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培养的大鼠交感神经元中125I-神经生长因子细胞内命运的超微结构研究

Ultrastructural studies on the intracellular fate of 125I-nerve growth factor in cultured rat sympathetic neurons.

作者信息

Claude P, Hawrot E, Parada I

出版信息

J Cell Biochem. 1982;20(1):1-13. doi: 10.1002/jcb.240200102.

DOI:10.1002/jcb.240200102
PMID:6761346
Abstract

Primary cell cultures of sympathetic neurons from rat were exposed to 125I-nerve growth factor (NGF) and the fate of the NGF in the cell was followed using electron microscopic autoradiography. The intracellular localization of NGF was determined in the cell bodies and in the proximal neurites of neurons that had been grown in three-chamber dishes, following 5 or 24 hr of retrograde transport of NGF from the distal portions of the neurites. Label in the proximal neurites was predominantly associated with lysosomes and multivesicular bodies (MVBs), and at 5 hr elongated tubular elements were especially heavily labeled. Most of the label in the cell bodies was concentrated in lysosomes and MVBs. Lysosomes accounted for the largest fraction (45-60%) of the grains in the cell body, with a labeling density (LD = % grains/% area) of 3-5, while MVBs accounted for 5-10% of the grains with an LD of 5-20. We observed no evidence of nuclear labeling after 5 or 24 hr of retrograde transport. Mass cultures of neurons were incubated for 22 hr with NGF in the presence of the lysosomal inhibitors chloroquine (CQ, 0.05 mM) or methylamine (MA, 10 mM). In both agents the lysosomes were swollen with membranous material but still sequestered NGF, especially in CQ where the lysosomes were associated with almost 65% of the grains and had an LD of 6. CQ and MA had different effects on the morphology of the MVBs: in CQ they were few in number and compact while in MA they were numerous and appeared swollen and vacuolated. We observed no evidence for the nuclear accumulation of NGF even in the presence of the lysosomotropic agents.

摘要

将大鼠交感神经元的原代细胞培养物暴露于125I - 神经生长因子(NGF),并使用电子显微镜放射自显影术追踪细胞中NGF的命运。在NGF从神经突远端逆行运输5或24小时后,在三室培养皿中生长的神经元的细胞体和近端神经突中确定NGF的细胞内定位。近端神经突中的标记主要与溶酶体和多囊泡体(MVBs)相关,在5小时时,细长的管状结构尤其被大量标记。细胞体中的大多数标记集中在溶酶体和MVBs中。溶酶体占细胞体中颗粒的最大比例(45 - 60%),标记密度(LD = 颗粒%/面积%)为3 - 5,而MVBs占颗粒的5 - 10%,LD为5 - 20。在逆行运输5或24小时后,我们没有观察到核标记的证据。将神经元的大规模培养物在溶酶体抑制剂氯喹(CQ,0.05 mM)或甲胺(MA,10 mM)存在的情况下与NGF孵育22小时。在这两种试剂中,溶酶体都充满了膜状物质而肿胀,但仍能隔离NGF,尤其是在CQ中,溶酶体与几乎65%的颗粒相关,标记密度为6。CQ和MA对MVBs的形态有不同影响:在CQ中它们数量少且紧密,而在MA中它们数量多且显得肿胀和空泡化。即使在存在溶酶体促渗剂的情况下,我们也没有观察到NGF在核内积累的证据。

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