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马内皮祖细胞包封在高度均匀的可注射水凝胶微球中,用于局部细胞递送。

Encapsulation of Equine Endothelial Colony Forming Cells in Highly Uniform, Injectable Hydrogel Microspheres for Local Cell Delivery.

机构信息

1 Department of Chemical Engineering, Auburn University, Auburn, Alabama.

2 Department of Clinical Sciences, College of Veterinary Medicine, Auburn University, Auburn, Alabama.

出版信息

Tissue Eng Part C Methods. 2017 Nov;23(11):815-825. doi: 10.1089/ten.TEC.2017.0233. Epub 2017 Oct 12.

DOI:10.1089/ten.TEC.2017.0233
PMID:28762895
Abstract

A common challenge in cell therapy is the inability to routinely maintain survival and localization of injected therapeutic cells. Delivering cells by direct injection increases the flexibility of clinical applications, but may cause low cell viability and retention rates due to the high shear forces in the needle and mechanical wash out. In this study, we encapsulated endothelial colony forming cells (ECFCs) in poly(ethylene glycol)-fibrinogen (PF) hydrogel microspheres using a custom-built microfluidic device; this system supports rapid encapsulation of high cell concentrations (10 million cells per mL) and resulting cell-laden microspheres are highly uniform in shape and size. The encapsulated ECFCs were shown to have >95% viability and continued to rapidly proliferate. Expression of cell markers (von Willebrand factor, CD105, and CD14), the ability to form tubules on basement membrane matrix, and the ability to take up low-density lipoprotein were similar between pre- and post-encapsulated cells. Viability of encapsulated ECFCs was maintained after shear through 18-23-gauge needles. Ex vivo and in vivo cell delivery studies were performed by encapsulating and injecting autologous equine ECFCs subcutaneously into distal limb full-thickness wounds of adult horses. Injected ECFCs were visualized by labeling with fluorescent nanodots before encapsulation. One week after injection, confocal microscopy analysis of biopsies of the leading edges of the wounds showed that the encapsulated ECFCs migrated into the surrounding host tissue indicating successful retention and survival of the delivered ECFCs. Rapid, scalable cell encapsulation into PF microspheres was demonstrated to be practical for use in large animal cell therapy and is a clinically relevant method to maintain cell retention and survival after local injection.

摘要

细胞治疗中普遍存在的一个挑战是,无法常规维持注射治疗细胞的存活和定位。通过直接注射递送细胞增加了临床应用的灵活性,但由于针内的高剪切力和机械冲洗,可能导致细胞活力和保留率低。在这项研究中,我们使用定制的微流控装置将内皮祖细胞(ECFCs)包封在聚乙二醇-纤维蛋白原(PF)水凝胶微球中;该系统支持高细胞浓度(每毫升 1000 万细胞)的快速包封,并且包封的细胞微球在形状和大小上高度均匀。研究表明,包封的 ECFCs 具有>95%的活力,并继续快速增殖。细胞标志物(血管假性血友病因子、CD105 和 CD14)的表达、在基底膜基质上形成小管的能力以及摄取低密度脂蛋白的能力在包封前后的细胞之间相似。通过 18-23 号针头进行剪切后,包封的 ECFCs 的活力得以维持。通过将自体马 ECFC 包封并注射到成年马四肢全层伤口的远端皮下,进行了离体和体内细胞递送研究。在包封前,用荧光纳米点标记包封的 ECFCs 进行注射。注射后 1 周,对伤口前缘活检进行共聚焦显微镜分析显示,包封的 ECFCs 迁移到周围宿主组织中,表明递送的 ECFCs 成功保留和存活。快速、可扩展的细胞包封到 PF 微球中,证明在大动物细胞治疗中具有实际应用价值,是一种在局部注射后维持细胞保留和存活的临床相关方法。

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