Hotchkiss Brain Institute, Libin Cardiovascular Institute, Department of Physiology & Pharmacology, University of Calgary, Alberta, Canada.
J Physiol. 2010 Oct 15;588(Pt 20):3983-4005. doi: 10.1113/jphysiol.2010.193300. Epub 2010 Aug 24.
This study examined whether elevated intravascular pressure stimulates asynchronous Ca(2+) waves in cerebral arterial smooth muscle cells and if their generation contributes to myogenic tone development. The endothelium was removed from rat cerebral arteries, which were then mounted in an arteriograph, pressurized (20-100 mmHg) and examined under a variety of experimental conditions. Diameter and membrane potential (V(M)) were monitored using conventional techniques; Ca(2+) wave generation and myosin light chain (MLC(20))/MYPT1 (myosin phosphatase targeting subunit) phosphorylation were assessed by confocal microscopy and Western blot analysis, respectively. Elevating intravascular pressure increased the proportion of smooth muscle cells firing asynchronous Ca(2+) waves as well as event frequency. Ca(2+) wave augmentation occurred primarily at lower intravascular pressures (<60 mmHg) and ryanodine, a plant alkaloid that depletes the sarcoplasmic reticulum (SR) of Ca(2+), eliminated these events. Ca(2+) wave generation was voltage insensitive as Ca(2+) channel blockade and perturbations in extracellular [K(+)] had little effect on measured parameters. Ryanodine-induced inhibition of Ca(2+) waves attenuated myogenic tone and MLC(20) phosphorylation without altering arterial V(M). Thapsigargin, an SR Ca(2+)-ATPase inhibitor also attenuated Ca(2+) waves, pressure-induced constriction and MLC(20) phosphorylation. The SR-driven component of the myogenic response was proportionally greater at lower intravascular pressures and subsequent MYPT1 phosphorylation measures revealed that SR Ca(2+) waves facilitated pressure-induced MLC(20) phosphorylation through mechanisms that include myosin light chain phosphatase inhibition. Cumulatively, our findings show that mechanical stimuli augment Ca(2+) wave generation in arterial smooth muscle and that these transient events facilitate tone development particularly at lower intravascular pressures by providing a proportion of the Ca(2+) required to directly control MLC(20) phosphorylation.
本研究旨在探讨血管内压升高是否会刺激脑血管平滑肌细胞产生非同步 Ca(2+)波,以及其产生是否有助于肌源性张力的发展。从大鼠脑中去除血管内皮细胞,然后将其安装在血管描记器中,在各种实验条件下加压(20-100mmHg)并进行检查。使用传统技术监测直径和膜电位(V(M));通过共聚焦显微镜和 Western blot 分析分别评估 Ca(2+)波的产生和肌球蛋白轻链(MLC(20))/肌球蛋白磷酸酶靶向亚基(MYPT1)磷酸化。升高血管内压会增加平滑肌细胞发射非同步 Ca(2+)波的比例和事件频率。Ca(2+)波增强主要发生在较低的血管内压(<60mmHg)下,而植物生物碱ryanodine 会耗尽肌浆网(SR)中的 Ca(2+),从而消除这些事件。Ca(2+)波的产生与电压无关,因为 Ca(2+)通道阻断和细胞外 [K(+)] 的改变对测量参数几乎没有影响。Ryanodine 诱导的 Ca(2+)波抑制减弱了肌源性张力和 MLC(20)磷酸化,而不改变动脉 V(M)。SR Ca(2+)-ATP 酶抑制剂 thapsigargin 也减弱了 Ca(2+)波、压力诱导的收缩和 MLC(20)磷酸化。在较低的血管内压下,SR 驱动的肌源性反应成分比例更大,随后的 MYPT1 磷酸化测量表明,SR Ca(2+)波通过抑制肌球蛋白轻链磷酸酶等机制促进压力诱导的 MLC(20)磷酸化。总的来说,我们的研究结果表明,机械刺激会增加动脉平滑肌中 Ca(2+)波的产生,这些瞬态事件通过提供直接控制 MLC(20)磷酸化所需的 Ca(2+)的一部分,有助于在较低的血管内压下发展张力。
