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Phylogenetic and amino acid conservation analyses of bacterial l-aspartate-α-decarboxylase and of its zymogen-maturation protein reveal a putative interaction domain

机译:细菌l-天门冬氨酸-α-脱羧酶及其酶原成熟蛋白的系统发育和氨基酸保守性分析揭示了推测的相互作用域

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摘要

BackgroundAll organisms must synthesize the enzymatic cofactor coenzyme A (CoA) from the precursor pantothenate. Most bacteria can synthesize pantothenate de novo by the condensation of pantoate and β-alanine. The synthesis of β-alanine is catalyzed by l-aspartate-α-decarboxylase (PanD), a pyruvoyl enzyme that is initially synthesized as a zymogen (pro-PanD). Active PanD is generated by self-cleavage of pro-PanD at Gly24-Ser25 creating the active-site pyruvoyl moiety. In Salmonella enterica, this cleavage requires PanM, an acetyl-CoA sensor related to the Gcn5-like N-acetyltransferases. PanM does not acetylate pro-PanD, but the recent publication of the three-dimensional crystal structure of the PanM homologue PanZ in complex with the PanD zymogen of Escherichia coli provides validation to our predictions and provides a framework in which to further examine the cleavage mechanism. In contrast, PanD from bacteria lacking PanM efficiently cleaved in the absence of PanM in vivo.
机译:背景所有生物都必须从前体泛酸酯合成酶促辅因子辅酶A(CoA)。大多数细菌可以通过泛酸和β-丙氨酸的缩合反应从头合成泛酸。 β-丙氨酸的合成由l-天门冬氨酸-α-脱羧酶(PanD)催化,该酶是一种丙酮酰酶,最初被合成为酶原(pro-PanD)。通过在Gly24-Ser25上Pro-PanD的自我切割产生活性PanD,从而形成活性位点丙酮酰基部分。在肠沙门氏菌中,这种切割需要PanM(一种与Gcn5样N-乙酰基转移酶有关的乙酰辅酶A传感器)。 PanM不会乙酰化前PanD,但是最近发表的PanM同源PanZ三维晶体结构与大肠杆菌PanD酶原复合的结果为我们的预测提供了依据,并为进一步研究裂解机理提供了框架。相反,缺乏PanM的细菌的PanD在体内不存在PanM的情况下被有效地裂解。

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