Agius E, Cochard P
Centre de Biologie du Développement, Centre National de la Recherche Scientifique Unité Mixte de Recherche 5547, affiliée à l'Institut National de la Santé et de la Recherche Médicale, Université Paul Sabatier, 31062 Toulouse, France.
J Neurosci. 1998 Jan 1;18(1):328-38. doi: 10.1523/JNEUROSCI.18-01-00328.1998.
Mechanisms regulating axon growth in the peripheral nervous system have been studied by means of an in vitro bioassay, the tissue section culture, in which regenerating neurons are grown on substrata made up of tissue sections. Sections from intact and degenerated sciatic nerves proved to be different in their ability to support neurite outgrowth of embryonic chick sensory neurons from both qualitative and quantitative points of view. On denervated nerve sections, the total length of neurites elaborated per neuron was almost twice that found on intact nerve sections. In addition, confocal microscopy revealed a striking difference between intact and denervated nerve substrata: on denervated nerve sections, neurites grew inside the internal structures of endoneurial Schwann cell tubes, within the underlying tissue sections, whereas on intact nerve sections neurites extended along endoneurial basal laminae but never entered Schwann cell tubes. Perturbation experiments were used to analyze some of the molecular determinants that control neurite outgrowth in this system. Antibodies directed against the beta1-integrin subunit inhibited neurite extension on both normal and degenerated rat sciatic nerve tissue. Strikingly, however, differential inhibition was observed using antibodies directed against extracellular matrix molecules. Anti-laminin-2 (merosin) antibodies drastically reduced both the percentage of growing neurons and the total length of neurites on denervated nerve sections, but they did not modify these parameters on sections of normal nerve. Taken together, these results suggest that laminin-2/merosin promotes neurite outgrowth in peripheral nerve environments but only after Wallerian degeneration, which is when axons are allowed to extend within endoneurial tubes.
通过一种体外生物测定法——组织切片培养,研究了调节外周神经系统轴突生长的机制。在这种方法中,再生神经元在由组织切片构成的基质上生长。从定性和定量的角度来看,完整和变性坐骨神经的切片在支持胚胎鸡感觉神经元神经突生长的能力方面被证明是不同的。在去神经支配的神经切片上,每个神经元形成的神经突总长度几乎是在完整神经切片上的两倍。此外,共聚焦显微镜显示完整和去神经支配的神经基质之间存在显著差异:在去神经支配的神经切片上,神经突生长在内神经膜雪旺细胞管的内部结构中,在下面的组织切片内,而在完整神经切片上,神经突沿着内神经膜基底层延伸,但从不进入雪旺细胞管。扰动实验被用来分析该系统中控制神经突生长的一些分子决定因素。针对β1整合素亚基的抗体抑制了在正常和变性大鼠坐骨神经组织上的神经突延伸。然而,令人惊讶的是,使用针对细胞外基质分子的抗体观察到了差异抑制。抗层粘连蛋白-2(髓磷脂素)抗体显著降低了去神经支配神经切片上生长神经元的百分比和神经突的总长度,但它们没有改变正常神经切片上的这些参数。综上所述,这些结果表明层粘连蛋白-2/髓磷脂素在外周神经环境中促进神经突生长,但仅在华勒氏变性后,即轴突被允许在内神经膜管内延伸时。