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牛心激活剂依赖性环核苷酸磷酸二酯酶的特性

Properties of the activator-dependent cyclic nucleotide phosphodiesterase from bovine heart.

作者信息

Donnelly T E

出版信息

Biochim Biophys Acta. 1977 Jan 11;480(1):194-203. doi: 10.1016/0005-2744(77)90333-3.

DOI:10.1016/0005-2744(77)90333-3
PMID:188479
Abstract

In the absence of activator, the activator-dependent cyclic nucleotide phosphodiesterase (EC 3.1.4.-) from bovine heart hydrolyzed 3.2-fold more cyclic GMP than cyclic AMP when assayed with 10(-6) M substrate in the presence of 5 mM Mg2+ and 10 muM Ca2+. The addition of saturating amounts of phosphodiesterase activator increased the hydrolysis of cyclic GMP 8-fold and cyclic AMP 6-fold. The pH maxima of the enzyme was rather broad from 6.0 to 7.0 for the hydrolysis of both cyclic GMP and cyclic AMP in the absnece or presence of phosphodiesterase activator. Substrate specificity of the enzyme in the absence or presence of phosphodiesterase activator varied depending on the divalent metal used to support activity in the absence of activator. The enzyme preferentially hydrolyzed cyclic GMP in the presence of Mg2+ while little substrate specificity was observed in the presence of Mn2+, Zn2+, Co2+ or Ni2+. The magnitude of the increase in enzyme activity due to activator and Ca2+ varied depending on the divalent metal used to support enzyme activity without activator. The addition of activator increased the V of cyclic AMP hydrolysis 1.7-fold while causing no significant change in the Km for cyclic AMP. Two apparent Km values for cyclic GMP (1 and 15 muM) were noted in the absence of activator and upon the addition of activator a single apparent Km (3 muM) was observed with a V approx. 2-fold above that in the absence of activator. Cyclic AMP competitively inhibitied the hydrolysis of cyclic GMP with a ki of 50 muM while cyclic GMP non-competitively inhibited the hydrolysis of cyclic AMP with a Ki of 1.8 muM. The results suggest there may be two or more binding sites for cyclic GMP on the enzyme and possibly only one binding site for cyclic AMP.

摘要

在没有激活剂的情况下,当在5 mM Mg2+和10 μM Ca2+存在下用10(-6) M底物进行测定时,来自牛心脏的依赖激活剂的环核苷酸磷酸二酯酶(EC 3.1.4.-)水解环鸟苷酸(cGMP)的能力比环腺苷酸(cAMP)高3.2倍。添加饱和量的磷酸二酯酶激活剂可使cGMP的水解增加8倍,cAMP的水解增加6倍。在没有或存在磷酸二酯酶激活剂的情况下,该酶水解cGMP和cAMP的最适pH范围相当宽,为6.0至7.0。在没有或存在磷酸二酯酶激活剂的情况下,该酶的底物特异性取决于在没有激活剂时用于支持活性的二价金属。在Mg2+存在下,该酶优先水解cGMP,而在Mn2+、Zn2+、Co2+或Ni2+存在下几乎没有观察到底物特异性。由于激活剂和Ca2+导致的酶活性增加幅度取决于在没有激活剂时用于支持酶活性的二价金属。添加激活剂使cAMP水解的V增加1.7倍,而对cAMP的Km没有显著影响。在没有激活剂时,观察到cGMP有两个表观Km值(1和15 μM),添加激活剂后,观察到一个单一的表观Km(3 μM),V比没有激活剂时高约2倍。cAMP竞争性抑制cGMP的水解,ki为50 μM,而cGMP非竞争性抑制cAMP的水解,Ki为1.8 μM。结果表明,该酶上可能有两个或更多cGMP结合位点,而cAMP可能只有一个结合位点。

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Biochem J. 1985 Mar 15;226(3):897-900. doi: 10.1042/bj2260897.