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在乳酸或苯乳酸存在下结晶的Y143F黄素细胞色素b2突变体的两种复合物的X射线结构。

X-ray structure of two complexes of the Y143F flavocytochrome b2 mutant crystallized in the presence of lactate or phenyl lactate.

作者信息

Tegoni M, Begotti S, Cambillau C

机构信息

Laboratoire de Cristallographie et Cristallisation des Macromolécules Biologiques, URA-1296 CNRS, Marseille, France.

出版信息

Biochemistry. 1995 Aug 8;34(31):9840-50.

PMID:7632684
Abstract

Flavocytochrome b2 is a flavohemo enzyme localized in the intermembrane space of yeast mitochondria, where it catalyzes the electron transfer from its substrate, L-lactate, to cytochrome c. We have obtained crystals of a flavocytochrome b2 mutant, Y143F, which are isostructural with those of the native recombinant enzyme [Tegoni, M., & Cambillau, C. (1994) Protein Sci.3, 303-314]. These crystals were grown under similar conditions to those used to obtain the recombinant enzyme, but in the presence of phenyl lactate or lactate. We report here on the structural analysis of the two complexes of flavocytochrome b2 with the reaction products at 2.9 A resolution. In both structures, the Phe143 phenyl ring keeps the same position as that of the phenolic ring of Tyr143 in both the native recombinant and in the native wild-type enzymes. The product of the reaction, phenyl pyruvate or pyruvate, is present at the active site of both subunits, and not only in subunit 2 as observed in the wild-type structure [Xia, Z.-X., & Mathews, F.S. (1990) J. Mol. Biol. 212, 837-863]. The number of interactions between the FMN and the heme domain is considerably lower in the Y143F mutant than in the native proteins. The latter finding strongly supports the hypothesis that the main role of Tyr143 in the native proteins. The latter findings strongly supports the hypothesis that the main role of Tyr143 in the native protein probably consists in establishing a hydrogen bond with the heme [Xia, Z.-X., & Mathews, F.S. (1990) J. Mol. Biol. 212, 837-863]. This interaction appears to be essential for the two domains to approach each other suitably so that the intramolecular electron transfer can occur.

摘要

黄素细胞色素b2是一种黄素血红蛋白酶,定位于酵母线粒体的膜间隙,在那里它催化电子从其底物L-乳酸转移到细胞色素c。我们获得了黄素细胞色素b2突变体Y143F的晶体,其与天然重组酶的晶体同构[Tegoni, M., & Cambillau, C. (1994) Protein Sci.3, 303 - 314]。这些晶体在与用于获得重组酶相似的条件下生长,但存在苯乳酸或乳酸。我们在此报告黄素细胞色素b2与反应产物的两种复合物在2.9埃分辨率下的结构分析。在两种结构中,Phe143苯环在天然重组酶和天然野生型酶中都保持与Tyr143酚环相同的位置。反应产物苯丙酮酸或丙酮酸存在于两个亚基的活性位点,而不像在野生型结构中那样仅存在于亚基2中[Xia, Z.-X., & Mathews, F.S. (1990) J. Mol. Biol. 212, 837 - 863]。在Y143F突变体中,FMN与血红素结构域之间的相互作用数量比天然蛋白质中显著减少。后一发现有力地支持了这样的假设,即Tyr143在天然蛋白质中的主要作用。后一发现有力地支持了这样的假设,即Tyr143在天然蛋白质中的主要作用可能在于与血红素形成氢键[Xia, Z.-X., & Mathews, F.S. (1990) J. Mol. Biol. 212, 837 - 863]。这种相互作用似乎对于两个结构域适当地相互靠近从而发生分子内电子转移至关重要。

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