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改变tRNA2Gly肘部区域的突变会降低T4基因60的翻译跳跃效率。

Mutations which alter the elbow region of tRNA2Gly reduce T4 gene 60 translational bypassing efficiency.

作者信息

Herr A J, Atkins J F, Gesteland R F

机构信息

Department of Human Genetics, 15N 2030 E RM 6160, University of Utah, Salt Lake City, UT 84112-5330, USA.

出版信息

EMBO J. 1999 May 17;18(10):2886-96. doi: 10.1093/emboj/18.10.2886.

Abstract

Translating ribosomes bypass a 50 nucleotide coding gap in bacteriophage T4 gene 60 mRNA between codons 46 and 47 in order to synthesize the full-length protein. Bypassing of the coding gap requires peptidyl-tRNA2Gly detachment from a GGA codon (codon 46) followed by re-pairing at a matching GGA codon just before codon 47. Using negative selection, based on the sacB gene from Bacillus subtilis, Escherichia coli mutants were isolated which reduce bypassing efficiency. All of the mutations are in the gene for tRNA2Gly. Most of the mutations disrupt the hydrogen bonding interactions between the D- and T-loops (G18psi55 and G19C56) which stabilize the elbow region in nearly all tRNAs. The lone mutation not in the elbow region destabilizes the anticodon stem at position 40. Previously described Salmonella typhimurium mutants of tRNA2Gly, which reduce the stability of the T-loop, were also tested and found to decrease bypassing efficiency. Each tRNA2Gly mutant is functional in translation (tRNA2Gly is essential), but has a decoding efficiency 10- to 20-fold lower than wild-type. This suggests that rigidity of the elbow region and the anticodon stem is critical for both codon-anticodon stability and bypassing.

摘要

在噬菌体T4基因60 mRNA中,密码子46和47之间存在一个50个核苷酸的编码间隙,核糖体通过跳跃该间隙来合成全长蛋白质。跳跃编码间隙需要肽基 - tRNA2Gly从GGA密码子(密码子46)上脱离,然后在密码子47之前的一个匹配GGA密码子处重新配对。利用基于枯草芽孢杆菌sacB基因的负筛选方法,分离出了降低跳跃效率的大肠杆菌突变体。所有突变都发生在tRNA2Gly基因中。大多数突变破坏了D环和T环之间的氢键相互作用(G18ψ55和G19C56),而这种相互作用在几乎所有tRNA中都能稳定其肘部区域。唯一不在肘部区域的突变使40位的反密码子茎不稳定。之前描述的降低T环稳定性的鼠伤寒沙门氏菌tRNA2Gly突变体也经过测试,发现其跳跃效率降低。每个tRNA2Gly突变体在翻译中都有功能(tRNA2Gly是必需的),但其解码效率比野生型低10到20倍。这表明肘部区域和反密码子茎的刚性对于密码子 - 反密码子稳定性和跳跃都是至关重要的。

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