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果蝇温度敏感突变体shibirets1培养神经元中内吞作用的可逆抑制

Reversible inhibition of endocytosis in cultured neurons from the Drosophila temperature-sensitive mutant shibirets1.

作者信息

Masur S K, Kim Y T, Wu C F

机构信息

Department of Biology, University of Iowa, Iowa City 52242.

出版信息

J Neurogenet. 1990 Apr;6(3):191-206. doi: 10.3109/01677069009107110.

DOI:10.3109/01677069009107110
PMID:2113575
Abstract

The Drosophila mutant, shibirets1 (shits1), is paralyzed at restrictive temperatures (greater than 29 degrees C) by a reversible block in synaptic transmission. Heat pulses deplete synaptic vesicles in nerve terminals and inhibit endocytic internalization of plasma membrane in garland cells and oocytes. In dissociated cultures of larval central nervous system (CNS), a temperature-sensitive defect is also expressed in shits1 neurons: at 30 degrees C, growth cone formation is retarded and neurite outgrowth is arrested. We now report that we have examined constitutive endocytosis in Drosophila CNS culture and have demonstrated directly an endocytic defect in shits1 neurons. At the permissive temperature, 20-22 degrees C, both shits1 and wild-type neurons actively endocytosed fluorescein-labelled dextran (40 KD, 5%) or horseradish peroxidase (HRP, 1%). Within 5 min, HRP was seen in vesicles, cup-shaped bodies, tubules and multivesicular bodies in neurites and cell bodies. In contrast, endocytosis was inhibited in cultures derived from the temperature-sensitive paralytic shits1 by a 15 min heat pulse (30 degrees C). Even after 30 min of HRP exposure at 30 degrees C, HRP-containing membranes were absent from almost all shits1 neurites; a minority of cell bodies had a few HRP-containing vesicles. The temperature-dependent block in endocytosis was readily reversed at 20 degrees C. Interestingly, the block was overcome by high concentration of external cations: shits1 neurons in culture actively took up HRP in numerous vesicles at 30 degrees C if 18 mM Ca2+ or Mg2+ was added to the medium. Our results support the notion that membrane recycling plays a critical role in regulating neurite outgrowth. This study also provides baseline information for further mutational analysis of the mechanism underlying the membrane cycling process in cultured neurons.

摘要

果蝇突变体“shibirets1”(shits1)在限制温度(高于29摄氏度)下会因突触传递的可逆阻断而瘫痪。热脉冲会耗尽神经末梢中的突触小泡,并抑制花环细胞和卵母细胞中质膜的内吞内化。在幼虫中枢神经系统(CNS)的解离培养物中,shits1神经元也表现出温度敏感缺陷:在30摄氏度时,生长锥形成受阻,神经突生长停滞。我们现在报告,我们已经研究了果蝇中枢神经系统培养物中的组成型内吞作用,并直接证明了shits1神经元存在内吞缺陷。在允许温度20 - 22摄氏度下,shits1和野生型神经元都能主动内吞荧光素标记的葡聚糖(40KD,5%)或辣根过氧化物酶(HRP,1%)。5分钟内,在神经突和细胞体的小泡、杯状小体、小管和多囊泡体中可见HRP。相比之下,15分钟的热脉冲(30摄氏度)会抑制来自温度敏感型瘫痪shits1的培养物中的内吞作用。即使在30摄氏度下暴露HRP 30分钟后,几乎所有shits1神经突中都没有含HRP的膜;少数细胞体有一些含HRP的小泡。内吞作用的温度依赖性阻断在温度恢复到20摄氏度时很容易逆转。有趣的是,高浓度的外部阳离子可以克服这种阻断:如果向培养基中添加18 mM的Ca2+或Mg2+,培养的shits1神经元在30摄氏度时会在许多小泡中主动摄取HRP。我们的结果支持膜循环在调节神经突生长中起关键作用这一观点。这项研究还为进一步对培养神经元中膜循环过程的潜在机制进行突变分析提供了基线信息。

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