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磷酸烯醇式丙酮酸羧化酶的三维结构:变构抑制的一种推测机制。

Three-dimensional structure of phosphoenolpyruvate carboxylase: a proposed mechanism for allosteric inhibition.

作者信息

Kai Y, Matsumura H, Inoue T, Terada K, Nagara Y, Yoshinaga T, Kihara A, Tsumura K, Izui K

机构信息

Department of Materials Chemistry, Graduate School of Engineering, Osaka University, Suita, 565-0871, Japan.

出版信息

Proc Natl Acad Sci U S A. 1999 Feb 2;96(3):823-8. doi: 10.1073/pnas.96.3.823.

DOI:10.1073/pnas.96.3.823
PMID:9927652
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC15309/
Abstract

The crystal structure of phosphoenolpyruvate carboxylase (PEPC; EC 4. 1.1.31) has been determined by x-ray diffraction methods at 2.8-A resolution by using Escherichia coli PEPC complexed with L-aspartate, an allosteric inhibitor of all known PEPCs. The four subunits are arranged in a "dimer-of-dimers" form with respect to subunit contact, resulting in an overall square arrangement. The contents of alpha-helices and beta-strands are 65% and 5%, respectively. All of the eight beta-strands, which are widely dispersed in the primary structure, participate in the formation of a single beta-barrel. Replacement of a conserved Arg residue (Arg-438) in this linkage with Cys increased the tendency of the enzyme to dissociate into dimers. The location of the catalytic site is likely to be near the C-terminal side of the beta-barrel. The binding site for L-aspartate is located about 20 A away from the catalytic site, and four residues (Lys-773, Arg-832, Arg-587, and Asn-881) are involved in effector binding. The participation of Arg-587 is unexpected, because it is known to be catalytically essential. Because this residue is in a highly conserved glycine-rich loop, which is characteristic of PEPC, L-aspartate seemingly causes inhibition by removing this glycine-rich loop from the catalytic site. There is another mobile loop from Lys-702 to Gly-708 that is missing in the crystal structure. The importance of this loop in catalytic activity was also shown. Thus, the crystal-structure determination of PEPC revealed two mobile loops bearing the enzymatic functions and accompanying allosteric inhibition by L-aspartate.

摘要

通过X射线衍射方法,以2.8埃的分辨率测定了磷酸烯醇丙酮酸羧化酶(PEPC;EC 4.1.1.31)的晶体结构,该研究使用了与L-天冬氨酸复合的大肠杆菌PEPC,L-天冬氨酸是所有已知PEPC的变构抑制剂。就亚基接触而言,四个亚基以“二聚体的二聚体”形式排列,形成整体的方形排列。α-螺旋和β-链的含量分别为65%和5%。所有八条β-链在一级结构中广泛分散,参与形成单个β-桶。用半胱氨酸取代该连接中保守的精氨酸残基(Arg-438)增加了酶解离成二聚体的倾向。催化位点可能位于β-桶的C端附近。L-天冬氨酸的结合位点位于距催化位点约20埃处,四个残基(Lys-773、Arg-832、Arg-587和Asn-881)参与效应物结合。Arg-587的参与出乎意料,因为已知它在催化中至关重要。由于该残基位于富含甘氨酸的高度保守环中,这是PEPC的特征,L-天冬氨酸似乎通过从催化位点去除这个富含甘氨酸的环而导致抑制。晶体结构中缺少另一个从Lys-702到Gly-708的可移动环。该环在催化活性中的重要性也得到了证明。因此,PEPC的晶体结构测定揭示了两个具有酶功能并伴随L-天冬氨酸变构抑制的可移动环。