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盐对谷胱甘肽促进还原型牛胰核糖核酸酶再活化的影响。

Salt effects in the glutathione-facilitated reactivation of reduced bovine pancreatic ribonuclease.

作者信息

Schaffer S W, Ahmed A K, Wetlaufer D B

出版信息

J Biol Chem. 1975 Nov 10;250(21):8483-6.

PMID:1104605
Abstract

The rate of regeneration of reduced RNase by glutathione was examined in the presence of several added substances: substrate, phospholipid, other proteins, bacterial ribosomes, and neutral salts. Of these, only neutral salts showed substantial effects. K2HOP4 and (NH4)2SO4 strongly accelerated regeneration, the alkali chlorides showed moderate acceleration or inhibition, while LiBr and KSCN strongly inhibited. The t1/2 for regeneration in 1 M Pi is 4 min compared to 75 min in the absence of Pi; in 0.5 M KSCN t1/2 greater than 100 min. The pattern of specific salt effects is similar to a Hofmeister series. There is a strong parallel between the pattern of specific salt effects on the kinetics of RNase regeneration and the pattern of effects of the same salts on the equilibrium stability of biopolymers. This suggests that the role of salts in the regeneration is to stabilize or destabilize rate-limiting folding intermediates. Pi-accelerated glutathione regenerations showed a broad temperature optimum from 30-37 degrees. In strong contrast with the virtual concentration independence of the Pi-free controls, with Pi = 1 M, both rates and yields of RNase activity were decreased markedly at [RNase] greater than 2 x 10(-6) M. Phosphate and pyrophosphate showed additive, and in some cases, synergistic accelerations. These results suggest that specific ion binding occurs in addition to general solvent effects.

摘要

在添加了几种物质的情况下,研究了谷胱甘肽对还原型核糖核酸酶(RNase)的再生速率:底物、磷脂、其他蛋白质、细菌核糖体和中性盐。其中,只有中性盐显示出显著影响。K2HOP4和(NH4)2SO4强烈加速再生,碱金属氯化物显示出适度的加速或抑制作用,而LiBr和KSCN则强烈抑制。在1 M Pi中再生的t1/2为4分钟,而在没有Pi的情况下为75分钟;在0.5 M KSCN中t1/2大于100分钟。特定盐效应的模式类似于霍夫迈斯特序列。特定盐对RNase再生动力学的效应模式与相同盐对生物聚合物平衡稳定性的效应模式之间存在很强的平行关系。这表明盐在再生中的作用是稳定或破坏限速折叠中间体。Pi加速的谷胱甘肽再生显示出30-37摄氏度的宽温度最佳范围。与无Pi对照的实际浓度独立性形成强烈对比的是,当Pi = 1 M时,在[RNase]大于2 x 10(-6) M时,RNase活性的速率和产率均显著降低。磷酸盐和焦磷酸盐显示出加和作用,在某些情况下还有协同加速作用。这些结果表明,除了一般的溶剂效应外,还发生了特定的离子结合。

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