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果蝇α-甘油磷酸脱氢酶的定量亚基杂交

Quantitative subunit hybridization of drosophila alpha-glycerophosphate dehydrogenase.

作者信息

Collier G E, MacIntyre R J

出版信息

J Mol Evol. 1978 Dec 29;12(2):173-82. doi: 10.1007/BF01733265.

Abstract

The dimeric enzyme, alpha-Glycerophosphate dehydrogenase, was purified from eight Drosophila species by the method of Collier et al. (1976). The enzymes were inactivated at high pH and the conditions sufficient for reactivation were established. Electrophoretic patterns of reactivated alpha-glycerophosphate dehydrogenases which were mixed following inactivation of two species' enzymes, demonstrate that high pH dissociates the enzyme into its constituent subunits and reactivation involves subunit reassociation. Twenty interspecific combinations of dissociated enzymes were allowed to reassociate, and the amounts of both heterospecific and homospecific enzyme activity and protein were determined by densitometry. In all 20 tests there were no differences between observed and expected heterospecific:homospecific enzyme ratios. These results are consistent with the very slow rate of evolution of this enzyme in the family Drosophilidae (Collier and MacIntyre, 1977).

摘要

采用科利尔等人(1976年)的方法,从八种果蝇中纯化出二聚体酶α-甘油磷酸脱氢酶。这些酶在高pH值下失活,并确定了足以使其重新激活的条件。在两种果蝇的酶失活后混合的重新激活的α-甘油磷酸脱氢酶的电泳图谱表明,高pH值会使该酶解离成其组成亚基,重新激活涉及亚基重新结合。让20种解离酶的种间组合进行重新结合,并通过密度测定法测定异源特异性和同源特异性酶活性及蛋白质的含量。在所有20次测试中,观察到的异源特异性:同源特异性酶比率与预期值之间没有差异。这些结果与果蝇科中这种酶非常缓慢的进化速率一致(科利尔和麦金太尔,1977年)。

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