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环磷酸腺苷(cAMP)对大鼠嗜铬细胞L型电流和分泌的独特增强作用。

Distinct potentiation of L-type currents and secretion by cAMP in rat chromaffin cells.

作者信息

Carabelli V, Giancippoli A, Baldelli P, Carbone E, Artalejo A R

机构信息

Dipartimento di Neuroscienze, Unità di Ricerca, Instituto Nazionale Fisica della Materia, 10125 Turin, Italy.

出版信息

Biophys J. 2003 Aug;85(2):1326-37. doi: 10.1016/S0006-3495(03)74567-6.

Abstract

We have investigated the potentiating action of cAMP on L-currents of rat chromaffin cells and the corresponding increase of Ca(2+)-evoked secretory responses with the aim of separating the action of cAMP on Ca(2+) entry through L-channels and the downstream effects of cAMP/protein kinase A (PKA) on exocytosis. In omega-toxin-treated rat chromaffin cells, exposure to the permeable cAMP analog 8-(4-chlorophenylthio)-adenosine 3',5'-monophosphate (pCPT-cAMP; 1 mM, 30 min) caused a moderate increase of Ca(2+) charge carried through L-channels (19% in 10 mM Ca(2+) at +10 mV) and a drastic potentiation of secretion ( approximately 100%), measured as membrane capacitance increments (deltaC). The apparent Ca(2+) dependency of exocytosis increased with pCPT-cAMP and was accompanied by 83% enhancement of the readily releasable pool of vesicles with no significant change of the probability of release, as evaluated with paired-pulse stimulation protocols. pCPT-cAMP effects could be mimicked by stimulation of beta(1)-adrenoreceptors and reversed by the PKA inhibitor H89, suggesting strict PKA dependence. For short pulses to +10 mV (100 ms), potentiation of exocytosis by pCPT-cAMP was proportional to the quantity of charge entering the cell and occurred independently of whether L, N, or P/Q channels were blocked, suggesting that cAMP acts as a constant amplification factor for secretion regardless of the channel type carrying Ca(2+). Analysis of statistical variations among depolarization-induced capacitance increments indicates that pCPT-cAMP acts downstream of Ca(2+) entry by almost doubling the mean size of unitary exocytic events, most likely as a consequence of an increased granule-to-granule rather than a granule-to-membrane fusion.

摘要

我们研究了环磷酸腺苷(cAMP)对大鼠嗜铬细胞L电流的增强作用以及相应的钙(Ca²⁺)诱发分泌反应的增加,目的是区分cAMP对通过L通道的Ca²⁺内流的作用以及cAMP/蛋白激酶A(PKA)对胞吐作用的下游效应。在经ω-芋螺毒素处理的大鼠嗜铬细胞中,暴露于可渗透的cAMP类似物8-(4-氯苯硫基)-腺苷3',5'-单磷酸(pCPT-cAMP;1 mM,30分钟)会导致通过L通道携带的Ca²⁺电荷量适度增加(在+10 mV的10 mM Ca²⁺中增加19%),并使分泌显著增强(约100%),以膜电容增加量(ΔC)来衡量。胞吐作用的表观Ca²⁺依赖性随pCPT-cAMP增加,并且伴随着易释放囊泡池增加83%,而释放概率无显著变化,这是通过双脉冲刺激方案评估得出的。pCPT-cAMP的作用可被β₁-肾上腺素能受体刺激模拟,并被PKA抑制剂H89逆转,表明严格依赖PKA。对于短脉冲至+10 mV(100毫秒),pCPT-cAMP对胞吐作用的增强与进入细胞的电荷量成正比,并且无论L、N或P/Q通道是否被阻断都会发生,这表明cAMP作为分泌的恒定放大因子,与携带Ca²⁺的通道类型无关。对去极化诱导的电容增加量之间的统计变化分析表明,pCPT-cAMP在Ca²⁺内流下游起作用,几乎使单个胞吐事件的平均大小增加一倍,最可能的原因是颗粒间融合增加而非颗粒与膜的融合。

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