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Enhancing functional production of a chaperone-dependent lipase in Escherichia coli using the dual expression cassette plasmid

机译:使用双重表达盒质粒增强大肠杆菌中伴侣蛋白依赖性脂肪酶的功能性生产

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摘要

AbstractsBackgroundThe lipase subfamilies I.1 and I.2 show more than 33% homology in the amino acid sequences and most members share another common property that their genes are clustered with the secondary genes whose protein products are required for folding the lipase into an active conformation and secretion into the culture medium. In previous studies, the lipase (LipA) and its chaperone (LipB) from Ralstonia sp. M1 were overexpressed in E. coli and the lipase was successfully refolded in vitro. The purpose of this study was to enhance the production of the active lipase LipA from Ralstonia sp. M1 in the heterologous host E. coli without in vitro refolding process, using two-plasmid co-expression systems and dual expression cassette plasmid systems.
机译:摘要背景脂肪酶亚家族I.1和I.2在氨基酸序列中具有超过33%的同源性,并且大多数成员具有另一个共同的特性,即它们的基因与次级基因聚集在一起,次级基因的蛋白质产物是将脂肪酶折叠成活性构象所必需的并分泌到培养基中在以前的研究中,来自Ralstonia sp。的脂肪酶(LipA)及其分子伴侣(LipB)。 M1在大肠杆菌中过表达,脂肪酶在体外成功折叠。这项研究的目的是提高来自Ralstonia sp。的活性脂肪酶LipA的产生。使用双质粒共表达系统和双表达盒质粒系统,无需体外重折叠过程即可在异源宿主大肠杆菌中产生M1。

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