Analysis of the expression of cloned genes using an Escherichia coli cell-free system.

Y P See, B R Glick
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引用次数: 6

Abstract

An Escherichia coli coupled transcription-translation cell-free system, which is efficient in the synthesis of proteins directed by exogenously added DNA, is described. These cell-free extracts direct protein synthesis against a low background of endogenous protein synthesis providing a means for analyzing the expression of isolated genes. This is especially important when using restriction enzyme-linearized DNAs which are less efficient templates than circular DNAs. This cell-free system has been used to study the expression of the proteins coded by plasmids pBR322 and pBL101.

利用无细胞大肠杆菌系统分析克隆基因的表达。
描述了一种大肠杆菌偶联转录-翻译无细胞系统,它在由外源添加的DNA指导的蛋白质合成中是有效的。这些无细胞提取物直接蛋白质合成对抗低背景的内源性蛋白质合成提供了一种手段,分析分离基因的表达。当使用限制性内切酶线性化的dna时,这一点尤其重要,因为它比环状dna的模板效率低。该无细胞系统已被用于研究pBR322和pBL101质粒编码蛋白的表达。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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