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横断后再髓鞘化小鼠坐骨神经轴突中的钠离子通道聚集

Na+ channel aggregation in remyelinating mouse sciatic axons following transection.

作者信息

Tzoumaka E E, Novaković S D, Levinson S R, Shrager P

机构信息

Department of Physiology, University of Rochester Medical Center, NY 14642-8642, USA.

出版信息

Glia. 1995 Oct;15(2):188-94. doi: 10.1002/glia.440150211.

Abstract

Mouse sciatic nerves from the degeneration-resistant strain C57BL/6/Wld (Ola) were surgically injected with lysolecithin to induce focal demyelination. Three days later they were transected adjacent to the spinal cord to eliminate contact of the axons with their cell bodies. The Na+ channel distribution was assessed by immunocytochemistry and followed at several stages of remyelination. Control experiments were performed on nerves that were injected but not cut. At (3 + 4) days, namely, nerves cut 3 days post-injection and examined 4 days after cutting, axons contained fully demyelinated regions. Na+ channel clusters appeared only at heminodes and at isolated sites that are likely to represent original nodes of Ranvier. During the next few days proliferating Schwann cells adhered to the axons and extended their processes. Clusters of Na+ channels appeared at their edges, and as the Schwann cells elongated the distance between these aggregates increased. A few clusters associated with neighboring Schwann cells approached each other and appeared to coalesce at sites where presumably new nodes of Ranvier would be formed. Beyond (3 + 6) days excessive degeneration of the transected axons precluded further observations. In the uncut controls, the spatio-temporal sequence of Schwann cell proliferation and channel patch formation and movement was similar to that described above, although myelin formation was somewhat faster than in the cut axons. It is concluded that Na+ channel aggregation associated with the early stages of remyelination is not dependent upon continuous communication of the axon with its cell body and is under local control.

摘要

对来自抗变性品系C57BL/6/Wld(Ola)的小鼠坐骨神经进行手术注射溶血卵磷脂,以诱导局灶性脱髓鞘。三天后,在靠近脊髓处将其横断,以消除轴突与其细胞体的接触。通过免疫细胞化学评估Na⁺通道分布,并在髓鞘再生的几个阶段进行跟踪。对注射但未切断的神经进行对照实验。在(3 + 4)天时,即注射后3天切断神经并在切断后4天进行检查,轴突包含完全脱髓鞘区域。Na⁺通道簇仅出现在半结处以及可能代表原始郎飞结的孤立部位。在接下来的几天里,增殖的雪旺细胞粘附到轴突上并伸出其突起。Na⁺通道簇出现在它们的边缘,随着雪旺细胞伸长,这些聚集体之间的距离增加。一些与相邻雪旺细胞相关的簇相互靠近,并似乎在可能形成新郎飞结的部位融合。超过(3 + 6)天后,横断轴突的过度变性使进一步观察无法进行。在未切断的对照中,雪旺细胞增殖以及通道斑块形成和移动的时空序列与上述情况相似,尽管髓鞘形成比切断的轴突稍快。结论是,与髓鞘再生早期相关的Na⁺通道聚集不依赖于轴突与其细胞体的持续通讯,而是受局部控制。

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