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苏氨酸醛缩酶复合物的X射线结构:底物识别的结构基础。

X-ray structures of threonine aldolase complexes: structural basis of substrate recognition.

作者信息

Kielkopf Clara L, Burley Stephen K

机构信息

Laboratories of Molecular Biophysics and Howard Hughes Medical Institute, The Rockefeller University, 1230 York Avenue, New York, NY 10021, USA.

出版信息

Biochemistry. 2002 Oct 1;41(39):11711-20. doi: 10.1021/bi020393+.

Abstract

L-Threonine acetaldehyde-lyase (threonine aldolase, TA) is a pyridoxal-5'-phosphate-dependent (PLP) enzyme that catalyzes conversion of L-threonine or L-allo-threonine to glycine and acetaldehyde in a secondary glycine biosynthetic pathway. X-ray structures of Thermatoga maritima TA have been determined as the apo-enzyme at 1.8 A resolution and bound to substrate L-allo-threonine and product glycine at 1.9 and 2.0 A resolution, respectively. Despite low pairwise sequence identities, TA is a member of aspartate aminotransferase (AATase) fold family of PLP enzymes. The enzyme forms a 222 homotetramer with the PLP cofactor bound via a Schiff-base linkage to Lys199 within a domain interface. The structure reveals bound calcium and chloride ions that appear to contribute to catalysis and oligomerization, respectively. Although L-threonine and L-allo-threonine are substrates for T. maritima TA, enzymatic assays revealed a strong preference for L-allo-threonine. Structures of the external aldimines with substrate/product reveal a pair of histidines that may provide flexibility in substrate recognition. Variation in the threonine binding pocket may explain preferences for L-allo-threonine versus L-threonine among TA family members.

摘要

L-苏氨酸乙醛裂解酶(苏氨酸醛缩酶,TA)是一种依赖磷酸吡哆醛(PLP)的酶,在次要的甘氨酸生物合成途径中催化L-苏氨酸或L-别苏氨酸转化为甘氨酸和乙醛。嗜热栖热菌TA的X射线结构已分别以1.8 Å分辨率确定为无辅基酶结构,以及以1.9 Å和2.0 Å分辨率确定为与底物L-别苏氨酸和产物甘氨酸结合的结构。尽管序列同源性较低,但TA是PLP酶的天冬氨酸氨基转移酶(AATase)折叠家族的成员。该酶形成一个222同型四聚体,PLP辅因子通过席夫碱连接与结构域界面内的Lys199结合。结构显示结合的钙离子和氯离子似乎分别有助于催化作用和寡聚化。虽然L-苏氨酸和L-别苏氨酸都是嗜热栖热菌TA的底物,但酶活性测定显示其对L-别苏氨酸有强烈偏好。底物/产物的外部醛亚胺结构显示出一对组氨酸,它们可能在底物识别中提供灵活性。苏氨酸结合口袋的差异可能解释了TA家族成员中对L-别苏氨酸与L-苏氨酸的偏好。

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