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软骨素酶ABC通过脊髓损伤后接种雪旺细胞的引导通道促进轴突再生。

Chondroitinase ABC enhances axonal regrowth through Schwann cell-seeded guidance channels after spinal cord injury.

作者信息

Chau C H, Shum D K Y, Li H, Pei J, Lui Y Y, Wirthlin L, Chan Y S, Xu X-M

机构信息

Department of Biochemistry, Faculty of Medicine, University of Hong Kong, Hong Kong, China.

出版信息

FASEB J. 2004 Jan;18(1):194-6. doi: 10.1096/fj.03-0196fje. Epub 2003 Nov 20.

Abstract

Grafting of Schwann cell-seeded channels into hemisected adult rat thoracic spinal cords has been tested as a strategy to bridge the injured cord. Despite success in guiding axonal growth into the graft, regeneration across the distal graft-host interface into the host spinal cord was limited. We hypothesized that chondroitin sulfate (CS) glycoforms deposited at the gliotic front of the interface constitute a molecular barrier to axonal growth into the host cord. Because CS glycoforms deposited by purified astrocytes in vitro were removable by digestion with chondroitinase ABC, we attempted to achieve likewise by infusion of the enzyme to the host side of the interface. By 1 month post-treatment, significant numbers of regenerating axons crossed an interface that was subdued in macrophage/microglia reaction and decreased in CS-immunopositivity. The axons extended as far into the caudal cord as 5 mm, in contrast to nil in vehicle-infused controls. Fascicular organizations of axon-Schwann cell units within the regenerated tissue cable were better-preserved in enzyme-treated cords than in vehicle-infused controls. We conclude that CS glycoforms deposited during gliosis at the distal graft-host interface could be cleared by the in vivo action of chondroitinase ABC to improve prospects of axonal regeneration into the host spinal cord.

摘要

将接种雪旺细胞的通道移植到成年大鼠半横断的胸段脊髓中,已作为一种连接受损脊髓的策略进行了测试。尽管在引导轴突生长进入移植物方面取得了成功,但轴突穿过远端移植物 - 宿主界面进入宿主脊髓的再生是有限的。我们假设沉积在界面胶质化前沿的硫酸软骨素(CS)糖型构成了轴突生长进入宿主脊髓的分子屏障。由于体外纯化星形胶质细胞沉积的CS糖型可通过用软骨素酶ABC消化去除,我们试图通过将该酶注入界面的宿主侧来达到同样的效果。治疗后1个月,大量再生轴突穿过了巨噬细胞/小胶质细胞反应减弱且CS免疫阳性降低的界面。与注入载体的对照组中轴突延伸为零相比,轴突向尾侧脊髓延伸了5毫米。与注入载体的对照组相比,酶处理组再生组织束中轴突 - 雪旺细胞单元的束状组织保存得更好。我们得出结论,胶质化过程中在远端移植物 - 宿主界面沉积的CS糖型可通过软骨素酶ABC的体内作用清除,以改善轴突再生进入宿主脊髓的前景。

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