Ahnak1 modulates L-type Ca2+ channel inactivation of rodent cardiomyocytes

被引:13
|
作者
Alvarez, Julio L. [2 ]
Petzhold, Daria [1 ]
Pankonien, Ines [1 ,3 ]
Behlke, Joachim [1 ]
Kouno, Michiyoshi [4 ]
Vassort, Guy [5 ]
Morano, Ingo [1 ,3 ]
Haase, Hannelore [1 ]
机构
[1] Max Delbruck Ctr Mol Med MDC, D-13092 Berlin, Germany
[2] Inst Cardiol & Cirugia Cardiovasc, Lab Electrofisiol, Havana, Cuba
[3] Charite, D-13353 Berlin, Germany
[4] Osaka Univ, Dept Social & Environm Med, Osaka, Japan
[5] INSERM, U637, Montpellier 5, France
来源
PFLUGERS ARCHIV-EUROPEAN JOURNAL OF PHYSIOLOGY | 2010年 / 460卷 / 04期
关键词
Ahnak1-deficient mice; Recombinant ahnak1 C-terminus; Calcium current kinetics; Calcium channel beta2 subunit; CALCIUM-CHANNEL; BETA-SUBUNITS; SPLICE VARIANTS; PROTEIN; VOLTAGE; EXPRESSION; MEMBRANE; IDENTIFICATION; ALPHA(1C); DYSFERLIN;
D O I
10.1007/s00424-010-0853-x
中图分类号
Q4 [生理学];
学科分类号
071003 ;
摘要
Ahnak1, a giant 700 kDa protein, has been implicated in Ca2+ signalling in various cells. Previous work suggested that the interaction between ahnak1 and Cav beta(2) subunit plays a role in L-type Ca2+ current (I (CaL)) regulation. Here, we performed structure-function studies with the most C-terminal domain of ahnak1 (188 amino acids) containing a PxxP consensus motif (designated as 188-PSTP) using ventricular cardiomyocytes isolated from rats, wild-type (WT) mice and ahnak1-deficient mice. In vitro binding studies revealed that 188-PSTP conferred high-affinity binding to Cav beta(2) (K (d) similar to aEuro parts per thousand 60 nM). Replacement of proline residues by alanines (188-ASTA) decreased Cav beta(2) affinity about 20-fold. Both 188-PSTP and 188-ASTA were functional in ahnak1-expressing rat and mouse cardiomyocytes during whole-cell patch clamp. Upon intracellular application, they increased the net Ca2+ influx by enhancing I (CaL) density and/or increasing I (CaL) inactivation time course without altering voltage dependency. Specifically, 188-ASTA, which failed to affect I (CaL) density, markedly slowed I (CaL) inactivation resulting in a 50-70% increase in transported Ca2+ during a 0 mV depolarising pulse. Both ahnak1 fragments also slowed current inactivation with Ba2+ as charge carrier. By contrast, neither 188-PSTP nor 188-ASTA affected any I (CaL) characteristics in ahnak1-deficient mouse cardiomyocytes. Our results indicate that the presence of endogenous ahnak1 is required for tuning the voltage-dependent component of I (CaL) inactivation by ahnak1 fragments. We suggest that ahnak1 modulates the accessibility of molecular determinants in Cav beta(2) and/or scaffolds selectively different beta-subunit isoforms in the heart.
引用
收藏
页码:719 / 730
页数:12
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