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Stimulation-dependent regulation of the pH volume and quantal size of bovine and rodent secretory vesicles

机译:刺激性调节牛和啮齿动物分泌性囊泡的pH体积和定量大小

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摘要

Trapping of weak bases was utilized to evaluate stimulus-induced changes in the internal pH of the secretory vesicles of chromaffin cells and enteric neurons. The internal acidity of chromaffin vesicles was increased by the nicotinic agonist 1,1-dimethyl-4-phenyl-piperazinium iodide (DMPP; in vivo and in vitro) and by high K+ (in vitro); and in enteric nerve terminals by exposure to veratridine or a plasmalemmal [Ca2+ ]o receptor agonist (Gd3+). Stimulation-induced acidification of chromaffin vesicles was [Ca2+ ]o-dependent and blocked by agents that inhibit the vacuolar proton pump (vH+-ATPase) or flux through Cl channels. Stimulation also increased the average volume of chromaffin vesicles and the proportion that displayed a clear halo around their dense cores (called active vesicles). Stimulation-induced increases in internal acidity and size were greatest in active vesicles. Stimulation of chromaffin cells in the presence of a plasma membrane marker revealed that membrane was internalized in endosomes but not in chromaffin vesicles. The stable expression of botulinum toxin E to prevent exocytosis did not affect the stimulation-induced acidification of the secretory vesicles of mouse neuroblastoma Neuro2A cells. Stimulation-induced acidification thus occurs independently of exocytosis. The quantal size of secreted catecholamines, measured by amperometry in cultured chromaffin cells, was found to be increased either by prior exposure to L-DOPA or stimulation by high K+, and decreased by inhibition of vH+-ATPase or flux through Cl channels. These observations are consistent with the hypothesis that the content of releasable small molecules in secretory vesicles is increased when the driving force for their uptake is enhanced, either by increasing the transmembrane concentration or pH gradients.
机译:捕获弱碱被用来评估嗜铬细胞和肠神经元分泌小泡的内部pH的刺激诱导的变化。烟碱激动剂1,1-二甲基-4-苯基碘化哌嗪(DMPP;体内和体外)和高K + (体外)提高了嗜铬菌素囊泡的内部酸度。暴露于维他命啶或血浆中[Ca 2 + ] o受体激动剂(Gd 3 + ),在肠道神经末梢。刺激诱导的嗜铬细胞囊泡的酸化是[Ca 2 + ] o依赖性的,并被抑制液泡质子泵的药物(vH + -ATPase)或通过Cl的通量所阻断-通道。刺激还增加了嗜铬菌素囊泡的平均体积,并增加了在其密集核心(称为活性囊泡)周围显示出清晰光环的比例。刺激引起的内部酸度和大小的增加在活性囊泡中最大。在质膜标记物存在下对嗜铬细胞的刺激表明,该膜被内在体包裹,而不在嗜铬囊泡中被内化。肉毒杆菌毒素E的稳定表达,以防止胞吐作用,不影响小鼠神经母细胞瘤Neuro2A细胞分泌囊泡的刺激诱导酸化。因此,刺激诱导的酸化独立于胞吐作用而发生。通过安培法测定培养的嗜铬细胞中分泌的儿茶酚胺的定量大小,可以通过事先暴露于L-DOPA或通过高K + 刺激来增加,而通过抑制vH + -ATPase或通过Cl -通道的通量。这些观察结果与以下假设一致:当通过增加跨膜浓度或pH梯度来增强分泌小泡摄取的驱动力时,分泌小泡中可释放小分子的含量会增加。

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