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在24孔板格式的分隔微流控装置上开发一种人体神经肌肉芯片组织模型。

Development of a human neuromuscular tissue-on-a-chip model on a 24-well-plate-format compartmentalized microfluidic device.

作者信息

Yamamoto Kazuki, Yamaoka Nao, Imaizumi Yu, Nagashima Takunori, Furutani Taiki, Ito Takuji, Okada Yohei, Honda Hiroyuki, Shimizu Kazunori

机构信息

Department of Biomolecular Engineering, Graduate School of Engineering, Nagoya University, Nagoya, Aichi, Japan.

Department of Neurology, Aichi Medical University School of Medicine, Nagakute, Aichi, Japan.

出版信息

Lab Chip. 2021 May 18;21(10):1897-1907. doi: 10.1039/d1lc00048a.

DOI:10.1039/d1lc00048a
PMID:34008665
Abstract

Engineered three-dimensional models of neuromuscular tissues are promising for use in mimicking their disorder states in vitro. Although several models have been developed, it is still challenging to mimic the physically separated structures of motor neurons (MNs) and skeletal muscle (SkM) fibers in the motor units in vivo. In this study, we aimed to develop microdevices for precisely compartmentalized coculturing of MNs and engineered SkM tissues. The developed microdevices, which fit a well of 24 well plates, had a chamber for MNs and chamber for SkM tissues. The two chambers were connected by microtunnels for axons, permissive to axons but not to cell bodies. Human iPSC (hiPSC)-derived MN spheroids in one chamber elongated their axons into microtunnels, which reached the tissue-engineered human SkM in the SkM chamber, and formed functional neuromuscular junctions with the muscle fibers. The cocultured SkM tissues with MNs on the device contracted spontaneously in response to spontaneous firing of MNs. The addition of a neurotransmitter, glutamate, into the MN chamber induced contraction of the cocultured SkM tissues. Selective addition of tetrodotoxin or vecuronium bromide into either chamber induced SkM tissue relaxation, which could be explained by the inhibitory mechanisms. We also demonstrated the application of chemical or mechanical stimuli to the middle of the axons of cocultured tissues on the device. Thus, compartmentalized neuromuscular tissue models fabricated on the device could be used for phenotypic screening to evaluate the cellular type specific efficacy of drug candidates and would be a useful tool in fundamental research and drug development for neuromuscular disorders.

摘要

工程化的神经肌肉组织三维模型有望用于在体外模拟其疾病状态。尽管已经开发了几种模型,但在体内模拟运动单位中运动神经元(MNs)和骨骼肌(SkM)纤维的物理分离结构仍然具有挑战性。在本研究中,我们旨在开发用于MNs和工程化SkM组织精确分隔共培养的微型装置。所开发的微型装置适合24孔板的一个孔,有一个用于MNs的腔室和一个用于SkM组织的腔室。两个腔室通过用于轴突的微通道相连,该微通道允许轴突通过但不允许细胞体通过。一个腔室中源自人诱导多能干细胞(hiPSC)的MN球体将其轴突延伸到微通道中,这些轴突到达SkM腔室中的组织工程化人SkM,并与肌纤维形成功能性神经肌肉接头。装置上与MNs共培养的SkM组织会响应MNs的自发放电而自发收缩。向MN腔室中添加神经递质谷氨酸会诱导共培养的SkM组织收缩。向任一腔室中选择性添加河豚毒素或维库溴铵会导致SkM组织松弛,这可以用抑制机制来解释。我们还展示了对装置上共培养组织轴突中部施加化学或机械刺激的应用。因此,在该装置上制造的分隔神经肌肉组织模型可用于表型筛选,以评估候选药物的细胞类型特异性疗效,并且将成为神经肌肉疾病基础研究和药物开发中的有用工具。

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