首页> 美国卫生研究院文献>Biochemical Journal >Proteins of the kidney microvillar membrane. Reconstitution of endopeptidase in liposomes shows that it is a short-stalked protein.
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Proteins of the kidney microvillar membrane. Reconstitution of endopeptidase in liposomes shows that it is a short-stalked protein.

机译:肾微绒毛膜的蛋白质。脂质体中内肽酶的重建表明它是一种短柄蛋白。

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摘要

Pig kidney microvillar proteins were extracted with octyl beta-glucoside and reconstituted in liposomes prepared from microvillar lipids of known composition. Four peptidases, namely endopeptidase (EC 3.4.24.11), aminopeptidases N (EC 3.4.11.2) and A (EC 3.4.11.7) and dipeptidyl peptidase IV (EC 3.4.14.5), were shown to be reconstituted. At lipid/protein ratios greater than 4:1, about half the detergent-solubilized protein and nearly all of the activity of the four peptidases were reconstituted. Dissolution of the liposomes with Triton X-100 did not increase the activity of any of these peptidases, a result consistent with an asymmetric, 'right-side-out', orientation of these enzymes. When purified, endopeptidase was subjected to the same procedure; the two amphipathic forms of the enzyme (the detergent form and the trypsin-treated detergent form) were fully reconstituted. The amphiphilic form, purified after toluene/trypsin treatment, failed to reconstitute. Electron microscopy of microvilli showed that the appearance of the surface particles was profoundly altered by treatment with papain. Before treatment, the microvilli were coated with particles of stalk lengths ranging from 2.5 to 9 nm. After papain treatment nearly all the particles had stalks of 2-3 nm. Reconstituted microvillar proteins in liposomes showed the same heterogeneity of stalk length. In contrast, liposomes containing reconstituted endopeptidase revealed a very homogeneous population of particles of stalk length 2 nm. Since the smallest dimension of a papain molecule is 3.7 nm, the ability of papain, and other proteinases of similar molecular size, to release microvillar enzymes is crucially affected by the length of the junctional peptide that constitutes the stalk of this type of membrane protein.
机译:用辛基β-葡萄糖苷提取猪肾微绒毛蛋白,并在由已知组成的微绒毛脂质制备的脂质体中重构。已证明重组了四个肽酶,即内肽酶(EC 3.4.24.11),氨基肽酶N(EC 3.4.11.2)和A(EC 3.4.11.7)和二肽基肽酶IV(EC 3.4.14.5)。当脂质/蛋白质比率大于4:1时,约有一半的去污剂溶解的蛋白质和四种肽酶的几乎所有活性均被重建。用Triton X-100溶解脂质体不会增加任何这些肽酶的活性,其结果与这些酶的不对称“右侧向外”方向一致。纯化后,对肽链内切酶进行相同的操作;酶的两种两亲形式(去垢剂形式和经胰蛋白酶处理的去垢剂形式)被完全重构。在甲苯/胰蛋白酶处理后纯化的两亲形式未能重构。电镜观察到的微绒毛表明,木瓜蛋白酶处理后表面颗粒的外观发生了深刻的变化。在处理之前,微绒毛被茎长度在2.5至9 nm范围内的颗粒覆盖。木瓜蛋白酶处理后,几乎所有颗粒都具有2-3 nm的茎。脂质体中重构的微绒毛蛋白显示出相同的茎长异质性。相反,含有重构的内肽酶的脂质体显示出茎长度为2 nm的颗粒非常均匀。由于木瓜蛋白酶分子的最小尺寸为3.7 nm,因此木瓜蛋白酶和其他类似分子大小的蛋白酶释放微绒毛酶的能力受到构成这种膜蛋白茎的连接肽长度的关键影响。

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