豚鼠冠状动脉肌细胞中,峰值钙电流(ICa)作为肌浆网钙释放触发因素的功效。
Efficacy of peak Ca2+ currents (ICa) as trigger of sarcoplasmic reticulum Ca2+ release in myocytes from the guinea-pig coronary artery.
作者信息
Isenberg G
机构信息
Department of Physiology, University of Cologne, Köln, Germany.
出版信息
J Physiol. 1995 Apr 15;484 ( Pt 2)(Pt 2):287-306. doi: 10.1113/jphysiol.1995.sp020665.
Abstract
- Increments in cytosolic Ca2+ concentration (delta[Ca2+]c) were measured in single smooth muscle cells from guinea-pig coronary artery together with the density of peak Ca2+ currents (ICa) in response to clamp steps from -50 to 0 mV. The comparison of depolarization- with caffeine-induced delta[Ca2+]c was used to define the efficacy by which ICa can trigger Ca2+ release from the sarcoplasmic reticulum (SR). 2. At 2.5 mM extracellular calcium concentration ([Ca2+]o), depolarization induced a rapid rise of delta[Ca2+]c followed by a slow creep. Peak [Ca2+]c occurred within ca 30 s and could be followed by an undershoot and a second rise in [Ca2+]c. The creep was blocked by ryanodine but was insensitive to block of InsP3 receptors with heparin. The creep was not observed in Cs(+)-filled cells. After disappearance of the creep, a tonic delta[Ca2+]c became unmasked. 3. At 2.5 mM [Ca2+]o, peak ICa was -0.80 +/- 0.17 microA cm-2. delta[Ca2+] peaked at the end of the 6 s pulse at 202 +/- 98 nM while caffeine-induced delta[Ca2+]c peaked at 1330 +/- 410 nM. The ratio of depolarization- to caffeine-induced delta[Ca2+]c was 10 +/- 6%. 4. In media containing 10 mM [Ca2+]o plus 1 microM Bay K 8644, peak ICa was -2.6 +/- 1.1 microA cm-2 and delta[Ca2+]c peaked within 2.5 s at 451 +/- 194 nM. Paired measurements yielded the ratio of depolarization- to caffeine induced delta[Ca2+]c as 30 +/- 10%. Depolarization-induced delta[Ca2+]c was nearly blocked by caffeine and reduced by ryanodine to 30%, suggesting the contribution of Ca2+ release from caffeine- and ryanodine-sensitive Ca2+ stores. 5. Trypsin (1 mg ml-1) in the electrode solution (10 mM [Ca2+]o plus 1 microM Bay K 8644) increased peak ICa up to 12.5 microA cm-2. ICa induced a delta[Ca2+]c of 990 +/- 210 nM and was accompanied by a 'hump' of IK,Ca. When applied briefly after peak delta[Ca2+]c, caffeine increased [Ca2+]c only moderately. The results suggest that a peak ICa can trigger a synchronized whole-cell Ca2+ release only if ICa is strongly augmented. 6. Amplitude and rate of rise of delta[Ca2+]c were graded by test step potentials along a bell-shaped voltage-dependent curve, similar to that of L-type ICa. Steps to +80 mV induced no delta[Ca2+]c when the electrode solution contained 10 mM Na+. However, with 150 mM intrapipette Na+, pulses to +80 mV induced delta[Ca2+]c.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
- 在豚鼠冠状动脉的单个平滑肌细胞中测量胞质Ca2+浓度的增量(δ[Ca2+]c),并同时测量响应于从-50 mV至0 mV的钳制阶跃时的峰值Ca2+电流(ICa)密度。通过比较去极化诱导的与咖啡因诱导的δ[Ca2+]c来确定ICa触发肌浆网(SR)释放Ca2+的效能。2. 在细胞外钙浓度([Ca2+]o)为2.5 mM时,去极化诱导δ[Ca2+]c迅速升高,随后缓慢上升。峰值[Ca2+]c在约30 s内出现,随后可能出现超射和[Ca2+]c的第二次升高。这种缓慢上升被兰尼碱阻断,但对用肝素阻断InsP3受体不敏感。在充满Cs(+)的细胞中未观察到这种缓慢上升。在缓慢上升消失后,持续性的δ[Ca2+]c变得明显。3. 在[Ca2+]o为2.5 mM时,峰值ICa为-0.80±0.17 μA/cm2。δ[Ca2+]在6 s脉冲结束时达到峰值,为202±98 nM,而咖啡因诱导的δ[Ca2+]c峰值为1330±410 nM。去极化诱导的与咖啡因诱导的δ[Ca2+]c的比值为10±6%。4. 在含有10 mM [Ca2+]o加1 μM Bay K 8644的培养基中,峰值ICa为-2.6±1.1 μA/cm2,δ[Ca2+]c在2.5 s内达到峰值,为451±194 nM。配对测量得出去极化诱导的与咖啡因诱导的δ[Ca2+]c的比值为30±10%。去极化诱导的δ[Ca2+]c几乎被咖啡因阻断,被兰尼碱降低至30%,表明来自对咖啡因和兰尼碱敏感的Ca2+储存库的Ca2+释放的贡献。5. 在电极溶液(10 mM [Ca2+]o加1 μM Bay K 8644)中加入胰蛋白酶(1 mg/ml)使峰值ICa增加至12.5 μA/cm2。ICa诱导的δ[Ca2+]c为990±210 nM,并伴有IK,Ca的“驼峰”。在峰值δ[Ca2+]c后短暂施加咖啡因时,[Ca2+]c仅适度增加。结果表明,只有当ICa强烈增强时,峰值ICa才能触发同步的全细胞Ca2+释放。6. δ[Ca2+]c的幅度和上升速率由测试阶跃电位沿着类似于L型ICa的钟形电压依赖性曲线分级。当电极溶液含有10 mM Na+时,向+80 mV的阶跃未诱导δ[Ca2+]c。然而,当移液管内含有150 mM Na+时,向+80 mV的脉冲诱导了δ[Ca2+]c。(摘要截断于400字)
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