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Crystal structure and biochemical characterization of PhaA from Ralstonia eutropha, a polyhydroxyalkanoate-producing bacterium

机译:来自Ralstonia Eutropha的Phaa晶体结构和生化特征,一种多羟基烷酸盐产生细菌

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PhaA from Ralstonia eutropha (RePhaA) is the first enzyme in the polyhydroxyalbutyrate (PHB) biosynthetic pathway and catalyzes the condensation of two molecules of acetyl-CoA to acetoacetyl-CoA. To investigate the molecular mechanism underlying PHB biosynthesis, we determined the crystal structures of the RePhaA protein in apo- and CoA-bound forms. The RePhaA structure adopts the type II biosynthetic thiolase fold forming a tetramer by means of dimerization of two dimers. The crystal structure of RePhaA in complex with CoA revealed that the enzyme contained a unique Phe219 residue, resulting that the ADP moiety binds in somewhat different position compared with that bound in other thiolase enzymes. Our study provides structural insight into the substrate specificity of RePhaA. Results indicate the presence of a small pocket near the Cys88 covalent catalytic residue leading to the possibility of the enzyme to accommodate acetyl-CoA as a sole substrate instead of larger acyl-CoA molecules such as propionyl-CoA. Furthermore, the roles of key residues involved in substrate binding and enzyme catalysis were confirmed by site-directed mutagenesis. (C) 2014 Elsevier Inc. All rights reserved.
机译:来自Ralstonia Eutropha(REPHA)的PHAA是多羟基丁酸酯(PHB)生物合成途径中的第一种酶,并催化两种乙酰乙酰-COA分子的凝结。为了研究pHB生物合成的分子机制,我们确定了α-和COA结合的形式中REPHA蛋白的晶体结构。 Rephaa结构采用II型生物合成硫酶折叠通过二聚体的二聚化形成四聚体。与COA复合物中Rephaa的晶体结构揭示了酶含有独特的PHE219残基,导致ADP部分与其他硫醇酶酶的结合相比在稍微不同的位置结合。我们的研究提供了对Rephaa的底物特异性的结构洞察力。结果表明Cys88共价催化残余物附近的小口袋的存在,导致酶的可能性将乙酰-CoA作为唯一的底物,而不是较大的酰基-CoA分子如丙酰基-CoA。此外,通过定点诱变证实了参与底物结合和酶催化催化的关键残留物的作用。 (c)2014年elsevier Inc.保留所有权利。

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