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Enhancement of presynaptic calcium current by cysteine string protein

机译:半胱氨酸串蛋白增强突触前钙电流

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摘要

The isolated chick ciliary neuron calyx synapse preparation was used to test cysteine string protein (CSP) action on presynaptic N-type Ca2+ channels. Endogenous CSP was localized primarily to secretory vesicle clusters in the presynaptic nerve terminal. Introduction of recombinant CSP into the voltage clamped terminal resulted in a prominent increase in Ca2+ current amplitude. However, this increase could not be attributed to a change in Ca2+ channel kinetics, voltage dependence, prepulse inactivation, or G protein inhibition but was attributed to the recruitment of dormant channels. Secretory vesicle associated endogenous CSP may play an important role in enhancing Ca2+ channel activity at the transmitter release site.
机译:分离的鸡睫状神经元萼突触制剂用于测试半胱氨酸串蛋白(CSP)对突触前N型Ca 2 + 通道的作用。内源性CSP主要定位于突触前神经末梢的分泌性囊泡簇。将重组CSP引入电压钳位端子导致Ca 2 + 电流幅度显着增加。然而,这种增加不能归因于Ca 2 + 通道动力学的变化,电压依赖性,脉冲前失活或G蛋白抑制,而归因于休眠通道的募集。分泌小泡相关的内源性CSP可能在增强递质释放部位的Ca 2 + 通道活性中起重要作用。

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