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通过伪一级动力学分析测定真核肽基转移酶活性。

Determination of eukaryotic peptidyltransferase activity by pseudo-first-order kinetic analysis.

作者信息

Ioannou M, Coutsogeorgopoulos C, Drainas D

机构信息

Department of Biochemistry, School of Medicine, University of Patras, Greece.

出版信息

Anal Biochem. 1997 Apr 5;247(1):115-22. doi: 10.1006/abio.1997.2034.

Abstract

We have developed an in vitro system for the determination of peptidyltransferase activity in rabbit reticulocyte ribosomes. Using this system, a detailed kinetic analysis of a model reaction for peptidyltransferase is described, with AcPhe-tRNA as the peptidyl donor and puromycin as the acceptor. The [AcPhe-tRNA-poly(U)-80S ribosome] complex (complex C) is isolated and then reacted with excess puromycin to give AcPhe-puromycin. This reaction (puromycin reaction) follows first-order kinetics at all concentrations of puromycin tested. At saturating concentrations of puromycin, the first-order rate (k3) constant is identical to the catalytic rate constant (kcat) of peptidyltransferase. This k3 of peptidyltransferase is equal to 2.9 min-1 at 37 degrees C. Moreover, the ratio k3/ Ks, which is an accurate measure of peptidyltransferase activity, was increased 80-fold when salt-washed ribosomes were replaced by unwashed ribosomes. Finally, the puromycin reaction was inhibited by several well-known antibiotics acting on the eukaryotic peptidyltransferase.

摘要

我们开发了一种用于测定兔网织红细胞核糖体中肽基转移酶活性的体外系统。利用该系统,描述了以乙酰苯丙氨酰 - tRNA为肽基供体、嘌呤霉素为受体的肽基转移酶模型反应的详细动力学分析。分离出[乙酰苯丙氨酰 - tRNA - 聚(U)- 80S核糖体]复合物(复合物C),然后使其与过量的嘌呤霉素反应生成乙酰苯丙氨酰 - 嘌呤霉素。该反应(嘌呤霉素反应)在所有测试的嘌呤霉素浓度下均遵循一级动力学。在嘌呤霉素饱和浓度下,一级速率(k3)常数与肽基转移酶的催化速率常数(kcat)相同。在37℃时,肽基转移酶的这个k3等于2.9 min-1。此外,当用未洗涤的核糖体替代盐洗涤的核糖体时,作为肽基转移酶活性准确衡量指标的k3 / Ks比值增加了80倍。最后,嘌呤霉素反应受到几种作用于真核肽基转移酶的知名抗生素的抑制。

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