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胰岛素原受体通过翻译后修饰获得胰岛素结合活性。与自身免疫抗体识别的相关性。

Post-translational acquisition of insulin binding activity by the insulin proreceptor. Correlation to recognition by autoimmune antibody.

作者信息

Olson T S, Lane M D

出版信息

J Biol Chem. 1987 May 15;262(14):6816-22.

PMID:3553193
Abstract

The post-translational acquisition of ligand binding activity by the insulin receptor was examined in 3T3-L1 adipocytes. In pulse-chase experiments with [35S] methionine, labeled receptor species were separated into "active" and "inactive" forms by affinity chromatography on insulin-agarose and then were characterized and quantitated. It was found that the newly translated high molecular weight proreceptor lacks the capacity to bind insulin. The acquisition of binding activity is relatively slow (t1/2 = 45 min) and occurs prior to conversion of the proreceptor to the mature alpha- and beta-subunits by proteolytic cleavage and maturation of its N-linked oligosaccharide chains (t1/2 = 3 h). Glycosylation appears to be required for this activation since the aglycoproreceptor, synthesized in the presence of tunicamycin, does not acquire insulin binding activity. However, once the proreceptor has acquired ligand binding activity, removal of its N-linked oligosaccharide chains with endoglycosidase H has no effect on the ability of the proreceptor to bind insulin. The modification of the proreceptor to bind insulin. The modification of the proreceptor that gives rise to insulin binding activity most likely involves a conformational change in the binding domain. A human autoimmune antibody that recognizes only the active insulin binding site does not interact with the inactive proreceptor, whereas a rabbit polyclonal antireceptor antibody recognizes all forms. Thus, the autoimmune antibody must recognize a new epitope created during conversion of the inactive proreceptor to the active form.

摘要

在3T3-L1脂肪细胞中研究了胰岛素受体通过翻译后修饰获得配体结合活性的过程。在用[35S]甲硫氨酸进行的脉冲追踪实验中,通过胰岛素-琼脂糖亲和层析将标记的受体种类分离为“活性”和“非活性”形式,然后对其进行表征和定量。结果发现,新翻译的高分子量前体受体缺乏结合胰岛素的能力。结合活性的获得相对较慢(t1/2 = 45分钟),且发生在通过蛋白水解切割和N-连接寡糖链成熟将前体受体转化为成熟的α和β亚基之前(t1/2 = 3小时)。糖基化似乎是这种激活所必需的,因为在衣霉素存在下合成的无糖基前体受体不会获得胰岛素结合活性。然而,一旦前体受体获得了配体结合活性,用内切糖苷酶H去除其N-连接寡糖链对前体受体结合胰岛素的能力没有影响。前体受体结合胰岛素的修饰。导致胰岛素结合活性的前体受体修饰很可能涉及结合结构域的构象变化。一种仅识别活性胰岛素结合位点的人类自身免疫抗体不会与非活性前体受体相互作用,而兔多克隆抗受体抗体则识别所有形式。因此,自身免疫抗体必须识别在非活性前体受体转化为活性形式过程中产生的新表位。

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