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大肠杆菌中转录错误的频率在很大程度上由tRNA竞争决定。

The frequency of translational misreading errors in E. coli is largely determined by tRNA competition.

作者信息

Kramer Emily B, Farabaugh Philip J

机构信息

Department of Biological Sciences and Program in Molecular and Cell Biology, University of Maryland, Baltimore, Maryland 21250, USA.

出版信息

RNA. 2007 Jan;13(1):87-96. doi: 10.1261/rna.294907. Epub 2006 Nov 9.

Abstract

Estimates of missense error rates (misreading) during protein synthesis vary from 10(-3) to 10(-4) per codon. The experiments reporting these rates have measured several distinct errors using several methods and reporter systems. Variation in reported rates may reflect real differences in rates among the errors tested or in sensitivity of the reporter systems. To develop a more accurate understanding of the range of error rates, we developed a system to quantify the frequency of every possible misreading error at a defined codon in Escherichia coli. This system uses an essential lysine in the active site of firefly luciferase. Mutations in Lys529 result in up to a 1600-fold reduction in activity, but the phenotype varies with amino acid. We hypothesized that residual activity of some of the mutant genes might result from misreading of the mutant codons by tRNA(Lys) (UUUU), the cognate tRNA for the lysine codons, AAA and AAG. Our data validate this hypothesis and reveal details about relative missense error rates of near-cognate codons. The error rates in E. coli do, in fact, vary widely. One source of variation is the effect of competition by cognate tRNAs for the mutant codons; higher error frequencies result from lower competition from low-abundance tRNAs. We also used the system to study the effect of ribosomal protein mutations known to affect error rates and the effect of error-inducing antibiotics, finding that they affect misreading on only a subset of near-cognate codons and that their effect may be less general than previously thought.

摘要

蛋白质合成过程中错义错误率(误读)的估计值为每个密码子10^(-3)至10^(-4)。报告这些错误率的实验使用了多种方法和报告系统来测量几种不同的错误。报告的错误率差异可能反映了所测试错误之间实际的错误率差异,或者报告系统的敏感性差异。为了更准确地了解错误率范围,我们开发了一种系统,用于量化大肠杆菌中特定密码子处每种可能的误读错误的频率。该系统利用萤火虫荧光素酶活性位点中的一个必需赖氨酸。Lys529的突变导致活性降低多达1600倍,但表型因氨基酸而异。我们假设一些突变基因的残余活性可能是由于赖氨酸密码子AAA和AAG的同源tRNA即tRNA(Lys)(UUUU)对突变密码子的误读所致。我们的数据验证了这一假设,并揭示了近义密码子相对错义错误率的细节。实际上,大肠杆菌中的错误率差异很大。差异的一个来源是同源tRNA对突变密码子的竞争效应;低丰度tRNA的竞争较低会导致更高的错误频率。我们还使用该系统研究了已知会影响错误率的核糖体蛋白突变的影响以及诱导错误的抗生素的影响,发现它们仅对一部分近义密码子的误读有影响,并且它们的影响可能不如先前认为的那么普遍。

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