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对用激素处理过的脂肪细胞粗膜中环磷酸腺苷(cAMP)合成与降解的相对速率进行检测。

Examination of relative rates of cAMP synthesis and degradation in crude membranes of adipocytes treated with hormones.

作者信息

Gettys T W, Okonogi K, Tarry W C, Johnston J, Horton C, Taylor I L

机构信息

Department of Medicine, Duke Medical Center, Durham, NC.

出版信息

Second Messengers Phosphoproteins. 1990;13(1):37-49.

PMID:1962820
Abstract

The impact of changes in the activation state of the low Km cAMP phosphodiesterase (PDE) on cAMP output in adipocyte membranes was assessed by measuring the product of cAMP synthesis and degradation in the membrane preparation simultaneously. Crude membranes were prepared from adipocytes treated with the cAMP analog, 8-pCl phi S-cAMP and from adipocytes treated with 2 nM insulin. Using membranes from control and treated cells, adenylate cyclase was activated with various concentrations of forskolin and cAMP production (synthesis minus degradation) was measured with and without complete PDE inhibition using the specific inhibitor CI-914. Half maximal inhibition of the low Km cAMP PDEs in control membranes was produced by 1.16 +/- 0.07 microM CI-914 and greater than 98% of the activity was inhibited by 100 microM CI-914. The I50 and the concentration of CI-914 producing complete PDE inhibition in membranes from 8-pCl phi S-cAMP or insulin-treated cells were identical to those seen in membranes from control cells. Treatment of adipocytes with 8-pCl phi S-cAMP or with insulin did not modify basal rates of cAMP synthesis or alter the ability of adenylate cyclase to be activated by forskolin. The impact of PDE activity on cAMP accumulation was relatively small in membranes from control cells, but treatment of adipocytes with 8-pCl phi S-cAMP or with insulin activated the low Km cAMP PDE and caused a marked decrease in cAMP accumulation.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过同时测量脂肪细胞膜制剂中cAMP合成与降解的产物,评估低Km cAMP磷酸二酯酶(PDE)激活状态的变化对脂肪细胞膜中cAMP输出的影响。粗制膜取自用cAMP类似物8-pCl phi S-cAMP处理的脂肪细胞以及用2 nM胰岛素处理的脂肪细胞。使用对照细胞和处理后细胞的膜,用不同浓度的福司可林激活腺苷酸环化酶,并使用特异性抑制剂CI-914在有或无完全PDE抑制的情况下测量cAMP生成量(合成减去降解)。对照膜中低Km cAMP PDEs的半数最大抑制浓度为1.16±0.07 microM CI-914,100 microM CI-914可抑制超过98%的活性。8-pCl phi S-cAMP或胰岛素处理细胞的膜中,CI-914产生完全PDE抑制的I50和浓度与对照细胞膜中的相同。用8-pCl phi S-cAMP或胰岛素处理脂肪细胞不会改变cAMP合成的基础速率,也不会改变腺苷酸环化酶被福司可林激活的能力。在对照细胞的膜中,PDE活性对cAMP积累的影响相对较小,但用8-pCl phi S-cAMP或胰岛素处理脂肪细胞会激活低Km cAMP PDE,并导致cAMP积累显著减少。(摘要截短于250字)

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