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关于细胞质和线粒体丝氨酸转羟甲基酶的机制、抑制作用及立体化学研究。

Mechanistic, inhibitory and stereochemical studies on cytoplasmic and mitochondrial serine transhydorxymethylases.

作者信息

Akhtar M, El-Obeid H A, Jordan P M

出版信息

Biochem J. 1975 Feb;145(2):159-68. doi: 10.1042/bj1450159.

Abstract

By using cytoplasmic and mitochondrial serine transhydroxymethylase isoenzymes from rabbit liver, it was shown that both enzymes exhibited similar ratios of serine transhydroxymethylase/threonine aldolase activities. Both enzymes catalysed the removal of the pro-S hydrogen atom of glycine, which was greatly enhanced by the presence of tetrahydrofolate. The cytoplasmic as well as the mitochondrial enzyme catalysed the synthesis of serine from glycine and [3H2]formaldehyde in the absence of tetrahydrofolate. The results are consistent with our previous suggestion that a role of tetrahydrofolate in the serine transhydroxymethylase reaction is to transport formaldehyde in and out of the active site (Jordan & Akhtar, 1970). The isoenzymes, however, showed remarkable differences in their inactivation by inhibitors. The serine transhydroxymethylase as well as the threonine aldolase activities of the cytoplasmic enzyme were inactivated in a similar fashion by chloroacetaldehyde, iodoacetamide, bromopyruvate and glycidaldehyde (2,3-epoxypropionaldehyde). These inhibitors had no effect on the two activities of the mitochondrial enzyme. The rate of inactivation of the cytoplasmic enzyme by glycidaldehyde was enhanced by the presence of glycine but decreased by the presence of serine. The implications of these results to the mechanism of catalysis and the nature of the active site of the enzymes are discussed.

摘要

通过使用兔肝中的细胞质和线粒体丝氨酸转羟甲基酶同工酶,结果表明这两种酶表现出相似的丝氨酸转羟甲基酶/苏氨酸醛缩酶活性比率。两种酶都催化甘氨酸的前-S氢原子的去除,四氢叶酸的存在会大大增强这种催化作用。在没有四氢叶酸的情况下,细胞质酶和线粒体酶都催化由甘氨酸和[3H2]甲醛合成丝氨酸。这些结果与我们之前提出的四氢叶酸在丝氨酸转羟甲基酶反应中的作用是将甲醛转运进出活性位点的观点一致(乔丹和阿赫塔尔,1970年)。然而,这两种同工酶在被抑制剂失活方面表现出显著差异。细胞质酶的丝氨酸转羟甲基酶以及苏氨酸醛缩酶活性以类似的方式被氯乙醛、碘乙酰胺、溴丙酮酸和缩水甘油醛(2,3-环氧丙醛)失活。这些抑制剂对线粒体酶的两种活性没有影响。缩水甘油醛对细胞质酶的失活速率在有甘氨酸存在时会增强,但在有丝氨酸存在时会降低。本文讨论了这些结果对催化机制和酶活性位点性质的影响。

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