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体内心脏中蛋白激酶A与A激酶锚定蛋白相互作用的破坏:对心脏收缩性、蛋白激酶A磷酸化及肌钙蛋白I蛋白水解的影响

Disruption of protein kinase A interaction with A-kinase-anchoring proteins in the heart in vivo: effects on cardiac contractility, protein kinase A phosphorylation, and troponin I proteolysis.

作者信息

McConnell Bradley K, Popovic Zoran, Mal Niladri, Lee Kwangdeok, Bautista James, Forudi Farhad, Schwartzman Raul, Jin J-P, Penn Marc, Bond Meredith

机构信息

Department of Physiology and Department of Medicine, University of Maryland School of Medicine, Baltimore, Maryland 21201, USA.

出版信息

J Biol Chem. 2009 Jan 16;284(3):1583-92. doi: 10.1074/jbc.M806321200. Epub 2008 Oct 21.

DOI:10.1074/jbc.M806321200
PMID:18945669
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2615525/
Abstract

Protein kinase A (PKA)-dependent phosphorylation is regulated by targeting of PKA to its substrate as a result of binding of regulatory subunit, R, to A-kinase-anchoring proteins (AKAPs). We investigated the effects of disrupting PKA targeting to AKAPs in the heart by expressing the 24-amino acid regulatory subunit RII-binding peptide, Ht31, its inactive analog, Ht31P, or enhanced green fluorescent protein by adenoviral gene transfer into rat hearts in vivo. Ht31 expression resulted in loss of the striated staining pattern of type II PKA (RII), indicating loss of PKA from binding sites on endogenous AKAPs. In the absence of isoproterenol stimulation, Ht31-expressing hearts had decreased +dP/dtmax and -dP/dtmin but no change in left ventricular ejection fraction or stroke volume and decreased end diastolic pressure versus controls. This suggests that cardiac output is unchanged despite decreased +dP/dt and -dP/dt. There was also no difference in PKA phosphorylation of cardiac troponin I (cTnI), phospholamban, or ryanodine receptor (RyR2). Upon isoproterenol infusion, +dP/dtmax and -dP/dtmin did not differ between Ht31 hearts and controls. At higher doses of isoproterenol, left ventricular ejection fraction and stroke volume increased versus isoproterenol-stimulated controls. This occurred in the context of decreased PKA phosphorylation of cTnI, RyR2, and phospholamban versus controls. We previously showed that expression of N-terminal-cleaved cTnI (cTnI-ND) in transgenic mice improves cardiac function. Increased cTnI N-terminal truncation was also observed in Ht31-expressing hearts versus controls. Increased cTnI-ND may help compensate for reduced PKA phosphorylation as occurs in heart failure.

摘要

蛋白激酶A(PKA)依赖性磷酸化通过调节亚基R与A激酶锚定蛋白(AKAPs)结合,将PKA靶向其底物来进行调控。我们通过腺病毒基因转染法将24个氨基酸的调节亚基RII结合肽Ht31、其无活性类似物Ht31P或增强型绿色荧光蛋白导入大鼠心脏,研究在心脏中破坏PKA与AKAPs靶向结合的影响。Ht31的表达导致II型PKA(RII)的横纹状染色模式消失,表明PKA从内源性AKAPs的结合位点上脱离。在没有异丙肾上腺素刺激的情况下,表达Ht31的心脏的 +dP/dtmax和 -dP/dtmin降低,但左心室射血分数、每搏输出量没有变化,与对照组相比舒张末期压力降低。这表明尽管 +dP/dt和 -dP/dt降低,但心输出量未改变。心肌肌钙蛋白I(cTnI)、受磷蛋白或兰尼碱受体(RyR2)的PKA磷酸化也没有差异。注入异丙肾上腺素后,Ht31心脏与对照组之间的 +dP/dtmax和 -dP/dtmin没有差异。在较高剂量的异丙肾上腺素作用下,与异丙肾上腺素刺激的对照组相比,左心室射血分数和每搏输出量增加。这发生在与对照组相比cTnI、RyR2和受磷蛋白的PKA磷酸化降低的情况下。我们之前表明,在转基因小鼠中表达N端裂解的cTnI(cTnI-ND)可改善心脏功能。与对照组相比,在表达Ht31的心脏中也观察到cTnI N端截短增加。增加的cTnI-ND可能有助于补偿心力衰竭时发生的PKA磷酸化减少。

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AKAP complex regulates Ca2+ re-uptake into heart sarcoplasmic reticulum.A激酶附着蛋白复合体调节钙离子重新摄取进入心脏肌浆网。
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The intermediate filament protein, synemin, is an AKAP in the heart.中间丝蛋白丝连蛋白是心脏中的一种A激酶附着蛋白。
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Scaling of diastolic intraventricular pressure gradients is related to filling time duration.舒张期心室内压力梯度的缩放与充盈持续时间有关。
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