辣椒素受体(TRPA1)离子通道刺激通过钙调蛋白依赖性激酶 II(CaMKII)途径增强心肌细胞的收缩功能。
TRPA1 ion channel stimulation enhances cardiomyocyte contractile function via a CaMKII-dependent pathway.
机构信息
a Department of Medicine , Vanderbilt University Medical Center , Nashville , TN , USA.
b Department of Biological Sciences , Kent State University , Kent , OH , USA.
出版信息
Channels (Austin). 2017 Nov 2;11(6):587-603. doi: 10.1080/19336950.2017.1365206. Epub 2017 Aug 25.
RATIONALE
Transient receptor potential channels of the ankyrin subtype-1 (TRPA1) are non-selective cation channels that show high permeability to calcium. Previous studies from our laboratory have demonstrated that TRPA1 ion channels are expressed in adult mouse ventricular cardiomyocytes (CMs) and are localized at the z-disk, costamere and intercalated disk. The functional significance of TRPA1 ion channels in the modulation of CM contractile function have not been explored.
OBJECTIVE
To identify the extent to which TRPA1 ion channels are involved in modulating CM contractile function and elucidate the cellular mechanism of action.
METHODS AND RESULTS
Freshly isolated CMs were obtained from murine heart and loaded with Fura-2 AM. Simultaneous measurement of intracellular free Ca concentration ([Ca]) and contractility was performed in individual CMs paced at 0.3 Hz. Our findings demonstrate that TRPA1 stimulation with AITC results in a dose-dependent increase in peak [Ca] and a concomitant increase in CM fractional shortening. Further analysis revealed a dose-dependent acceleration in time to peak [Ca] and velocity of shortening as well as an acceleration in [Ca] decay and velocity of relengthening. These effects of TRPA1 stimulation were not observed in CMs pre-treated with the TRPA1 antagonist, HC-030031 (10 µmol/L) nor in CMs obtained from TRPA1 mice. Moreover, we observed no significant increase in cAMP levels or PKA activity in response to TRPA1 stimulation and the PKA inhibitor peptide (PKI 14-22; 100 nmol/L) failed to have any effect on the TRPA1-mediated increase in CM contractile function. However, TRPA1 stimulation resulted in a rapid phosphorylation of Ca/calmodulin-dependent kinase II (CaMKII) (1-5 min) that correlated with increases in CM [Ca] and contractile function. Finally, all aspects of TRPA1-dependent increases in CM [Ca], contractile function and CaMKII phosphorylation were virtually abolished by the CaMKII inhibitors, KN-93 (10 µmol/L) and autocamtide-2-related peptide (AIP; 20 µmol/L).
CONCLUSIONS
These novel findings demonstrate that stimulation of TRPA1 ion channels in CMs results in activation of a CaMKII-dependent signaling pathway resulting in modulation of intracellular Ca availability and handling leading to increases in CM contractile function. Cardiac TRPA1 ion channels may represent a novel therapeutic target for increasing the inotropic and lusitropic state of the heart.
原理
锚蛋白重复域跨膜蛋白 1(TRPA1)型瞬时受体电位通道是非选择性阳离子通道,对钙具有高通透性。我们实验室的先前研究表明,TRPA1 离子通道在成年小鼠心室心肌细胞(CMs)中表达,并定位于 Z 盘、连接蛋白和闰盘。TRPA1 离子通道在调节 CM 收缩功能方面的功能意义尚未得到探索。
目的
确定 TRPA1 离子通道在调节 CM 收缩功能中的参与程度,并阐明其作用的细胞机制。
方法和结果
从鼠心中分离出新鲜的 CMs,并加载 Fura-2 AM。在 0.3 Hz 的频率下对单个 CMs 进行细胞内游离 Ca 浓度 ([Ca]) 和收缩性的同步测量。我们的研究结果表明,AITC 刺激 TRPA1 会导致峰值 [Ca] 呈剂量依赖性增加,并伴有 CM 分数缩短的增加。进一步分析显示,TRPA1 刺激后,[Ca] 达峰时间和缩短速度呈剂量依赖性加速,[Ca] 衰减和再延长速度也呈剂量依赖性加速。在 TRPA1 拮抗剂 HC-030031(10 μmol/L)预处理的 CMs 或 TRPA1 敲除小鼠获得的 CMs 中未观察到 TRPA1 刺激的这些作用。此外,我们观察到对 TRPA1 刺激没有明显的 cAMP 水平或 PKA 活性增加,PKA 抑制剂肽(PKI 14-22;100 nmol/L)对 TRPA1 介导的 CM 收缩功能增加没有任何影响。然而,TRPA1 刺激导致钙/钙调蛋白依赖性激酶 II(CaMKII)的快速磷酸化(1-5 分钟),与 CM [Ca] 和收缩功能的增加相关。最后,CaMKII 抑制剂 KN-93(10 μmol/L)和自催化肽(AIP;20 μmol/L)几乎完全消除了 TRPA1 依赖性增加 CM [Ca]、收缩功能和 CaMKII 磷酸化的所有方面。
结论
这些新发现表明,CM 中 TRPA1 离子通道的刺激导致钙调蛋白激酶 II(CaMKII)依赖性信号通路的激活,从而调节细胞内 Ca 可用性和处理,导致 CM 收缩功能增加。心脏 TRPA1 离子通道可能成为增加心脏变力和舒张功能的新的治疗靶点。
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