神经激肽A和钙离子电流可诱导豚鼠气管肌细胞中钙激活氯离子电流。

Neurokinin A and Ca2+ current induce Ca(2+)-activated Cl(-) currents in guinea-pig tracheal myocytes.

作者信息

Hazama H, Nakajima T, Hamada E, Omata M, Kurachi Y

机构信息

The Second Department of Internal Medicine, Faculty of Medicine, University of Tokyo, Tokyo, Japan.

出版信息

J Physiol. 1996 Apr 15;492 ( Pt 2)(Pt 2):377-93. doi: 10.1113/jphysiol.1996.sp021315.

DOI:10.1113/jphysiol.1996.sp021315

PMID:9019536

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1158834/

Abstract

Membrane currents were recorded by a patch clamp technique in guinea-pig tracheal myocytes, using the whole cell mode with Cs(+) internal solution. 2. Both neurokinin A (NKA, 1 mu M) and caffeine (10 mM) evoked Ca(2+)-activated Cl- currents (I[Cl(Ca)]) transiently. In Ca(2+)-free bathing solution, the first application of NKA or caffeine elicited I[Cl(Ca)] but the second application of these substances failed to activate it. In addition, pretreatment with ryanodine in the presence of caffeine abolished the response to both NKA and caffeine whilst heparin (200 mu g ml(-1)) only blocked the NKA-induced response. I[Cl(Ca)] was also elicited by inositol 1,4,5-trisphosphate (IP(3)). 3. Command voltage pulses positive to 0 mV from a holding potential of -60 mV activated the voltage-dependent L-type Ca2+ current (I(Ca,L)) and late outward current. Upon repolarization to the holding potential, slowly decaying inward tail currents were recorded. The outward current during the depolarizing pulses and the inward tail current were enhanced by Bay K 8644, but completely blocked by Cd2+ or nifedipine. Replacement of external Ca2+ with Ba2+, removal of Ca2+ from the bath solution, or inclusion of EGTA (5 mM) in the patch pipette, also led to abolition of these currents, indicating that they were Ca2+ dependent, and that Ca2+ influx due to I(Ca,L) activated the currents. 4. When Cl(-) or Cl(-) was changed, the reversal potential (E(rev)) of the Ca2+-activated currents shifted, thus behaving like a Cl(-)-selective ion channel as predicted by the Nernst equation. DIDS (1 mM) completely abolished the currents, also suggesting that they were I[Cl(Ca)]. 5. NKA (1 mu M) and caffeine (30 mM) transiently activated I[Cl(Ca)], and after that both agents markedly reduced I[Cl(Ca)] induced by I(Ca,L). This is probably due to sarcoplasmic reticulum (SR) Ca2+ release induced by NKA or caffeine, followed by inhibition of the Ca(2+)-induced Ca2+ release from the SR. 6. The present results indicate that I[Cl(Ca)] can be activated by SR Ca2+ release due to NKA or caffeine (through IP(3) or ryanodine receptors) as well as by Ca2+ influx due to I(Ca,L). It also suggests that activation of I[Cl(Ca)] by NKA may be mediated by the production of IP(3), which releases Ca2+ from the SR.

摘要

采用膜片钳技术，在豚鼠气管肌细胞中记录膜电流，使用含Cs(+)内液的全细胞模式。2. 神经激肽A（NKA，1 μM）和咖啡因（10 mM）均可短暂诱发Ca(2+)激活的Cl-电流（I[Cl(Ca)]）。在无Ca(2+)的浴液中，首次施加NKA或咖啡因可诱发I[Cl(Ca)]，但再次施加这些物质则无法激活该电流。此外，在咖啡因存在的情况下用ryanodine预处理可消除对NKA和咖啡因的反应，而肝素（200 μg/ml）仅阻断NKA诱导的反应。肌醇1,4,5-三磷酸（IP(3)）也可诱发I[Cl(Ca)]。3. 从 -60 mV的 holding 电位向0 mV以上的指令电压脉冲可激活电压依赖性L型Ca2+电流（I(Ca,L)）和延迟外向电流。复极化至holding电位时，可记录到缓慢衰减的内向尾电流。去极化脉冲期间的外向电流和内向尾电流可被Bay K 8644增强，但被Cd2+或硝苯地平完全阻断。用Ba2+替代细胞外Ca2+、从浴液中去除Ca2+或在膜片钳吸管中加入EGTA（5 mM），也会导致这些电流消失，表明它们依赖Ca2+，且由于I(Ca,L)引起的Ca2+内流激活了这些电流。4. 当改变Cl(-)或Cl(-)时，Ca2+激活电流的反转电位（E(rev)）发生偏移，因此表现得像Nernst方程预测的Cl(-)选择性离子通道。DIDS（1 mM）可完全消除这些电流，也表明它们是I[Cl(Ca)]。5. NKA（1 μM）和咖啡因（30 mM）可短暂激活I[Cl(Ca)]，之后两种试剂均显著降低由I(Ca,L)诱导的I[Cl(Ca)]。这可能是由于NKA或咖啡因诱导的肌浆网（SR）Ca2+释放，随后抑制了SR中Ca(2+)诱导的Ca2+释放。6. 目前的结果表明，I[Cl(Ca)]可被NKA或咖啡因（通过IP(3)或ryanodine受体）引起的SR Ca2+释放以及I(Ca,L)引起的Ca2+内流激活。这也表明NKA对I[Cl(Ca)]的激活可能由IP(3)的产生介导，IP(3)从SR释放Ca2+。