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酵母苯丙氨酸转运核糖核酸中尿苷33的替换对其与核糖体反应的影响。

Effect of replacing uridine 33 in yeast tRNAPhe on the reaction with ribosomes.

作者信息

Dix D B, Wittenberg W L, Uhlenbeck O C, Thompson R C

出版信息

J Biol Chem. 1986 Aug 5;261(22):10112-8.

PMID:2426258
Abstract

We have determined several kinetic parameters for the reaction of poly(U)-programmed ribosomes with ternary complexes of elongation factor Tu, GTP, and yeast Phe-tRNA analogs with different bases substituted for uridine in position 33. These analogs test whether disruption of the hydrogen bonds normally formed by uridine 33 and steric crowding in the anticodon loop are detrimental to tRNA function on the ribosome. Single-turnover kinetic studies of the reaction of these ternary complexes with ribosomes show that these Phe-tRNA analogs decrease the apparent rate of GTP hydrolysis (kGTP) and the ratio of peptide formed to GTP hydrolyzed. Thus, the substitution of uridine 33 affects not only the selection of a ternary complex by the ribosome but also the selection of an aminoacyl-tRNA in the proofreading reaction. The effects become greater as first one, and then the other, H-bond is disrupted. Steric crowding in the anticodon loop is also important, but does not have as great an effect on the rate constants. An analysis of the elementary rate constants which comprise the rate constant, kGTP, demonstrates that the reduction in kGTP results from a decreased rate of ternary complex association with the ribosome (k1) and that there is little or no effect on the rate of GTP cleavage (k2). An analysis of the rate constants involved in proofreading shows that all the modified (tRNAs have increased rates of aminoacyl-tRNA rejection (k4) but that the rate of peptide bond formation (k3) is unaffected.

摘要

我们已经确定了聚(U)编程核糖体与延伸因子Tu、GTP和酵母苯丙氨酰-tRNA类似物的三元复合物反应的几个动力学参数,这些类似物在33位用不同碱基取代了尿苷。这些类似物用于测试通常由尿苷33形成的氢键的破坏以及反密码子环中的空间拥挤是否对核糖体上的tRNA功能有害。对这些三元复合物与核糖体反应的单周转动力学研究表明,这些苯丙氨酰-tRNA类似物降低了GTP水解的表观速率(kGTP)以及形成的肽与水解的GTP的比率。因此,尿苷33的取代不仅影响核糖体对三元复合物的选择,还影响校对反应中氨酰-tRNA的选择。随着一个氢键,然后是另一个氢键被破坏,这种影响变得更大。反密码子环中的空间拥挤也很重要,但对速率常数的影响没有那么大。对构成速率常数kGTP的基本速率常数的分析表明,kGTP的降低是由于三元复合物与核糖体结合的速率(k1)降低,并且对GTP裂解的速率(k2)几乎没有影响。对校对过程中涉及的速率常数的分析表明,所有修饰的tRNA氨酰-tRNA排斥速率(k4)都增加,但肽键形成速率(k3)不受影响。

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