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钙调蛋白的第四个EF手型结构域及其螺旋-环-螺旋组件:对钙结合和酶激活的影响。

The fourth EF-hand of calmodulin and its helix-loop-helix components: impact on calcium binding and enzyme activation.

作者信息

George S E, Su Z, Fan D, Wang S, Johnson J D

机构信息

Department of Medicine, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

Biochemistry. 1996 Jun 25;35(25):8307-13. doi: 10.1021/bi960495y.

DOI:10.1021/bi960495y
PMID:8679587
Abstract

CaM (4 cTnC) is a calmodulin--cardiac troponin C chimeric protein containing the first, second, and third calcium-binding EF-hands of calmodulin (CaM) and the fourth EF-hand of cardiac troponin C (cTnC) [George, S.E., Su, Z., Fan, D., & Means, A.R. (1993) J. Biol. Chem. 268, 25213-25220]. CaM (4 cTnC) showed 2-fold-enhanced carboxy-terminal Ca2+ affinity relative to CaM and also exhibited impaired activation of the CaM-regulated enzymes smooth muscle myosin light chain kinase (smMLCK), neuronal nitric oxide synthase (nNOS), and phosphodiesterase (PDE). To investigate the molecular basis for these effects, we constructed (1) additional chimeras, replacing most of CaM helix 7, Ca2+-binding loop 4, and helix 8 with the corresponding helices and loops of cTnC; and (2) point mutants in the fourth EF-hand of CaM. Replacement of CaM's fourth loop with the corresponding loop of cTnC enhanced Ca2+ affinity by over 3-fold through an increase in the Ca2+ on rate and also reduced cooperativity of Ca2+ binding. In contrast, substitution of CaM helix 7 or 8 modestly decreased Ca2+ affinity by increasing the Ca2+ off rate, without impairment of cooperativity. All three of the helix and loop chimeras fully activated PDE, with minor shifts in Kact. CaM (helix 7 cTnC) showed a significantly impaired ability to activate smMLCK and nNOS, whereas the other two chimeras retained about 80% of the maximal smMLCK and nNOS activation observed with CaM.

摘要

CaM (4 cTnC) 是一种钙调蛋白-心肌肌钙蛋白C嵌合蛋白,它包含钙调蛋白(CaM)的第一、第二和第三个钙结合EF手型结构域以及心肌肌钙蛋白C(cTnC)的第四个EF手型结构域[乔治,S.E.,苏,Z.,范,D.,& 米恩斯,A.R.(1993年)《生物化学杂志》268卷,25213 - 25220页]。与CaM相比,CaM (4 cTnC) 的羧基末端对Ca2+ 的亲和力提高了2倍,并且对CaM调节的酶平滑肌肌球蛋白轻链激酶(smMLCK)、神经元型一氧化氮合酶(nNOS)和磷酸二酯酶(PDE)的激活能力受损。为了研究这些效应的分子基础,我们构建了:(1)其他嵌合体,用cTnC相应的螺旋和环取代CaM的大部分螺旋7、钙结合环4和螺旋8;以及(2)CaM第四个EF手型结构域中的点突变体。用cTnC相应的环取代CaM的第四个环,通过增加Ca2+ 的结合速率,使Ca2+ 亲和力提高了3倍以上,同时也降低了Ca2+ 结合的协同性。相比之下,取代CaM的螺旋7或8通过增加Ca2+ 的解离速率适度降低了Ca2+ 亲和力,但不影响协同性。所有三种螺旋和环嵌合体均能完全激活PDE,激活常数(Kact)有微小变化。CaM(螺旋7 cTnC)激活smMLCK和nNOS的能力显著受损,而其他两种嵌合体保留了约80% 的CaM观察到的smMLCK和nNOS最大激活能力。

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