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Gateway-compatible vectors for high-throughput protein expression in pro- and eukaryotic cell-free systems.

J Biotechnol.. 2014-12;  195C:1-7
Gagoski D, Mureev S, Giles N, Johnston W, Dahmer-Heath M, ?kalamera D, Gonda TJ, Alexandrov K. Institute for Molecular Bioscience, University of Queensland, Australia.
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摘要

Although numerous techniques for protein expression and production are available the pace of genome sequencing outstrips our ability to analyze the encoded proteins. To address this bottleneck, we have established a system for parallelized cloning, DNA production and cell-free expression of large numbers of proteins. This system is based on a suite of pCellFree Gateway destination vectors that utilize a Species Independent Translation Initiation Sequence (SITS) that mediates recombinant protein expression in any in vitro translation system. These vectors introduce C or N terminal EGFP and mCherry fluorescent and affinity tags, enabling direct analysis and purification of the expressed proteins. To maximize thro... More

关键词

Gateway cloning; Cell-free protein expression; Species Independent Translation Initiation Sequence; Rolling Circle DNA Amplification