing unpublished results. ... Get A Quote

摘要

Undesirable truncated recombinant protein products pose a special expression and purification challenge because such products often share similar chromatographic properties as the desired full length protein. We describe here our observation of both full length and a truncated form of a yeast protein (Gcn5) expressed in Escherichia coli, and the reduction or elimination of the truncated form by mutating a cryptic Shine-Dalgarno or START codon within the Gcn5 coding region. Unsuccessful attempts to engineer in a cryptic translation initiation site into other recombinant proteins suggest that cryptic Shine-Dalgarno or START codon sequences are necessary but not sufficient for cryptic translation in E. coli.

关键词

Cryptic initiation; Escherichia coli expression; Recombinant protein expression
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