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A fluorescence stopped-flow kinetic study of the conformational activation of α-chymotrypsin and several mutants

机译:α-胰凝乳蛋白酶和几个突变体构象激活的荧光停止流动力学研究

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摘要

The kinetic activation parameters (activation free energy, activation free enthalpy, and activation free entropy change) of the conformational change of α-chymotrypsin from an inactive to the active conformation were determined after a pH jump from pH 11.0 to pH 6.8 by the fluorescence stopped-flow method. The conformational change was followed by measuring changes in the protein fluorescence. For the bovine wild-type protein, the same kinetic parameters are obtained as in the study of proflavin binding. Several mutants were made with the goal to accelerate or decelerate this conformational transition. The inspiration for the choice of the mutants came from a previous modelling study done on the bovine wild-type chymotrypsin. The results of the fluorescence stopped flow experiments show that several mutants behaved as was expected based on the information provided by the modeling study on the wild-type variant. For some mutants our assumptions were not correct, and therefore additional modeling studies of the activation pathways of these mutant proteins are necessary to be able to explain the observed kinetic behavior.
机译:在pH值从11.0跃升至6.8时,通过荧光停止,测定了α-胰凝乳蛋白酶从非活性构象到活性构象的构象变化的动力学活化参数(活化自由能,活化自由焓和活化自由熵变化)。流方法。构象变化之后,测量蛋白质荧光的变化。对于牛野生型蛋白,获得与黄素结合研究相同的动力学参数。为了加速或减速这种构象转变,制备了几种突变体。选择突变体的灵感来自先前对牛野生型胰凝乳蛋白酶进行的建模研究。荧光终止流动实验的结果表明,基于对野生型变体的建模研究提供的信息,一些突变体表现出预期的行为。对于某些突变体,我们的假设是不正确的,因此有必要对这些突变蛋白的激活途径进行其他建模研究,才能解释观察到的动力学行为。

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