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tRNAIle氨基酰化过程中动力学校正的直接实验证据。

Direct experimental evidence for kinetic proofreading in amino acylation of tRNAIle.

作者信息

Hopfield J J, Yamane T, Yue V, Coutts S M

出版信息

Proc Natl Acad Sci U S A. 1976 Apr;73(4):1164-8. doi: 10.1073/pnas.73.4.1164.

Abstract

Kinetic proofreading is a reaction scheme with a structure more complicated than that of Michaelis kinetics, which leads to a proofreading for errors in the recognition of a correct substrate by an enzyme. We have measured the stoichiometry between ATP hydrolysis and tRNAIle charging, using the enzyme isoleucyl-tRNA synthetase [L-isoleucine:tRNAIle ligase (AMP-forming), EC 6.1.1.5] and the amino acids isoleucine (correct) and valine (incorrect). The enzymatic deacylation of charged tRNA, which would normally prevent meaningful stoichiometry studies, was eliminated by the use of transfer factor Tu-GTP, (which binds strongly to charged tRNA) in the reaction mixture. For isoleucine, 1.5 ATP molecules are hydrolyzed per tRNA charged, but for valine, 270. These stoichiometry ratios are fundamental to kinetic proofreading, for the energy coupling is essential and proofreading is obtained only by departing from 1:1 stoichiometry between energy coupling and product formation. Within the known reaction pathway, these ratios demonstrate that kinetic proofreading induces a reduction in errors by a factor of 1/180. An overall error rate of about 10(-4) for tRNA charging is obtained by a kinetic proofreading using a fundamental discrimination level of about 10(-2), and is compatible with the low in vivo error rate of protein synthesis.

摘要

动力学校正(Kinetic proofreading)是一种反应机制,其结构比米氏动力学更为复杂,它能对酶识别正确底物时出现的错误进行校正。我们使用异亮氨酰 - tRNA合成酶[L - 异亮氨酸:tRNAIle连接酶(生成AMP),EC 6.1.1.5]以及氨基酸异亮氨酸(正确)和缬氨酸(错误),测量了ATP水解与tRNAIle氨酰化之间的化学计量关系。通过在反应混合物中使用转移因子Tu - GTP(它能与氨酰化tRNA紧密结合),消除了氨酰化tRNA的酶促去酰化反应,而这种反应通常会妨碍有意义的化学计量研究。对于异亮氨酸,每氨酰化一个tRNA会水解1.5个ATP分子,但对于缬氨酸,则会水解270个。这些化学计量比对于动力学校正至关重要,因为能量偶联是必不可少的,而且只有偏离能量偶联与产物形成之间1:1的化学计量关系才能实现校正。在已知的反应途径中,这些比例表明动力学校正能将错误减少1/180倍。通过使用约为10^(-2)的基本辨别水平进行动力学校正,可得到tRNA氨酰化约10^(-4)的总体错误率,这与蛋白质合成在体内的低错误率是相符的。

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