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发育中和成年小鼠坐骨神经中主要的外周神经系统糖蛋白P0以及L2/HNK-1和L3碳水化合物结构的免疫细胞定位。

Immunocytological localization of the major peripheral nervous system glycoprotein P0 and the L2/HNK-1 and L3 carbohydrate structures in developing and adult mouse sciatic nerve.

作者信息

Martini R, Bollensen E, Schachner M

机构信息

Department of Neurobiology, University of Heidelberg, Federal Republic of Germany.

出版信息

Dev Biol. 1988 Oct;129(2):330-8. doi: 10.1016/0012-1606(88)90380-6.

DOI:10.1016/0012-1606(88)90380-6
PMID:2458286
Abstract

Immunocytological localization of the major glycoprotein of peripheral myelin P0 and its associated carbohydrate structures L2/HNK-1 and L3 was performed at the light- and electron-microscopic levels in mouse sciatic nerves at several developmental stages and in adulthood. P0 was first expressed on Schwann cells at the time that Schwann cells associated with axons on a 1:1 basis. P0 remains expressed at all times of myelin formation and in compact myelin. After cessation of myelination P0 is no longer detectable in the uncompacted parts of myelin, i.e., Schmidt-Lanterman incisures, paranodal loops, and outer and inner mesaxons. P0 is not detectable on basement membranes, interstitial collagens, and non-myelin-forming Schwann cells. The associated carbohydrate epitope L2 does not follow the expression of P0 at any developmental or adult stage. Until 21 days the L2 epitope is confined to nonmyelinated fibers. In sciatic nerves of mice older than 8 weeks, however, only a few nonmyelinated fibers remain L2-positive. L2 immunoreactivity is clearly seen in a subpopulation of compact myelin figures largely associated with motor fibers. The L3 epitope is never detectable on nonmyelinated fibers and becomes first visible when compact myelin is discerned. Unlike the L2 epitope L3 is present in most, if not all, compact myelin figures. These observations suggest that P0 may be involved in ensheathment of axons by Schwann cells at the decisive stages of initiation of myelination and later on, possibly in conjunction with the L3 carbohydrate structure, in maintenance of compact myelin. The appearance of the L2 carbohydrate epitopes in compact myelin of largely motor and fewer sensory nerve fibers at times when morphogenesis of myelin has ceased remains to be elucidated in functional terms.

摘要

在几个发育阶段及成年期的小鼠坐骨神经中,利用光镜和电镜技术对外周髓磷脂主要糖蛋白P0及其相关碳水化合物结构L2/HNK-1和L3进行了免疫细胞定位。P0最初在雪旺细胞与轴突以1:1比例结合时在雪旺细胞上表达。在髓磷脂形成的所有阶段以及致密髓磷脂中,P0持续表达。髓鞘形成停止后,在髓磷脂未致密化的部分,即施密特-兰特尔曼切迹、结旁环以及内外系膜中,不再能检测到P0。在基底膜、间质胶原以及非形成髓磷脂的雪旺细胞上检测不到P0。相关碳水化合物表位L2在任何发育阶段或成年期均不随P0的表达而变化。直到21天,L2表位局限于无髓纤维。然而,在8周龄以上小鼠的坐骨神经中,只有少数无髓纤维仍为L2阳性。在主要与运动纤维相关的致密髓磷脂亚群中可清晰见到L2免疫反应性。在无髓纤维上从未检测到L3表位,当致密髓磷脂可辨时首次可见L3表位。与L2表位不同,L3存在于大多数(如果不是全部)致密髓磷脂结构中。这些观察结果表明,P0可能在髓鞘形成起始的决定性阶段参与雪旺细胞对轴突的包裹,随后可能与L3碳水化合物结构一起参与致密髓磷脂的维持。在髓鞘形态发生停止时,L2碳水化合物表位在主要为运动神经纤维和较少感觉神经纤维的致密髓磷脂中的出现,其功能方面仍有待阐明。

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