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克氏锥虫磷酸丙糖异构酶在盐酸胍中的可逆平衡去折叠涉及稳定的二聚体和单体中间体。

Reversible equilibrium unfolding of triosephosphate isomerase from Trypanosoma cruzi in guanidinium hydrochloride involves stable dimeric and monomeric intermediates.

作者信息

Chánez-Cárdenas María Elena, Pérez-Hernández Gerardo, Sánchez-Rebollar Brenda Guadalupe, Costas Miguel, Vázquez-Contreras Edgar

机构信息

Laboratorio de Patología Vascular Cerebral, Instituto Nacional de Neurología y Neurocirugía Manuel Velasco Suárez, México, DF, Mexico.

出版信息

Biochemistry. 2005 Aug 16;44(32):10883-92. doi: 10.1021/bi047687a.

DOI:10.1021/bi047687a
PMID:16086591
Abstract

The reversible guanidinium hydrochloride-induced unfolding of Trypanosoma cruzi triosephosphate isomerase (TcTIM) was characterized under equilibrium conditions. The catalytic activity was followed as a native homodimeric functional probe. Circular dichroism, intrinsic fluorescence, and size-exclusion chromatography were used as secondary, tertiary, and quaternary structural probes, respectively. The change in ANS fluorescence intensity with increasing denaturant concentrations was also determined. The results show that two stable intermediates exist in the transition from the homodimeric native enzyme to the unfolded monomers: one (N(2*)) is a slightly more expanded, non-native, and active dimer, and the other is a partially expanded monomer (M) that binds ANS. Spectroscopic and activity data were used to reach a thermodynamic characterization. The results indicate that the Gibbs free energies for the partial reactions are 4.5 (N(2) <==> N(2*)), 65.8 (N(2*) <==> 2M), and 17.8 kJ/mol (M <==> U). It appears that TcTIM monomers are more stable than those found for other TIM species (except yeast TIM), where monomer stability is only marginal. These results are compared with those for the guanidinium hydrochloride-induced denaturation of TIM from different species, where despite the functional and three-dimensional similarities, a remarkable heterogeneity exists in the unfolding pathways.

摘要

在平衡条件下,对盐酸胍诱导的克氏锥虫磷酸丙糖异构酶(TcTIM)可逆去折叠进行了表征。以天然同源二聚体功能探针追踪催化活性。分别使用圆二色性、内源荧光和尺寸排阻色谱作为二级、三级和四级结构探针。还测定了随着变性剂浓度增加ANS荧光强度的变化。结果表明,从同源二聚体天然酶到去折叠单体的转变过程中存在两个稳定中间体:一个(N(2*))是略微更伸展、非天然且有活性的二聚体,另一个是结合ANS的部分伸展单体(M)。利用光谱和活性数据进行了热力学表征。结果表明,部分反应的吉布斯自由能分别为4.5(N(2)⇌N(2*))、65.8(N(2*)⇌2M)和17.8 kJ/mol(M⇌U)。似乎TcTIM单体比其他TIM物种(酵母TIM除外)的单体更稳定,在其他物种中单体稳定性只是勉强维持。将这些结果与不同物种的TIM在盐酸胍诱导变性方面的结果进行了比较,尽管它们在功能和三维结构上有相似性,但在去折叠途径中存在显著的异质性。

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