Epinephrine-induced sequestration of the beta-adrenergic receptor in cultured S49 WT and cyc- lymphoma cells.

R B Clark, J Friedman, N Prashad, A E Ruoho
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Abstract

Pretreatment of either intact wild type S49 lymphoma cells (WT) or the uncoupled variants, cyc-, H21a, or UNC with epinephrine results in the redistribution of 20-30% of the beta-adrenergic receptors into a light vesicle fraction in sucrose gradients. Since the variants are uncoupled with respect to hormonal stimulation of adenylate cyclase, it appears that productive interaction with Gs is not required for the sequestration of beta-adrenergic receptors. Characterization of the epinephrine-induced redistribution of the beta-adrenergic receptor has revealed the following: The EC50 for the redistribution in WT cells was between 100 and 200 nM. Pretreatment of WT cells with 50 nM epinephrine for 30 min induced only a slight redistribution of receptors in sucrose gradients but produced a significant desensitization of adenylate cyclase. The desensitization was characterized by an increase in the Kact of epinephrine stimulation of adenylate cyclase while the Vmax was unaltered. Pretreatment with 10 microM epinephrine resulted in a significant decrease in the Vmax (50%) of epinephrine stimulation of adenylate cyclase and a 3-fold increase in Kact in the heavy vesicles. The beta-receptors in the light vesicle fraction of WT were uncoupled from adenylate cyclase and displayed low affinity for epinephrine binding, comparable to the cyc-. The "desensitized" receptor in the light vesicle fractions of cyc- was capable of stimulating adenylate following reconstitution with cholate extracts of WT membranes containing Gs. The molecular weight of the photolabeled beta-receptor in the light vesicle fractions (65,000 +/- 2,000) was not significantly different from the Mr 65,000 polypeptide photolabeled in the heavy fractions. The Mr 55,000 beta-receptor polypeptide was not detected in the light vesicles. Our results suggest first that the redistribution of the beta-receptor into light vesicles may follow an earlier stage of desensitization, and second that the beta-receptor in light vesicles while sequestered from Gs is capable of activating adenylate cyclase.

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肾上腺素诱导的-肾上腺素能受体在培养的s49wt和cyc-淋巴瘤细胞中的隔离。
用肾上腺素预处理完整的野生型S49淋巴瘤细胞(WT)或未偶联的cyc-、H21a或UNC,可导致20-30%的β -肾上腺素能受体在蔗糖梯度中重新分布到轻的囊泡部分。由于这些变异与腺苷酸环化酶的激素刺激不耦合,因此β -肾上腺素能受体的隔离似乎不需要与Gs产生有效的相互作用。对肾上腺素诱导的β -肾上腺素能受体再分配的表征显示:WT细胞中再分配的EC50在100 ~ 200 nM之间。用50 nM的肾上腺素预处理WT细胞30分钟,仅诱导受体在蔗糖梯度上的轻微重新分布,但产生了腺苷酸环化酶的显著脱敏。脱敏的特点是肾上腺素刺激腺苷酸环化酶的Kact增加,而Vmax不变。10微米肾上腺素预处理导致肾上腺素刺激腺苷酸环化酶的Vmax显著降低(50%),重囊中Kact增加3倍。WT轻囊泡部分的β受体与腺苷酸环化酶解偶联,对肾上腺素的结合表现出较低的亲和力,与环化酶相似。cyc-的轻囊泡部分中的“脱敏”受体能够在含Gs的WT膜的胆酸提取物重建后刺激腺苷酸。光标记的β受体在轻囊泡组分(65,000 +/- 2,000)中的分子量与在重囊泡组分中光标记的Mr 65,000多肽的分子量没有显著差异。在轻囊泡中未检测到Mr 55000 β受体多肽。我们的研究结果表明,首先,β受体重新分布到轻囊泡中可能遵循早期的脱敏阶段,其次,轻囊泡中的β受体在与Gs隔离时能够激活腺苷酸环化酶。
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