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激动剂诱导鸟嘌呤核苷酸结合调节蛋白Gq和G11的α亚基以及毒蕈碱型m1乙酰胆碱受体从质膜转移至轻小泡膜组分。

Agonist-induced transfer of the alpha subunits of the guanine-nucleotide-binding regulatory proteins Gq and G11 and of muscarinic m1 acetylcholine receptors from plasma membranes to a light-vesicular membrane fraction.

作者信息

Svoboda P, Milligan G

机构信息

Department of Biochemistry, University of Glasgow, Scotland.

出版信息

Eur J Biochem. 1994 Sep 1;224(2):455-62. doi: 10.1111/j.1432-1033.1994.00455.x.

Abstract

A clone of a Chinese hamster ovary (CHO) cell line expressing high levels of the human muscarinic M1 acetylcholine (Hm1) receptor undergoes a substantial agonist-specific down-regulation of both Hm1 receptors and the alpha subunits of the guanine-nucleotide-binding (G)-proteins Gq and G11 which is accompanied by a desensitization of inositol-phospholipid-specific-phospholipase-C response [Mullaney, I., Dodd, M. W., Buckley, N. J. & Milligan, G. (1993) Biochem. J. 289, 125-131]. To examine early events in this process, the effect of agonist on subcellular distribution of Gq alpha and G11 alpha and of Hm1 receptors was assessed after short-term and long-term treatment with carbachol. Short-term (30 min) incubation with carbachol (1 mM) induced a simultaneous transfer of a proportion of both Gq alpha and G11 alpha and Hm1 receptors from plasma membranes to distinct light vesicular membranes. The total number of receptors and of Gq alpha and G11 alpha in each cell remained unchanged under these conditions. A similar transfer was noted for the G-protein Gs alpha but not for intrinsic plasma membrane markers. The plasma membrane, as well as light vesicular membrane, pool of Gs alpha subunit was unaffected by further sustained incubation with carbachol (16 h), whereas Hm1 receptors and both Gq alpha and G11 alpha proteins were down-regulated to 25% and 40%, respectively, when compared with untreated cells. Such observations support the idea that down-regulation of both the Hm1 receptor and its associated inositol-phospholipid-specific-phospholipase-C-linked G-proteins is produced by two sequential steps. The first is a transfer of signal-transducing polypeptides from the plasma membrane to a non-plasma membrane light vesicle fraction. The second step is represented by an agonist-specific down-regulation pathway. Both the Hm1 receptor and Gq alpha/G11 alpha appear to follow similar sequestration and down-regulation patterns.

摘要

一株表达高水平人毒蕈碱型M1乙酰胆碱(Hm1)受体的中国仓鼠卵巢(CHO)细胞系,其Hm1受体以及鸟嘌呤核苷酸结合(G)蛋白Gq和G11的α亚基会发生显著的激动剂特异性下调,同时伴有肌醇磷脂特异性磷脂酶C反应的脱敏[Mullaney, I., Dodd, M. W., Buckley, N. J. & Milligan, G. (1993) Biochem. J. 289, 125 - 131]。为了研究这一过程中的早期事件,在用卡巴胆碱进行短期和长期处理后,评估了激动剂对Gqα和G11α以及Hm1受体亚细胞分布的影响。用卡巴胆碱(1 mM)短期(30分钟)孵育诱导了一部分Gqα和G11α以及Hm1受体同时从质膜转移到不同的轻囊泡膜。在这些条件下,每个细胞中受体以及Gqα和G11α的总数保持不变。对于G蛋白Gsα也观察到了类似的转移,但对于内在质膜标记物则没有。Gsα亚基的质膜池以及轻囊泡膜池不受与卡巴胆碱(16小时)进一步持续孵育的影响,而与未处理的细胞相比,Hm1受体以及Gqα和G11α蛋白分别下调至25%和40%。这些观察结果支持这样一种观点,即Hm1受体及其相关的肌醇磷脂特异性磷脂酶C连接的G蛋白的下调是由两个连续步骤产生的。第一步是信号转导多肽从质膜转移到非质膜轻囊泡部分。第二步由激动剂特异性下调途径代表。Hm1受体和Gqα/G11α似乎遵循相似的隔离和下调模式。

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