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对来自布氏乳杆菌的PLP依赖性折叠I型异亮氨酸2-表异构酶的底物识别和反应特异性的结构见解。

Structural insights into the substrate recognition and reaction specificity of the PLP-dependent fold-type I isoleucine 2-epimerase from Lactobacillus buchneri.

作者信息

Awad Rida, Gans Pierre, Reiser Jean-Baptiste

机构信息

Institut de Biologie Structurale (IBS), Univ. Grenoble Alpes, CEA, CNRS, 38044, Grenoble, France.

Institut de Biologie Structurale (IBS), Univ. Grenoble Alpes, CEA, CNRS, 38044, Grenoble, France.

出版信息

Biochimie. 2017 Jun;137:165-173. doi: 10.1016/j.biochi.2017.03.015. Epub 2017 Mar 23.

DOI:10.1016/j.biochi.2017.03.015
PMID:28344038
Abstract

The isoleucine 2-epimerase from Lactobacillus buchneri has been previously identified and characterized to catalyze the pyridoxal 5'-phosphate (PLP)-dependent racemization and epimerization of a broad spectrum of nonpolar amino acids from L- to D-form and vice versa, in particular isoleucine. In this study, crystal structures of both native and PLP-complex forms of this racemase are presented at 2.6 and 2.15 Å resolution, respectively. Both structures show that the protein belongs to the fold-type I subgroup of PLP-dependent enzymes and is very close to aminobutyrate aminotransferases family, as it has been suspected because of their sequence homology. The extensive structural comparison with fold-type I enzymes with known amino acid racemization activities, including the α-amino-ε-caprolactam racemase from Achromobacter obae and the cystathionine β-lyase from Escherichia coli, allows us to identify the active site residues responsible for its nonpolar amino acid recognition and reactivity specificity. Our observations also suggest that the racemization reaction by the fold-type I racemases may generally occur thanks to a revised two-base mechanism. Lastly, both structures reveal details on the conformational changes provoked by PLP binding that suggest an induced fit of the active site "entrance door", necessary to accommodate PLP and substrate molecules.

摘要

先前已鉴定并表征了来自布氏乳杆菌的异亮氨酸2-表异构酶,它可催化5'-磷酸吡哆醛(PLP)依赖性的多种非极性氨基酸从L型到D型以及反之亦然的消旋化和差向异构化反应,尤其是异亮氨酸。在本研究中,分别以2.6 Å和2.15 Å的分辨率展示了该消旋酶的天然形式和PLP复合物形式的晶体结构。两种结构均表明,该蛋白质属于PLP依赖性酶的折叠I型亚组,并且由于其序列同源性,它与氨基丁酸转氨酶家族非常接近,这一点正如之前所推测的那样。与具有已知氨基酸消旋化活性的折叠I型酶进行广泛的结构比较,包括来自浅黄无色杆菌的α-氨基-ε-己内酰胺消旋酶和来自大肠杆菌的胱硫醚β-裂解酶,使我们能够确定负责其对非极性氨基酸识别和反应特异性的活性位点残基。我们的观察结果还表明,折叠I型消旋酶的消旋化反应可能通常得益于一种经过修正的双碱基机制。最后,两种结构都揭示了由PLP结合引起的构象变化的细节,这表明活性位点“入口门”的诱导契合对于容纳PLP和底物分子是必要的。

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