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人绒毛膜癌细胞合成的绒毛膜促性腺激素αβ二聚体以及未结合的α和β亚基的加工与分泌的动力学比较。

A kinetic comparison of the processing and secretion of the alpha beta dimer and the uncombined alpha and beta subunits of chorionic gonadotropin synthesized by human choriocarcinoma cells.

作者信息

Peters B P, Krzesicki R F, Hartle R J, Perini F, Ruddon R W

出版信息

J Biol Chem. 1984 Dec 25;259(24):15123-30.

PMID:6210286
Abstract

Human choriocarcinoma cells (JAR) synthesize the alpha and beta subunits of the glycoprotein hormone chorionic gonadotropin (hCG) (R.W. Ruddon, C.A. Hanson, A. H. Bryan, G.J. Putterman, E.L. White, F. Perini, K. S. Meade, and P.H. Aldenderfer (1980) J. Biol. Chem. 255, 1000-1007). In addition to the hCG dimer (alpha beta), JAR cells secrete uncombined alpha and beta subunits into the culture medium (L.A. Cole, R.J. Hartle, J.A. Laferla, and R.W. Ruddon (1983) Endocrinology 113, 1176-1178). Pulse-chase studies with [35S]methionine or [3H]mannose were carried out in order to compare free alpha, free beta, and the alpha beta dimer with regard to the kinetics of synthesis, N-linked oligosaccharide processing, and secretion and to determine the kinetics of alpha-beta subunit combination. A panel of three antisera was used to immunoprecipitate directly the free subunits and the alpha beta dimer sequentially from the same cell lysates and culture media. The alpha subunit of hCG was synthesized in a slight molar excess (1.2-1.5-fold) over the beta subunit, and alpha beta dimer was rapidly formed by combination of the intracellular alpha and beta precursors. Dimer formation was already apparent in JAR cells following a 10-min biosynthetic labeling incubation with [35S]methionine. The combination of subunits ceased by 30 min of chase even though 51% of alpha and 44% of beta remained free within the cells. Combination of the alpha and beta precursors had occurred before their N-linked oligosaccharides were processed beyond the Man8GlcNAc2 structure. The initial trimming of glucosyl and mannosyl units from the high-mannose oligosaccharides of the hCG precursors occurred more rapidly for free alpha and CG-alpha than for free beta and CG-beta. JAR cells accumulated alpha precursors bearing mostly Man8GlcNAc2 units and beta precursors bearing Man8GlcNAc2 units that represent the substrates of the rate-limiting step in the secretory pathway. In spite of the fact that their N-linked oligosaccharides were trimmed at different rates, free alpha, free beta, and alpha beta dimer were all secreted into the medium at the same rate, with a half-time of 35 min. The secreted hCG forms were stable in the chase medium between 4 and 8h, indicating that extracellular degradation, combination of free subunits to form dimer, or dissociation of dimer to form free subunits did not occur.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

人绒毛膜癌细胞(JAR)能合成糖蛋白激素绒毛膜促性腺激素(hCG)的α和β亚基(R.W. 鲁登、C.A. 汉森、A.H. 布莱恩、G.J. 帕特曼、E.L. 怀特、F. 佩里尼、K.S. 米德和P.H. 阿尔登德弗(1980年)《生物化学杂志》255卷,1000 - 1007页)。除了hCG二聚体(αβ)外,JAR细胞还将未结合的α和β亚基分泌到培养基中(L.A. 科尔、R.J. 哈特尔、J.A. 拉弗拉和R.W. 鲁登(1983年)《内分泌学》113卷,1176 - 1178页)。用[35S]甲硫氨酸或[3H]甘露糖进行脉冲追踪研究,以便比较游离α、游离β和αβ二聚体在合成动力学、N - 连接寡糖加工、分泌方面的情况,并确定α - β亚基结合的动力学。使用一组三种抗血清从同一细胞裂解物和培养基中依次直接免疫沉淀游离亚基和αβ二聚体。hCG的α亚基合成量比β亚基略多(1.2 - 1.5倍),细胞内的α和β前体迅速结合形成αβ二聚体。在用[35S]甲硫氨酸进行10分钟生物合成标记孵育后,JAR细胞中已经明显形成二聚体。追踪30分钟后亚基结合停止,尽管细胞内仍有51%的α和44%的β保持游离状态。α和β前体在其N - 连接寡糖加工到超过Man8GlcNAc2结构之前就已经发生了结合。hCG前体高甘露糖寡糖中葡萄糖基和甘露糖基单元的初始修剪,游离α和CG - α比游离β和CG - β发生得更快。JAR细胞积累了主要带有Man8GlcNAc2单元的α前体和带有Man8GlcNAc2单元的β前体,这些代表了分泌途径中限速步骤的底物。尽管它们的N - 连接寡糖以不同速率修剪,但游离α、游离β和αβ二聚体都以相同速率分泌到培养基中,半衰期为35分钟。分泌的hCG形式在追踪培养基中4至8小时内稳定,表明细胞外降解、游离亚基结合形成二聚体或二聚体解离形成游离亚基均未发生。(摘要截短至400字)

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