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β-氰基丙氨酸合酶:纯化与特性鉴定

Beta-cyanoalanine synthase: purification and characterization.

作者信息

Akopyan T N, Braunstein A E, Goryachenkova E V

出版信息

Proc Natl Acad Sci U S A. 1975 Apr;72(4):1617-21. doi: 10.1073/pnas.72.4.1617.

Abstract

Beta-cyano-L-alanine synthase [L-cysteine hydrogen-sulfide-lyase (adding HCN), EC 4.4.1.9] was purified about 4000-fold from blue lupine seedlings. The enzyme was homoegeneous on gel electrophoresis and free of contamination by other pyridoxal-P-dependent lyases. The enzyme has a molecular weight of 52,000 and contains 1 mole of pyridoxal-P per mole of protein; its isoelectric point is situated at pH 4.7. Its absorption spectrum has two maxima, at 280 and 410 nm. L-Cysteine is the natural primary (amino acid) substrate; beta-chloro- and beta-thiocyano can serve (with considerably lower affinity) instead of cyanide as cosubstrates for cyanoalanine synthase. The synthase is refractory to DL-cycloserine and D-penicillamine, potent inhibitors of many pyridoxal-P-dependent enzymes. Cyanoalanine synthase catalyzes slow isotopic alpha-H exchange in cysteine and in end-product amino acids; the rates of alpha-H exchange in nonreacted (excess) cysteine are markedly increased in the presence of an adequate cosubstrate; no exchange is observed of H atoms in beta-position.

摘要

β-氰基-L-丙氨酸合酶[L-半胱氨酸硫化氢裂解酶(加HCN),EC 4.4.1.9]从蓝羽扇豆幼苗中纯化了约4000倍。该酶在凝胶电泳上呈均一性,且不受其他依赖磷酸吡哆醛的裂解酶的污染。该酶的分子量为52,000,每摩尔蛋白质含有1摩尔磷酸吡哆醛;其等电点位于pH 4.7。其吸收光谱在280和410nm处有两个最大值。L-半胱氨酸是天然的主要(氨基酸)底物;β-氯和β-硫氰基可以(亲和力低得多)替代氰化物作为氰基丙氨酸合酶的共底物。该合酶对DL-环丝氨酸和D-青霉胺不敏感,而DL-环丝氨酸和D-青霉胺是许多依赖磷酸吡哆醛的酶的有效抑制剂。氰基丙氨酸合酶催化半胱氨酸和终产物氨基酸中缓慢的同位素α-H交换;在存在足够共底物的情况下未反应(过量)半胱氨酸中α-H交换的速率显著增加;在β位未观察到H原子的交换。

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