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体外培养的人雪旺细胞。II. 经过广泛纯化和Heregulin诱导扩增后感觉轴突的髓鞘形成。

Human Schwann cells in vitro. II. Myelination of sensory axons following extensive purification and heregulin-induced expansion.

作者信息

Morrissey T K, Kleitman N, Bunge R P

机构信息

Miami Project to Cure Paralysis, University of Miami School of Medicine, Florida 33136, USA.

出版信息

J Neurobiol. 1995 Oct;28(2):190-201. doi: 10.1002/neu.480280206.

DOI:10.1002/neu.480280206
PMID:8537824
Abstract

Co-culture conditions are well established in which Schwann cells (SCs) derived from immature or adult rats proliferate and form myelin in response to contact with sensory axons. In a companion article, we report that populations of adult-derived human Schwann cells (HASCs) fail to function under these co-culture conditions. Furthermore, we report progressive atrophy of neurons in co-cultures containing populations of either human fibroblasts or HASCs (which contain both SCs and fibroblasts). Two factors that might account for the insufficiency of the co-culture system to support HASC differentiation are the failure of many HASCs to proliferate and the influence of contaminating fibroblasts. To minimize fibroblast contamination of neuron-HASC co-cultures, we used fluorescence-activated cell sorting to highly purify HASC populations (to more than 99.8%). To stimulate expansion of the HASC population, a mitogenic mixture of heregulin (HRG beta 1 amino acid residues 177-244; 10 nM), cholera toxin (100 ng/mL), and forskolin (1 microM) was used. When these purified and expanded HASCs were co-cultured with embryo-derived rat sensory neurons, neuronal shrinkage did not occur and after 4 to 6 weeks some myelin segments were seen in living co-cultures. This myelin was positively identified as human by immunostaining with a monoclonal antibody specific to the human peripheral myelin protein P0 (antibody 592). Although this is the first reported observation of myelination by HASCs in tissue culture, it should be noted that myelination occurred more slowly and in much less abundance than in comparable cultures containing adult rat-derived SCs. We anticipate that further refinements of the HASC co-culture system that enhance myelin formation will provide insights into important aspects of human SC biology and provide new opportunities for studies of human peripheral neuropathies.

摘要

共培养条件已得到充分确立,在此条件下,源自未成熟或成年大鼠的雪旺细胞(SCs)会增殖,并在与感觉轴突接触时形成髓鞘。在一篇配套文章中,我们报道成年来源的人雪旺细胞(HASCs)群体在这些共培养条件下无法发挥功能。此外,我们报道在含有人类成纤维细胞群体或HASCs群体(其中包含SCs和成纤维细胞)的共培养物中,神经元会逐渐萎缩。共培养系统支持HASC分化不足的两个可能因素是许多HASCs无法增殖以及污染的成纤维细胞的影响。为了尽量减少神经元 - HASC共培养物中的成纤维细胞污染,我们使用荧光激活细胞分选技术高度纯化HASC群体(纯度超过99.8%)。为了刺激HASC群体的扩增,使用了由heregulin(HRGβ1氨基酸残基177 - 244;10 nM)、霍乱毒素(100 ng/mL)和福司可林(1 μM)组成的促有丝分裂混合物。当这些纯化和扩增的HASCs与胚胎来源的大鼠感觉神经元共培养时,未观察到神经元萎缩,并且在4至6周后,在活的共培养物中可见一些髓鞘节段。通过用针对人外周髓鞘蛋白P0的单克隆抗体(抗体592)进行免疫染色,这种髓鞘被确认为人源。尽管这是首次报道在组织培养中HASCs形成髓鞘的观察结果,但应该注意的是,与含有成年大鼠来源SCs的类似培养物相比,髓鞘形成更慢且数量更少。我们预计,进一步优化HASC共培养系统以增强髓鞘形成,将为深入了解人SCs生物学的重要方面提供见解,并为研究人类周围神经病变提供新的机会。

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