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去细胞化神经移植物构建具有轴向排列通道的外周神经再生导管

Decellularized grafts with axially aligned channels for peripheral nerve regeneration.

机构信息

Trinity Centre for Bioengineering, Trinity Biomedical Sciences Institute, Trinity College Dublin, Dublin, Ireland; School of Engineering, Trinity College Dublin, Dublin, Ireland; Tissue Engineering Research Group, Department of Anatomy, Royal College of Surgeons in Ireland, Dublin, Ireland.

Trinity Centre for Bioengineering, Trinity Biomedical Sciences Institute, Trinity College Dublin, Dublin, Ireland; School of Engineering, Trinity College Dublin, Dublin, Ireland; School of Medicine, Trinity College Dublin, Dublin, Ireland.

出版信息

J Mech Behav Biomed Mater. 2015 Jan;41:124-35. doi: 10.1016/j.jmbbm.2014.10.002. Epub 2014 Oct 14.

Abstract

At least 2 million people worldwide suffer annually from peripheral nerve injuries (PNI), with estimated costs of $7 billion incurred due to paralysis alone. The current "gold" standard for treatment of PNI is the autograft, which poses disadvantages such as high fiscal cost, possible loss of sensation at donor site and the requirement of two surgeries. Allografts are viable alternatives; however, intensive immunosuppressive treatments are often necessary to prevent host rejection. For this reason, significant efforts have been made to remove cellular material from allografts. These decellularized nerve grafts perform better than other clinically available grafts but not as well as autografts; therefore, current research on these grafts includes the incorporation of additional components such as growth factors and cells to provide chemical guidance to regenerating axons. However, effective cellular and axonal penetration is not achieved due to the small pore size (5-10μm) of the decellularized grafts. The overall objective of this study was to induce axially aligned channels in decellularized nerve grafts to facilitate enhanced cell penetration. The specific aims of this study were to optimize a decellularization method to enhance cellular removal, to induce axially aligned pore formation in decellularized grafts through a novel unidirectional freeze drying method, to study the bulk mechanical properties of these modified decellularized grafts and to assess cell penetration into these grafts. To this end we modified an existing decellularization protocol to improve cellular removal while preserving matrix structure in rat sciatic nerve sections. Standard freeze drying and unidirectional freeze drying were employed to impart the necessary pore architecture, and our results suggest that unidirectional freezing is a pertinent modification to the freeze drying process to obtain axially aligned channels. These highly porous scaffolds obtained using unidirectional freeze-drying possessed similar tensile properties to native nerve tissue and exhibited enhanced cellular penetration after 14 days of culture when compared to non-freeze dried and standard freeze-dried scaffolds. The results of this study not only highlight the importance of aligned pores of diameters ~20-60μm on cellular infiltration, but also presents unidirectional freeze drying as a viable technique for producing this required architecture in decellularized nerves. To the best of our knowledge, this study represents the first attempt to manipulate the physical structure of decellularized nerves to enhance cell penetration which may serve as a basis for future peripheral nerve regenerative strategies using decellularized allografts.

摘要

全世界每年至少有 200 万人患有周围神经损伤(PNI),仅瘫痪一项就造成了 70 亿美元的估计损失。目前 PNI 的“金标准”治疗方法是自体移植物,但存在高财政成本、供体部位感觉丧失的可能性以及需要进行两次手术等缺点。同种异体移植物是可行的替代品;然而,为了防止宿主排斥反应,通常需要进行密集的免疫抑制治疗。出于这个原因,人们已经做出了巨大的努力来去除同种异体移植物中的细胞物质。这些去细胞化神经移植物的性能优于其他临床可用的移植物,但不如自体移植物;因此,目前对这些移植物的研究包括加入其他成分,如生长因子和细胞,为再生轴突提供化学导向。然而,由于去细胞化移植物的小孔径(5-10μm),有效细胞和轴突穿透并未实现。本研究的总体目标是在去细胞化神经移植物中诱导轴向对齐的通道,以促进增强的细胞穿透。本研究的具体目标是优化一种去细胞化方法以增强细胞去除,通过新颖的单向冷冻干燥方法在去细胞化移植物中诱导轴向对齐的孔形成,研究这些改性去细胞化移植物的整体力学性能,并评估细胞穿透这些移植物。为此,我们修改了现有的去细胞化方案,以在保留基质结构的同时提高细胞去除率。标准冷冻干燥和单向冷冻干燥用于赋予必要的孔结构,我们的结果表明,单向冷冻是冷冻干燥过程的一个相关改进,以获得轴向对齐的通道。使用单向冷冻干燥获得的这些高多孔支架具有与天然神经组织相似的拉伸性能,并且在 14 天的培养后与未冷冻干燥和标准冷冻干燥支架相比,表现出增强的细胞穿透性。这项研究的结果不仅强调了直径为~20-60μm的对齐孔对细胞渗透的重要性,还提出了单向冷冻干燥作为在去细胞化神经中产生这种所需结构的可行技术。据我们所知,这项研究代表了首次尝试操纵去细胞化神经的物理结构以增强细胞穿透性,这可能为未来使用去细胞化同种异体移植物进行周围神经再生策略提供基础。

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