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膜电位和血管内压力对大鼠脑动脉直径和壁内[Ca2+]的调节作用

Regulation of arterial diameter and wall [Ca2+] in cerebral arteries of rat by membrane potential and intravascular pressure.

作者信息

Knot H J, Nelson M T

机构信息

Department of Pharmacology, Given Building, The University of Vermont, Burlington, VT 05405, USA.

出版信息

J Physiol. 1998 Apr 1;508 ( Pt 1)(Pt 1):199-209. doi: 10.1111/j.1469-7793.1998.199br.x.

Abstract
  1. The regulation of intracellular [Ca2+] in the smooth muscle cells in the wall of small pressurized cerebral arteries (100-200 micron) of rat was studied using simultaneous digital fluorescence video imaging of arterial diameter and wall [Ca2+], combined with microelectrode measurements of arterial membrane potential. 2. Elevation of intravascular pressure (from 10 to 100 mmHg) caused a membrane depolarization from -63 +/- 1 to -36 +/- 2 mV, increased arterial wall [Ca2+] from 119 +/- 10 to 245 +/- 9 nM, and constricted the arteries from 208 +/- 10 micron (fully dilated, Ca2+ free) to 116 +/- 7 micron or by 45 % ('myogenic tone'). 3. Pressure-induced increases in arterial wall [Ca2+] and vasoconstriction were blocked by inhibitors of voltage-dependent Ca2+ channels (diltiazem and nisoldipine) or to the same extent by removal of external Ca2+. 4. At a steady pressure (i.e. under isobaric conditions at 60 mmHg), the membrane potential was stable at -45 +/- 1 mV, intracellular [Ca2+] was 190 +/- 10 nM, and arteries were constricted by 41 % (to 115 +/- 7 micron from 196 +/- 8 micron fully dilated). Under this condition of -45 +/- 5 mV at 60 mmHg, the voltage sensitivity of wall [Ca2+] and diameter were 7.5 nM mV-1 and 7.5 micron mV-1, respectively, resulting in a Ca2+ sensitivity of diameter of 1 mum nM-1. 5. Membrane potential depolarization from -58 to -23 mV caused pressurized arteries (to 60 mmHg) to constrict over their entire working range, i.e. from maximally dilated to constricted. This depolarization was associated with an elevation of arterial wall [Ca2+] from 124 +/- 7 to 347 +/- 12 nM. These increases in arterial wall [Ca2+] and vasoconstriction were blocked by L-type voltage-dependent Ca2+ channel inhibitors. 6. The relationship between arterial wall [Ca2+] and membrane potential was not significantly different under isobaric (60 mmHg) and non-isobaric conditions (10-100 mmHg), suggesting that intravascular pressure regulates arterial wall [Ca2+] through changes in membrane potential. 7. The results are consistent with the idea that intravascular pressure causes membrane potential depolarization, which opens voltage-dependent Ca2+ channels, acting as 'voltage sensors', thus increasing Ca2+ entry and arterial wall [Ca2+], which leads to vasoconstriction.
摘要
  1. 采用同步数字荧光视频成像技术,对大鼠小的加压脑动脉(100 - 200微米)壁平滑肌细胞内[Ca2+]进行调节研究,同时测量动脉直径和壁内[Ca2+],并结合微电极测量动脉膜电位。2. 血管内压力升高(从10至100 mmHg)导致膜去极化,从 - 63±1 mV变为 - 36±2 mV,动脉壁[Ca2+]从119±10 nM增加至245±9 nM,动脉从208±10微米(完全舒张,无Ca2+)收缩至116±7微米,收缩45%(“肌源性张力”)。3. 压力诱导的动脉壁[Ca2+]增加和血管收缩被电压依赖性Ca2+通道抑制剂(地尔硫卓和尼索地平)阻断,或在同等程度上被去除细胞外Ca2+所阻断。4. 在稳定压力下(即60 mmHg等压条件下),膜电位稳定在 - 45±1 mV,细胞内[Ca2+]为190±10 nM,动脉收缩41%(从完全舒张的196±8微米收缩至115±7微米)。在60 mmHg时 - 45±5 mV的这种条件下,壁内[Ca2+]和直径的电压敏感性分别为7.5 nM mV-1和7.5微米mV-1,导致直径的Ca2+敏感性为1微米 nM-1。5. 膜电位从 - 58 mV去极化至 - 23 mV导致加压动脉(至60 mmHg)在其整个工作范围内收缩,即从最大舒张至收缩。这种去极化与动脉壁[Ca2+]从124±7 nM升高至347±12 nM相关。这些动脉壁[Ca2+]的增加和血管收缩被L型电压依赖性Ca2+通道抑制剂阻断。6. 在等压(60 mmHg)和非等压条件(10 - 100 mmHg)下,动脉壁[Ca2+]与膜电位之间的关系无显著差异,表明血管内压力通过膜电位变化调节动脉壁[Ca2+]。7. 结果与以下观点一致,即血管内压力导致膜电位去极化,从而打开作为“电压传感器”的电压依赖性Ca2+通道,增加Ca2+内流和动脉壁[Ca2+],进而导致血管收缩。

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