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大鼠睾丸中葡萄糖6-磷酸-D-肌醇1-磷酸环化酶的机制。氢原子的参与。

The mechanism of glucose 6-phosphate-D-myo-inositol 1-phosphate cyclase of rat testis. The involvement of hydrogen atoms.

作者信息

Barnett J E, Corina D L

出版信息

Biochem J. 1968 Jun;108(1):125-9. doi: 10.1042/bj1080125.

Abstract

Comparison of the initial (3)H/(14)C ratios in specifically labelled d-glucose 6-phosphates with the final ratios in myo-inositol produced by glucose 6-phosphate-d-myo-inositol 1-phosphate cyclase from rat testis showed that, during the conversion, the hydrogen atoms at C-1 and C-3 were fully retained, one hydrogen atom was lost from C-6, and that at C-5 was apparently retained to the extent of 80-90%. The loss of (3)H could not be stimulated by addition of unlabelled NADH, and when unlabelled substrate was used (3)H from [(3)H]NADH and [(3)H]water was not incorporated. Treatment of the enzyme with charcoal abolished the activity, and this was restored to 25-50% of the original activity by NAD(+). The charcoal-treated enzyme again apparently gave 85% retention of hydrogen with [5-(3)H]glucose 6-phosphate as substrate in the presence of NAD(+) alone, but the retention was decreased to 65% with excess of NADH. The results are interpreted as indicating that the cyclization proceeds by an aldol condensation in which C-5 is oxidized by NAD(+) in a tightly-bound ternary complex, and that the apparent loss of (3)H when untreated enzyme is used is due to an isotope effect. It is suggested that after treatment with charcoal some exchange of NADH with an external pool may take place.

摘要

将大鼠睾丸中经特定标记的6-磷酸 -d-葡萄糖的初始(³H/¹⁴C)比率与由6-磷酸 -d-肌醇1-磷酸环化酶将其转化生成的肌醇的最终比率进行比较,结果表明,在转化过程中,C-1和C-3位的氢原子完全保留,C-6位失去一个氢原子,C-5位的氢原子显然保留了80 - 90%。添加未标记的NADH并不能刺激³H的损失,当使用未标记的底物时,[(³H)NADH]和[(³H)水]中的³H不会掺入。用活性炭处理该酶会使其活性丧失,而通过NAD⁺可将其活性恢复至原始活性的25 - 50%。在仅存在NAD⁺的情况下,用活性炭处理后的酶以[5-(³H)]6-磷酸葡萄糖作为底物时,氢的保留率显然再次达到85%,但在过量NADH存在时,保留率降至65%。这些结果被解释为表明环化反应通过醛醇缩合进行,其中在紧密结合的三元复合物中C-5被NAD⁺氧化,并且当使用未处理的酶时³H的明显损失是由于同位素效应。有人提出,用活性炭处理后,NADH可能会与外部池发生一些交换。

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Biochem Biophys Res Commun. 1964;14:419-24. doi: 10.1016/0006-291x(64)90079-8.
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