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2
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Chronic exercise normalizes changes in Cav 1.2 and KCa 1.1 channels in mesenteric arteries from spontaneously hypertensive rats.长期运动可使自发性高血压大鼠肠系膜动脉中Cav 1.2和KCa 1.1通道的变化恢复正常。
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Stiff substrates enhance cultured neuronal network activity.坚硬的底物可增强培养的神经网络活动。
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Spherical indentation method for determining the constitutive parameters of hyperelastic soft materials.球形压痕法测定超弹性软材料的本构参数。
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Myofibroblast-mediated mechanisms of pathological remodelling of the heart.肌成纤维细胞介导的心脏病理性重塑机制。
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Substrate stiffness modulates gene expression and phenotype in neonatal cardiomyocytes in vitro.基质硬度可调节体外原代培养新生大鼠心肌细胞的基因表达和表型。
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Effects of familial hemiplegic migraine type 1 mutation T666M on voltage-gated calcium channel activities in trigeminal ganglion neurons.家族性偏瘫性偏头痛 1 型突变 T666M 对三叉神经节神经元电压门控钙通道活性的影响。
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BK通道在底物硬度对心室肌细胞钙通道调节中的作用。

A Role of BK Channel in Regulation of Ca Channel in Ventricular Myocytes by Substrate Stiffness.

作者信息

Zhao Hucheng, Yu Yang, Wu Xiaoan, Liu Sisi, Liu Bailin, Du Jing, Li Bo, Jiang Linhua, Feng Xiqiao

机构信息

Institute of Biomechanics and Medical Engineering, Department of Engineering Mechanics, Tsinghua University, Beijing, China.

Institute of Biomechanics and Medical Engineering, Department of Engineering Mechanics, Tsinghua University, Beijing, China.

出版信息

Biophys J. 2017 Apr 11;112(7):1406-1416. doi: 10.1016/j.bpj.2017.01.036.

DOI:10.1016/j.bpj.2017.01.036
PMID:28402883
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5389963/
Abstract

Substrate stiffness is crucial for diverse cell functions, but the mechanisms conferring cells with mechanosensitivity are still elusive. By tailoring substrate stiffness with 10-fold difference, we showed that L-type voltage-gated Ca channel current density was greater in chick ventricular myocytes cultured on the stiff substrate than on the soft substrate. Blockage of the BK channel increased the Ca current density on the soft substrate and consequently eliminated substrate stiffness regulation of the Ca channel. The expression of the BK channel, including the STREX-containing α-subunit that forms stretch-activated BK channel in myocytes and the BK channel function in myocytes (and also in HEK293 cells heterologously expressing STREX-containing α- and β-subunits) was reduced in cells cultured on the stiff substrate. Furthermore, in HEK293 cells coexpressing the cardiac Ca1.2 channel and STREX-containing BK channel, the Ca current density was greater in cells on the stiff substrate, which was not observed in cells expressing the Ca1.2 channel alone or coexpressing with the STREX-deleted BK channel. These results provide strong evidence to show that the stretch-activated BK channel plays a key role in functional regulation of cardiac voltage-gated Ca channel by substrate stiffness, revealing, to our knowledge, a novel mechanosensing mechanism in ventricular myocytes.

摘要

底物硬度对多种细胞功能至关重要,但赋予细胞机械敏感性的机制仍不清楚。通过制备具有10倍差异的底物硬度,我们发现,在硬底物上培养的鸡心室肌细胞中,L型电压门控钙通道电流密度比在软底物上培养的细胞更大。阻断BK通道可增加软底物上的钙电流密度,从而消除底物硬度对钙通道的调节作用。在硬底物上培养的细胞中,BK通道的表达降低,包括在心肌细胞中形成拉伸激活BK通道的含STREX的α亚基以及心肌细胞(以及在异源表达含STREX的α和β亚基的HEK293细胞中)的BK通道功能。此外,在共表达心脏Ca1.2通道和含STREX的BK通道的HEK293细胞中,硬底物上的细胞钙电流密度更大,而在单独表达Ca1.2通道或与缺失STREX的BK通道共表达的细胞中未观察到这种现象。这些结果提供了有力证据,表明拉伸激活的BK通道在底物硬度对心脏电压门控钙通道的功能调节中起关键作用,据我们所知,这揭示了心室肌细胞中一种新的机械传感机制。