Catholic University of Louvain, Laboratory of Cell Biology; 5, place Croix du Sud, B-1348 Louvain-la-Neuve (Belgium).
Restor Neurol Neurosci. 1993 Jan 1;5(2):103-17. doi: 10.3233/RNN-1993-5201.
The damaged septohippocampal pathway was utilized to study the axonal regeneration of injured neurons. Semipermeable tubes, 2-mm long, were placed in the axis of the transected septohippocampal pathway of adult rats. In a first series of experiments, empty tubes were implanted. Even six weeks after the operation, no regenerated axons were observed in the conduit. In a second series of experiments, in order to validate our approach, segments of pre-degenerated sciatic nerves were introduced into the tubes. Under these experimental conditions, acetylcholinesterase (AChE)-containing regenerated axonal processes were detected in the grafted sciatic nerves. Glial fibrillary acidic protein (GFAP)-immunodetection showed that astroglial cells and astrocyte processes were able to progress on and into the peripheral grafts. At the electron microscopic level, axons were observed in close contact with Schwann cells which myelinated some of them. In some other cases, unmyelinated axons were also present at the surface of reactive astroglial cells filled by numerous intermediate filaments. These central glial cells had migrated among the sciatic nerve collagen fibers. No axon was detected without glial cell contact. In a third series of experiments, we implanted semipermeable tubes previously filled with a fibrin-fibronectin-containing matrix provided by peripheral regeneration chambers. One week after the implantation of the tubes containing this peripheral substrate, different cell types were observed migrating into the conduit and replacing the fibrin-fibronectin-containing matrix. Among these cells astrocytes were present as revealed by GFAP-immunocytochemistry and electron microscopic examinations. During the following weeks, axons were detected in contact with the reactive astroglial cells. AChE-histochemistry showed that axons were able to cross the two millimeter distance separating the septal part and the hippocampal part of the lesion site. GABA (γ-aminobutyric acid)-ergic fibers were also detected in the regenerated structure. These experiments show that cellular or acellular substrates provided by the PNS can promote the regeneration of CNS GABAergic and cholinergic neurons. Our observations suggest that astrocytes can take an important part, after their migration or after extending processes, in the axonal regeneration in the adult CNS of the rat, possibly in furnishing a cellular terrain for the progression of growth cones over a distance of two millimeters and in maintaining regenerated axons at least until the sixth week after the operation.
损伤的隔海马通路被用于研究受伤神经元的轴突再生。半渗透管长 2 毫米,放置在成年大鼠横断隔海马通路的轴线上。在一系列实验中,植入了空管。即使在手术后六周,在导管中也没有观察到再生轴突。在第二系列实验中,为了验证我们的方法,将预先退化的坐骨神经段引入管中。在这些实验条件下,在移植的坐骨神经中检测到含有乙酰胆碱酯酶 (AChE) 的再生轴突过程。胶质纤维酸性蛋白 (GFAP) 的免疫检测显示,星形胶质细胞和星形胶质细胞突起能够在移植的周围神经中前进和进入。在电子显微镜水平上,观察到轴突与施万细胞紧密接触,其中一些轴突被施万细胞髓鞘化。在其他一些情况下,未髓鞘化的轴突也存在于充满大量中间丝的反应性星形胶质细胞的表面。这些中枢神经胶质细胞已经在坐骨神经胶原纤维之间迁移。没有与神经胶质细胞接触的轴突被检测到。在第三系列实验中,我们植入了先前用外周再生室提供的含有纤维蛋白-纤维连接蛋白基质的半渗透管。在植入含有这种周围基质的管后一周,观察到不同的细胞类型迁移到导管中并取代含有纤维蛋白-纤维连接蛋白的基质。其中,GFAP 免疫细胞化学和电镜检查显示星形胶质细胞存在。在接下来的几周内,检测到与反应性星形胶质细胞接触的轴突。AChE 组织化学显示,轴突能够穿过分隔部分和损伤部位海马部分之间 2 毫米的距离。在再生结构中还检测到 GABA (γ-氨基丁酸) 能纤维。这些实验表明,PNS 提供的细胞或无细胞基质可以促进 CNS GABA 能和胆碱能神经元的再生。我们的观察表明,星形胶质细胞在迁移后或延伸突起后,可以在成年大鼠中枢神经系统的轴突再生中发挥重要作用,可能为生长锥在 2 毫米的距离上前进提供一个细胞地形,并至少在手术后第六周维持再生轴突。
