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首页> 外文期刊>Proceedings of the National Academy of Sciences of the United States of America >TRANSCRIBING OF ESCHERICHIA COLI GENES WITH MUTANT T7 RNA POLYMERASES - STABILITY OF LACZ MRNA INVERSELY CORRELATES WITH POLYMERASE SPEED
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TRANSCRIBING OF ESCHERICHIA COLI GENES WITH MUTANT T7 RNA POLYMERASES - STABILITY OF LACZ MRNA INVERSELY CORRELATES WITH POLYMERASE SPEED

机译:突变T7 RNA聚合酶转化大肠埃希氏菌基因-Lacz MRNA的稳定性与聚合酶速度反向相关。

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摘要

When in Escherichia coil the host RNA polymerase is replaced by the 8-fold faster bacteriophage T7 enzyme for transcription of the lacZ gene, the beta-galactosidase yield per transcript drops as a result of transcript destabilization, We have measured the beta-galactosidase yield per transcript from T7 RNA polymerase mutants that exhibit a reduced elongation speed in vitro. Aside from very slow mutants that were not sufficiently processive to transcribe the lacZ gene, the lower the polymerase speed, the higher the beta-galactosidase yield per transcript, In particular, a mutant, which was 2.7-fold slower than the wild-type enzyme yielded 3.4- to 4.6-fold more beta-galactosidase per transcript, These differences in yield vanished in the presence of the rne-50 mutation and therefore reflect the unequal sensitivity of the transcripts to RNase E, We propose that the instability of the T7 RNA polymerase transcripts stems from the unmasking of an RNase E-sensitive site(s) between the polymerase and the leading ribosome: the faster the polymerase, the longer the lag between the synthesis of this site(s) and its shielding by ribosomes, and the lower the transcript stability.
机译:当在大肠杆菌中,宿主RNA聚合酶被快8倍的噬菌体T7酶替代lacZ基因的转录时,由于转录不稳定,每个转录本的β-半乳糖苷酶产率下降。 T7 RNA聚合酶突变体的转录本,在体外表现出降低的延伸速度。除了非常慢的突变体,其不足以进行lacZ基因的转录,聚合酶速度越低,每个转录本的β-半乳糖苷酶产量就越高,特别是突变体,它比野生型酶慢2.7倍产生每个转录本3.4-4.6倍的β-半乳糖苷酶,这些产率差异在rne-50突变的存在下消失,因此反映了转录本对RNase E的不平等敏感性,我们建议T7 RNA的不稳定性聚合酶转录本源自聚合酶和主要核糖体之间的RNase E敏感位点的不暴露:聚合酶越快,该位点的合成与其被核糖体屏蔽之间的滞后时间就越长,并且降低笔录稳定性。

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