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周围神经退变与再生过程中髓磷脂脂质的命运:一项放射自显影研究。

Fate of myelin lipids during degeneration and regeneration of peripheral nerve: an autoradiographic study.

作者信息

Goodrum J F, Earnhardt T, Goines N, Bouldin T W

机构信息

Brain and Development Research Center, University of North Carolina at Chapel Hill 27599.

出版信息

J Neurosci. 1994 Jan;14(1):357-67. doi: 10.1523/JNEUROSCI.14-01-00357.1994.

Abstract

Four weeks after labeling myelin lipids with an intraneural injection of 3H-acetate, sciatic nerves were crushed, and the distribution of radiolabeled myelin lipids was followed by autoradiography from 1 d to 10 weeks later. Just prior to crush, silver grains were localized to the myelin sheath. Three days after crush, axons were degenerating and myelin sheaths were breaking down; silver grains appeared over lipid droplets within Schwann cells, fibroblasts, and macrophages. One week after crush the basal-lamina-delimited Schwann-cell tubes (Büngner bands) contained myelin debris, and some tubes already contained regenerating axons. Schwann cells were often displaced to the periphery of the tubes by phagocytes containing heavily labeled myelin debris; extratubal macrophages within the endoneurium contained labeled lipid droplets but no myelin debris. Two weeks after nerve crush silver grains were associated with newly formed myelin around regenerating axons. Many extratubal endoneurial macrophages now contained labeled myelin debris and lipid droplets. By 3 weeks myelination of regenerating axons was advanced, and the myelin sheaths were well labeled. Extratubal macrophages had become the major labeled structure within the nerve because they contained large amounts of labeled myelin debris and lipid droplets. From 4 to 10 weeks after nerve crush the new myelin sheaths continued to thicken and to be well labeled. Debris-laden extratubal macrophages remained the major site of labeled material within the endoneurium. Our results confirm that there is reutilization of myelin cholesterol by Schwann cells to form new myelin, and indicate that some lipid catabolism takes place in Schwann cells and endoneurial fibroblasts prior to infiltration of the nerve by macrophages. However, most of the myelin debris is phagocytized by macrophages within 1-2 weeks following nerve injury. These debris-laden macrophages persist within the nerve for many weeks, indicating that much of the salvaged cholesterol is not reutilized for myelin regeneration.

摘要

在通过神经内注射³H - 醋酸盐标记髓磷脂脂质四周后,对坐骨神经进行挤压,然后通过放射自显影追踪放射性标记的髓磷脂脂质从挤压后1天到10周的分布情况。在挤压前,银颗粒定位于髓鞘。挤压三天后,轴突开始退化,髓鞘开始分解;银颗粒出现在施万细胞、成纤维细胞和巨噬细胞内的脂滴上。挤压一周后,基膜界定的施万细胞管(Büngner带)含有髓磷脂碎片,一些管中已经含有再生轴突。施万细胞常常被含有大量标记髓磷脂碎片的吞噬细胞挤到管的周边;神经内膜内的管外巨噬细胞含有标记的脂滴但没有髓磷脂碎片。神经挤压两周后,银颗粒与再生轴突周围新形成的髓磷脂相关。许多管外神经内膜巨噬细胞现在含有标记的髓磷脂碎片和脂滴。到3周时,再生轴突的髓鞘化进程加快,髓鞘被很好地标记。管外巨噬细胞已成为神经内主要的标记结构,因为它们含有大量标记的髓磷脂碎片和脂滴。在神经挤压后4至10周,新的髓鞘继续增厚并被很好地标记。充满碎片的管外巨噬细胞仍然是神经内膜内标记物质的主要部位。我们的结果证实施万细胞会重新利用髓磷脂胆固醇来形成新的髓磷脂,并表明在巨噬细胞侵入神经之前,施万细胞和神经内膜成纤维细胞会发生一些脂质分解代谢。然而,大多数髓磷脂碎片在神经损伤后1 - 2周内被巨噬细胞吞噬。这些充满碎片的巨噬细胞在神经内持续存在数周,这表明许多 salvaged胆固醇并未被重新用于髓磷脂再生。

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