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蛋白质折叠与脯氨酰异构化之间的动力学偶联。II. 核糖核酸酶A和核糖核酸酶T1的折叠

Kinetic coupling between protein folding and prolyl isomerization. II. Folding of ribonuclease A and ribonuclease T1.

作者信息

Kiefhaber T, Schmid F X

机构信息

Universität Bayreuth, Laboratorium für Biochemie, Germany.

出版信息

J Mol Biol. 1992 Mar 5;224(1):231-40. doi: 10.1016/0022-2836(92)90586-9.

Abstract

The folding and unfolding kinetics within the transition region were measured for RNase A and for RNase T1. The data were used to evaluate the theoretical models for the influence of prolyl isomerization on the observed folding kinetics. These two proteins were selected, since the folding reaction of RNase A is faster than prolyl isomerization, whereas in RNase T1, folding is slower than isomerization in the transition region. Folding of RNase T1 was investigated for three variants with different numbers of cis prolyl residues. The results indicate that in the transition region the folding rates are indeed strongly dependent on the number of prolyl residues. The variant of RNase T1 that contains only one cis prolyl residue folds about ten times faster than two variants that contain two cis prolyl residues. For both RNase A and RNase T1, the apparent rates of folding and unfolding as well as the corresponding amplitudes depend on the concentration of denaturant in a manner that was predicted by the model calculations. When refolding was started from the fast-folding species, additional kinetic phases could be observed in the transition region for both proteins. The obtained values could be used to calculate the microscopic rate constants of folding and isomerization on the basis of theoretical models.

摘要

测定了核糖核酸酶A和核糖核酸酶T1在过渡区域内的折叠与去折叠动力学。这些数据用于评估脯氨酰异构化对观察到的折叠动力学影响的理论模型。选择这两种蛋白质是因为核糖核酸酶A的折叠反应比脯氨酰异构化快,而在核糖核酸酶T1中,在过渡区域折叠比异构化慢。研究了具有不同顺式脯氨酰残基数量的三种核糖核酸酶T1变体的折叠情况。结果表明,在过渡区域,折叠速率确实强烈依赖于脯氨酰残基的数量。仅含有一个顺式脯氨酰残基的核糖核酸酶T1变体的折叠速度比含有两个顺式脯氨酰残基的两个变体快约十倍。对于核糖核酸酶A和核糖核酸酶T1,折叠和去折叠的表观速率以及相应的幅度都以模型计算预测的方式依赖于变性剂的浓度。当从快速折叠物种开始重折叠时,在两种蛋白质的过渡区域都可以观察到额外的动力学阶段。获得的值可用于根据理论模型计算折叠和异构化的微观速率常数。

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