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β,β,β-三氟丙氨酸使丙氨酸消旋酶失活的机制。

Mechanism of inactivation of alanine racemase by beta, beta, beta-trifluoroalanine.

作者信息

Faraci W S, Walsh C T

机构信息

Department of Biological Chemistry and Molecular Pharmacology, Harvard Medical School, Boston, Massachusetts 02115.

出版信息

Biochemistry. 1989 Jan 24;28(2):431-7. doi: 10.1021/bi00428a004.

DOI:10.1021/bi00428a004
PMID:2496744
Abstract

The alanine racemases are a group of PLP-dependent bacterial enzymes that catalyze the racemization of alanine, providing D-alanine for cell wall synthesis. Inactivation of the alanine racemases from the Gram-negative organism Salmonella typhimurium and Gram-positive organism Bacillus stearothermophilus with beta, beta, beta-trifluoroalanine has been studied. The inactivation occurs with the same rate constant as that for formation of a broad 460-490-nm chromophore. Loss of two fluoride ions per mole of inactivated enzyme and retention of [1-14C]trifluoroalanine label accompany inhibition, suggesting a monofluoro enzyme adduct. Partial denaturation (1 M guanidine) leads to rapid return of the initial 420-nm chromophore, followed by a slower (t1/2 approximately 30 min-1 h) loss of the fluoride ion and 14CO2 release. At this point, reduction by NaB3H4 and tryptic digestion yield a single radiolabeled peptide. Purification and sequencing of the peptide reveals that lysine-38 is covalently attached to the PLP cofactor. A mechanism for enzyme inactivation by trifluoroalanine is proposed and contrasted with earlier results on monohaloalanines, in which nucleophilic attack of released aminoacrylate on the PLP aldimine leads to enzyme inactivation. For trifluoroalanine inactivation, nucleophilic attack of lysine-38 on the electrophilic beta-difluoro-alpha, beta-unsaturated imine provides an alternative mode of inhibition for these enzymes.

摘要

丙氨酸消旋酶是一类依赖磷酸吡哆醛(PLP)的细菌酶,可催化丙氨酸的消旋作用,为细胞壁合成提供D-丙氨酸。已对用β,β,β-三氟丙氨酸使革兰氏阴性菌鼠伤寒沙门氏菌和革兰氏阳性菌嗜热脂肪芽孢杆菌的丙氨酸消旋酶失活进行了研究。失活的速率常数与形成宽460 - 490纳米发色团的速率常数相同。每摩尔失活酶损失两个氟离子,并伴随[1-14C]三氟丙氨酸标记的保留,表明形成了单氟酶加合物。部分变性(1 M胍)导致最初420纳米发色团迅速恢复,随后氟离子缓慢损失(半衰期约30分钟 - 1小时)并释放14CO2。此时,用NaB3H4还原并经胰蛋白酶消化产生一个单一的放射性标记肽段。该肽段的纯化和测序表明赖氨酸-38与PLP辅因子共价连接。提出了三氟丙氨酸使酶失活的机制,并与早期关于单卤代丙氨酸的结果进行了对比,在单卤代丙氨酸的情况中,释放的氨基丙烯酸对PLP醛亚胺的亲核攻击导致酶失活。对于三氟丙氨酸失活,赖氨酸-38对亲电β-二氟-α,β-不饱和亚胺的亲核攻击为这些酶提供了另一种抑制模式。

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