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促甲状腺激素对猪甲状腺细胞培养物中与环磷酸腺苷依赖性蛋白激酶调节亚基结合的环磷酸腺苷的作用。

TSH action on cAMP binding to the regulatory subunits of cAMP-dependent protein kinases in pig thyroid cell cultures.

作者信息

Ben Abdelkhalek M, Breton M F, Feliers D, Haye B, Pavlovic-Hournac M

机构信息

Laboratoire de Physiologie Animale, Faculté des Sciences, Rabat, Marocco.

出版信息

Mol Cell Endocrinol. 1994 Feb;99(1):103-10. doi: 10.1016/0303-7207(94)90152-x.

DOI:10.1016/0303-7207(94)90152-x
PMID:7514548
Abstract

This study examines the mechanism of TSH action on the cAMP-dependent protein kinases (PKA) by measuring the catalytic activity of the two PKA isozymes (PKA I and PKA II) and their capacity to bind cAMP to the regulatory subunits (RI and RII) in thyroid cell cultures exposed for two days to different doses of TSH. In TSH-treated cell cultures a selective down regulation (up to 60%) of the catalytic activity was found; the PKA I was down regulated at lower TSH doses (0.1 mU/ml and even 0.05 mU/ml) than was the PKA II (1.0 mU/ml TSH). At the dose of 1.0 mU/ml the loss of the catalytic activity in PKA I and PKA II was respectively 60% and 40%. No free catalytic activity was found either in control or in TSH-treated cells. Binding of cAMP to regulatory subunits (R) measured under exchange conditions at 37 degrees C, showed that no change in total regulatory subunit protein content occurs in TSH-treated cells. Binding of cAMP to R subunits at 4 degrees C (when only free cAMP binding sites are measured) revealed an important endogenous occupancy of cAMP binding sites of RI and RII isoreceptors under basal conditions (40%) and a significantly increased occupancy after exposure of cells to TSH (60%). Pools of regulatory subunits with more than 50% of sites occupied, which were devoid of enzyme activity, were found both, in control and TSH-exposed cells. They were identified as RI subunits which represented a mixed population of native and partly degraded molecules.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

本研究通过测量两种蛋白激酶A同工酶(PKA I和PKA II)的催化活性及其在不同剂量促甲状腺激素(TSH)作用两天的甲状腺细胞培养物中与调节亚基(RI和RII)结合环磷酸腺苷(cAMP)的能力,来研究TSH对环磷酸腺苷依赖性蛋白激酶(PKA)的作用机制。在TSH处理的细胞培养物中,发现催化活性有选择性下调(高达60%);PKA I在比PKA II更低的TSH剂量(0.1 mU/ml甚至0.05 mU/ml)下就被下调(PKA II在1.0 mU/ml TSH时被下调)。在1.0 mU/ml剂量下,PKA I和PKA II的催化活性损失分别为60%和40%。在对照细胞和TSH处理的细胞中均未发现游离催化活性。在37℃交换条件下测量cAMP与调节亚基(R)的结合,结果表明TSH处理的细胞中调节亚基总蛋白含量没有变化。在4℃测量cAMP与R亚基的结合(此时仅测量游离cAMP结合位点)显示,在基础条件下RI和RII同种受体的cAMP结合位点有重要的内源性占据(40%),细胞暴露于TSH后占据率显著增加(60%)。在对照细胞和TSH处理的细胞中均发现了超过50%位点被占据且缺乏酶活性的调节亚基池。它们被鉴定为RI亚基,代表天然和部分降解分子的混合群体。(摘要截断于250字)

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