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高钙离子存在下的快速轴突运输:微管并非必需的证据。

Fast axonal transport in the presence of high Ca2+: evidence that microtubules are not required.

作者信息

Brady S T, Crothers S D, Nosal C, McClure W O

出版信息

Proc Natl Acad Sci U S A. 1980 Oct;77(10):5909-13. doi: 10.1073/pnas.77.10.5909.

Abstract

Microtubules have long been associated with the mechanism of fast axoplasmic transport, although experimental evidence to support an involvement has been equivocal. Electron microscopic studies demonstrated that incubation of the axons of excised rat sciatic nerves in media containing 75 mM Ca2+ caused complete loss of microtubules within 6 hr. To evaluate the role of microtubules in fast anterograde transport, studies of transport in nerves exposed to these conditions were undertaken. Prior to measurement of axoplasmic transport, nerves ligated distal to the dorsal root ganglia were preincubated in vitro in 75 mM Ca2+ for 0-6 hr. Fast axonal transport was subsequently monitored by measuring the amount of trichloroacetic acid-insoluble radioactivity that accumulated at the ligature after incubation for 12-18 hr with L-[3H]proline. Nerves in which microtubules had been depolymerized by preincubation in high Ca2+ maintained control levels of transport. We conclude that intact microtubules are not required for fast anterograde axoplasmic transport.

摘要

长期以来,微管一直与快速轴质运输的机制相关联,尽管支持其参与该过程的实验证据并不明确。电子显微镜研究表明,将切除的大鼠坐骨神经轴突在含有75 mM Ca2+的培养基中孵育6小时内,微管会完全丧失。为了评估微管在快速顺向运输中的作用,对暴露于这些条件下的神经中的运输进行了研究。在测量轴质运输之前,将结扎于背根神经节远端的神经在体外于75 mM Ca2+中预孵育0 - 6小时。随后通过测量在与L-[3H]脯氨酸孵育12 - 18小时后在结扎处积累的三氯乙酸不溶性放射性物质的量来监测快速轴突运输。通过在高钙中预孵育而使微管解聚的神经维持了对照水平的运输。我们得出结论,快速顺向轴质运输并不需要完整的微管。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/de5c/350181/d4f20ac325d9/pnas00497-0371-a.jpg

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