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在一个明确的体外系统中,感觉神经元的髓鞘形成和郎飞氏结的形成。

Myelination and node of Ranvier formation on sensory neurons in a defined in vitro system.

机构信息

NanoScience Technology Center, University Central Florida, Orlando, FL 32826, USA.

College of Medicine, University Central Florida, Orlando, FL 32826, USA.

出版信息

In Vitro Cell Dev Biol Anim. 2013 Sep;49(8):608-618. doi: 10.1007/s11626-013-9647-8. Epub 2013 Aug 16.

Abstract

One of the most important developmental modifications of the nervous system is Schwann cell myelination of axons. Schwann cells ensheath axons to create myelin segments to provide protection to the axon as well as increase the conduction of action potentials. In vitro neuronal systems provide a unique modality to study a variety of factors influencing myelination as well as diseases associated with myelin sheath degradation. This work details the development of a patterned in vitro myelinating dorsal root ganglion culture. This defined system utilized a serum-free medium in combination with a patterned substrate, utilizing the cytophobic and cytophilic molecules (poly)ethylene glycol (PEG) and N-1[3 (trimethoxysilyl) propyl] diethylenetriamine (DETA), respectively. Directional outgrowth of the neurites and subsequent myelination was controlled by surface modifications, and conformity to the pattern was measured over the duration of the experiments. The myelinated segments and nodal proteins were visualized and quantified using confocal microscopy. This tissue-engineered system provides a highly controlled, reproducible model for studying Schwann cell interactions with sensory neurons, as well as the myelination process, and its effect on neuronal plasticity and peripheral nerve regeneration. It is also compatible for use in bio-hybrid constructs to reproduce the stretch reflex arc on a chip because the media combination used is the same that we have used previously for motoneurons, muscle, and for neuromuscular junction (NMJ) formation. This work could have application for the study of demyelinating diseases such as diabetes induced peripheral neuropathy and could rapidly translate to a role in the discovery of drugs promoting enhanced peripheral nervous system (PNS) remyelination.

摘要

神经系统最重要的发育性改变之一是轴突的施万细胞髓鞘形成。施万细胞包裹轴突形成髓鞘段,为轴突提供保护,并增加动作电位的传导。体外神经元系统为研究影响髓鞘形成的各种因素以及与髓鞘降解相关的疾病提供了一种独特的方式。这项工作详细介绍了体外有图案的背根神经节培养物的髓鞘形成。该定义系统在无血清培养基中结合图案化基质,分别利用亲脂性和疏脂性分子(聚)乙二醇(PEG)和 N-1[3(三甲氧基硅基)丙基]二乙撑三胺(DETA)。神经突的定向生长和随后的髓鞘形成由表面修饰控制,并在实验过程中测量与图案的一致性。使用共聚焦显微镜可视化和量化髓鞘化段和节蛋白。该组织工程系统提供了一种高度可控、可重复的模型,用于研究施万细胞与感觉神经元的相互作用以及髓鞘形成过程及其对神经元可塑性和周围神经再生的影响。它也可用于生物混合结构,在芯片上再现牵张反射弧,因为我们之前已经使用过相同的培养基组合来培养运动神经元、肌肉和运动终板(NMJ)形成。这项工作可应用于研究脱髓鞘疾病,如糖尿病引起的周围神经病变,并可迅速转化为促进增强周围神经系统(PNS)髓鞘形成药物发现的作用。

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本文引用的文献

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A new long term in vitro model of myelination.一种新的长时程体外髓鞘形成模型。
Exp Cell Res. 2011 Oct 1;317(16):2374-83. doi: 10.1016/j.yexcr.2011.07.002. Epub 2011 Jul 12.

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