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施万细胞在神经肌肉接头处表达Nav1.6钠通道:在运动终板疾病表型中的作用。

Expression of Nav1.6 sodium channels by Schwann cells at neuromuscular junctions: role in the motor endplate disease phenotype.

作者信息

Musarella Magali, Alcaraz Gisèle, Caillol Ghislaine, Boudier Jean-Louis, Couraud François, Autillo-Touati Amapola

机构信息

INSERM, UMR 641, IFR Jean Roche, Marseille, France; Université de la Méditerranée,Faculté de Médecine Nord, Marseille, Cedex, France.

出版信息

Glia. 2006 Jan 1;53(1):13-23. doi: 10.1002/glia.20252.

DOI:10.1002/glia.20252
PMID:16078241
Abstract

In addition to their role in action potential generation and fast synaptic transmission in neurons, voltage-dependent sodium channels can also be active in glia. Terminal Schwann cells (TSCs) wrap around the nerve terminal arborization at the neuromuscular junction, which they contribute to shape during development and in the postdenervation processes. Using fluorescent in situ hybridization (FISH), immunofluorescence, and confocal microscopy, we detected the neuronal Nav1.6 sodium channel transcripts and proteins in TSCs in normal adult rats and mice. Nav1.6 protein co-localized with the Schwann cell marker S-100 but was not detected in the SV2-positive nerve terminals. The med phenotype in mice is due to a mutation in the SCN8A gene resulting in loss of Nav1.6 expression. It leads to early onset in postnatal life of defects in neuromuscular transmission with minimal alteration of axonal conduction. Strikingly, in mutant mice, the nonmyelinated pre-terminal region of axons showed abundant sprouting at neuromuscular junctions, and most of the alpha-bungarotoxin-labeled endplates were devoid of S-100- or GFAP-positive TSCs. Using specific antibodies against the Nav1.2 and Nav1.6 sodium channels, ankyrin G and Caspr 1, and a pan sodium channel antibody, we found that a similar proportion of ankyrin G-positive nodes of Ranvier express sodium channels in mutant and wild-type animals and that nodal expression of Nav1.2 persists in med mice. Our data supports the hypothesis that the lack of expression of Nav1.6 in Schwann cells at neuromuscular junctions might play a role in the med phenotype.

摘要

除了在神经元动作电位产生和快速突触传递中发挥作用外,电压依赖性钠通道在神经胶质细胞中也具有活性。终末施万细胞(TSCs)包裹在神经肌肉接头处的神经末梢分支周围,在发育过程和去神经支配后的过程中,它们参与塑造神经末梢分支。通过荧光原位杂交(FISH)、免疫荧光和共聚焦显微镜技术,我们在正常成年大鼠和小鼠的TSCs中检测到了神经元Nav1.6钠通道转录本和蛋白。Nav1.6蛋白与施万细胞标志物S-100共定位,但在SV2阳性神经末梢中未检测到。小鼠的med表型是由于SCN8A基因突变导致Nav1.6表达缺失所致。它导致出生后早期神经肌肉传递缺陷,而轴突传导仅有轻微改变。引人注目的是,在突变小鼠中,轴突的无髓鞘终末前区域在神经肌肉接头处出现大量发芽,并且大多数α-银环蛇毒素标记的终板缺乏S-100或GFAP阳性的TSCs。使用针对Nav1.2和Nav1.6钠通道、锚蛋白G和Caspr 1的特异性抗体以及一种泛钠通道抗体,我们发现,在突变和野生型动物中,Ranvier结中锚蛋白G阳性的结表达钠通道的比例相似,并且Nav1.2在med小鼠的结处持续表达。我们的数据支持这样一种假说,即神经肌肉接头处施万细胞中Nav1.6表达的缺失可能在med表型中起作用。

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