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鸡肠道刷状缘膜中蔗糖酶-异麦芽糖酶和麦芽糖酶-葡糖淀粉酶的锚定模式及前体形式。系统发育意义。

The mode of anchoring and precursor forms of sucrase-isomaltase and maltase-glucoamylase in chicken intestinal brush-border membrane. Phylogenetic implications.

作者信息

Hu C B, Spiess M, Semenza G

出版信息

Biochim Biophys Acta. 1987 Jan 26;896(2):275-86. doi: 10.1016/0005-2736(87)90188-x.

Abstract

Chicken intestinal sucrase-isomaltase and maltase-glucoamylase have been isolated in their intact form by detergent solubilization and characterized as to their subunit composition and mode of anchoring in the brush-border membrane. Both are heterodimeric enzyme complexes composed of two subunits each of approximately 140 and 130 kDa. Contrary to the mammalian sucrase-isomaltase, chicken isomaltase was identified as the smaller of the two subunits. As was shown by hydrophobic labeling, only one of the two subunits in each heterodimer is anchored in the bilayer, the smaller 130 kDa isomaltase subunit of the sucrase-isomaltase complex, and the larger 140 kDa subunit of the maltase-glucoamylase complex. Both preparations contain a high-molecular weight polypeptide of approximately 250 kDa which in the case of sucrase-isomaltase could be identified by peptide mapping as a single-chain precursor not (yet) proteolytically processed to the final heterodimer. These first data on the mode of membrane anchoring of non-mammalian glycosidases indicate that they are synthesized, inserted into the membrane, and processed in ways similar to the mammalian enzymes. The fundamental unity between avian and mammalian sucrase-isomaltases suggests that the partial gene duplication of an ancestral isomaltase gene and the subsequent mutation of one of the active sites resulting in pro-sucrase-isomaltase has occurred prior to the separation of mammals from reptiles, i.e. more than 300 million years ago.

摘要

鸡肠道蔗糖酶 - 异麦芽糖酶和麦芽糖酶 - 葡糖淀粉酶已通过去污剂增溶法以完整形式分离出来,并对其亚基组成和在刷状缘膜中的锚定方式进行了表征。两者都是异二聚体酶复合物,各自由两个亚基组成,分子量分别约为140 kDa和130 kDa。与哺乳动物的蔗糖酶 - 异麦芽糖酶相反,鸡的异麦芽糖酶被鉴定为两个亚基中较小的那个。如疏水标记所示,每个异二聚体中的两个亚基只有一个锚定在双层膜中,蔗糖酶 - 异麦芽糖酶复合物中较小的130 kDa异麦芽糖酶亚基,以及麦芽糖酶 - 葡糖淀粉酶复合物中较大的140 kDa亚基。两种制剂都含有一种分子量约为250 kDa的高分子量多肽,就蔗糖酶 - 异麦芽糖酶而言,通过肽图谱分析可将其鉴定为尚未经过蛋白水解加工成最终异二聚体的单链前体。这些关于非哺乳动物糖苷酶膜锚定方式的初步数据表明,它们的合成、插入膜以及加工方式与哺乳动物酶相似。禽类和哺乳动物蔗糖酶 - 异麦芽糖酶之间的基本统一性表明,祖先异麦芽糖酶基因的部分基因复制以及随后一个活性位点的突变导致原蔗糖酶 - 异麦芽糖酶的出现发生在哺乳动物与爬行动物分化之前,即超过3亿年前。

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