A synthetic translation-terminator gene

Ichiro N. Maruyama , Kazuhiro Horikoshi , Yasukazu Nagase , Masaaki Soma , Masahiro Nobuhara , Seiichi Yasuda , Yukinori Hirota
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引用次数: 2

Abstract

A 41-nucleotide-long duplex DNA, which contains the translation termination codon TAA in six reading frames and lactose operator sequence of Escherichiacoli, has been synthesized. This fragment may be useful not only for producing a truncated protein encoded in a plasmid, but also for the identification of the precise coding region and translation direction of a bacterial gene in the cloned chromosomal segment. The synthetic fragment was inserted into ß-lactamase structural gene in pBR322 in order to test the in vivo activity. The plasmid produced mutant ß-lactamase reduced in size, as expected from the insertion site, and rendered the host bacterium constitutive for ß-galactosidase. Thus, termination codons and lactose operator in synthetic nucleotide appear to be functional in vivo.

合成的翻译终止基因
合成了一个41核苷酸长的双链DNA,该DNA包含六个阅读框中的翻译终止密码子TAA和Escherichiacoli的乳糖操作子序列。该片段不仅可用于产生质粒中编码的截短蛋白,而且可用于鉴定克隆染色体片段中细菌基因的精确编码区和翻译方向。将合成片段插入pBR322中的ß-内酰胺酶结构基因中,以检测其体内活性。质粒产生的突变型ß-内酰胺酶的大小如从插入位点预期的那样减小,并使宿主细菌成为ß;-半乳糖苷酶的组成部分。因此,合成核苷酸中的终止密码子和乳糖操作子似乎在体内具有功能。
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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