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Regulation of the Ca2+ sensitivity of exocytosis by Rab3a.

机译:Rab3a对胞吐作用的Ca2 +敏感性的调节。

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摘要

Ca2+ ions trigger the release of hormones and neurotransmitters and contribute to making the secretory vesicles competent for fusion. Here, we present evidence for the involvement of the GTP-binding protein Rab3a in the sensitivity of the exocytotic process to internal [Ca2+]. The secretory activity of bovine adrenal chromaffin cells was elicited by Ca2+ dialysis through a patch-clamp pipette and assayed by monitoring changes in cell membrane capacitance. Microinjection of antisense oligonucleotides directed to rab3a mRNA increased the secretory activity observed at low (0.2-4 microM) [Ca2+], but did not change the maximal activity observed at 10 microM free [Ca2+]. Moreover, after a train of depolarizing stimuli, the secretory activity of antisense-injected cells dialyzed with 10 microM [Ca2+] was increased significantly compared with that of control cells. This result suggests that the activity of either Rab3a or its partners might change upon stimulation. We conclude that Rab3a, together with its partners, participates in the Ca2+ dependence of exocytosis and that its activity is modulated further in a stimulus-dependent manner. These findings should provide some clues to elucidate the role of Rab3a in synaptic plasticity.
机译:Ca2 +离子触发激素和神经递质的释放,并有助于使分泌性囊泡具有融合能力。在这里,我们为GTP结合蛋白Rab3a参与胞外过程对内部[Ca2 +]的敏感性提供了证据。通过膜片钳移液器通过Ca 2+透析引发牛肾上腺嗜铬细胞的分泌活性,并通过监测细胞膜电容的变化进行测定。显微注射针对rab3a mRNA的反义寡核苷酸可增加在低(0.2-4 microM)[Ca2 +]下观察到的分泌活性,但不会改变在10 microM游离[Ca2 +]下观察到的最大活性。此外,经过一连串的去极化刺激后,与对照细胞相比,用10 microM [Ca2 +]透析的反义注射细胞的分泌活性显着增加。该结果表明Rab3a或其伴侣的活性可能在刺激后改变。我们得出的结论是,Rab3a及其合作伙伴一起参与了胞吐作用的Ca2 +依赖性,并且其活性以刺激依赖性的方式进一步受到调节。这些发现应提供一些线索,阐明Rab3a在突触可塑性中的作用。

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