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Overexpression of outer membrane porins in E. coli using pBluescript-derived vectors.

机译:使用pBluescript衍生的载体在大肠杆菌中过度表达外膜孔蛋白。

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摘要

The genes coding for four major outer membrane porins of Escherichia coli, ompF, ompC, phoE, and lamB, have been cloned into pBluescript-derived vectors and overexpressed to very high level (approximately 80% of the total membrane protein) in widely used host strains lacking one or more porins. For OmpF, OmpC, and PhoE porins it is shown that, contrary to current dogma, the genes can be overexpressed without undue deleterious effects upon cell growth and are stable, even under conditions of continuous expression. In contrast, overexpression of LamB is toxic to cell growth, but can be performed using tightly regulated lac promotor-driven expression. The vectors described allow overexpression, sequencing, and mutagenesis to be performed using a single system, without the necessity of subcloning, thus simplifying genetic manipulation. A particular advantage of these new vectors (with the exception of the vector for LamB) is that they do not require a particular regime for inducing the recombinant protein. To our knowledge, this study is the only comparative study of widely used membrane porin expression systems and the first to show that several porins can be stably expressed individually and maintained on high copy number vectors.
机译:已将编码大肠杆菌,ompF,ompC,phoE和lamB的四种主要外膜孔蛋白的基因克隆到pBluescript衍生的载体中,并在广泛使用的宿主中过表达至很高水平(约占总膜蛋白的80%)缺乏一种或多种孔蛋白的菌株。对于OmpF,OmpC和PhoE孔蛋白,与目前的教条相反,该基因可以过表达,而对细胞生长没有过度的有害影响,并且即使在连续表达的条件下也稳定。相反,LamB的过表达对细胞生长有毒性,但是可以使用受到严格调控的lac启动子驱动的表达来执行。所描述的载体允许使用单个系统进行过表达,测序和诱变,而无需亚克隆,从而简化了基因操作。这些新载体的特殊优势(LamB载体除外)是它们不需要用于诱导重组蛋白的特定方案。据我们所知,该研究是广泛使用的膜孔蛋白表达系统的唯一比较研究,并且是第一个表明几种孔蛋白可以单独稳定表达并维持在高拷贝数载体上的研究。

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