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使用可控灌注法对全人肝移植物进行去细胞处理以制备可移植器官生物支架

Decellularization of Whole Human Liver Grafts Using Controlled Perfusion for Transplantable Organ Bioscaffolds.

作者信息

Verstegen Monique M A, Willemse Jorke, van den Hoek Sjoerd, Kremers Gert-Jan, Luider Theo M, van Huizen Nick A, Willemssen Francois E J A, Metselaar Herold J, IJzermans Jan N M, van der Laan Luc J W, de Jonge Jeroen

机构信息

1 Department of Surgery, Erasmus MC-University Medical Center , Rotterdam, the Netherlands .

2 Erasmus Optical Imaging Centre, Erasmus MC-University Medical Center , Rotterdam, the Netherlands .

出版信息

Stem Cells Dev. 2017 Sep 15;26(18):1304-1315. doi: 10.1089/scd.2017.0095. Epub 2017 Jul 31.

DOI:10.1089/scd.2017.0095
PMID:28665233
Abstract

Liver transplantation is the only effective treatment for end-stage liver disease, but absolute donor shortage remains a limiting factor. Recent advances in tissue engineering focus on generation of native extracellular matrix (ECM) by decellularized complete livers in animal models. Although proof of concept has been reported for human livers, this study aims to perform whole liver decellularization in a clinically relevant series using controlled machine perfusion. In this study, we describe a mild nondestructive decellularization protocol, effective in 11 discarded human whole liver grafts to generate constructs that reliably maintain hepatic architecture and ECM components using machine perfusion, while completely removing cellular DNA and RNA. The decellularization process preserved the ultrastructural ECM components confirmed by histology, electron microscopy, and proteomic analysis. Anatomical characteristics of the native microvascular network and biliary drainage of the liver were confirmed by contrast computed tomography scanning. Decellularized vascular matrix remained suitable for normal suturing and no major histocompatibility complex molecules were detected, suggesting absence of allo-reactivity when used for transplantation. After extensive washing, decellularized scaffolds were nontoxic for cells after reseeding human mesenchymal stromal or umbilical vein endothelial endothelium cells. Indeed, evidence of effective recellularization of the vascular lining was obtained. In conclusion, we established an effective method to generate clinically applicable liver scaffolds from human discarded whole liver grafts and show proof of concept that reseeding of normal human cells in the scaffold is feasible. This supports new opportunities for bioengineering of transplantable grafts in the future.

摘要

肝移植是终末期肝病的唯一有效治疗方法,但供体绝对短缺仍然是一个限制因素。组织工程学的最新进展集中在通过动物模型中去细胞化的完整肝脏生成天然细胞外基质(ECM)。尽管已经报道了人类肝脏的概念验证,但本研究旨在使用可控机器灌注在一系列临床相关的肝脏中进行全肝去细胞化。在本研究中,我们描述了一种温和的非破坏性去细胞化方案,该方案对11个废弃的人类全肝移植物有效,通过机器灌注生成能够可靠维持肝脏结构和ECM成分的构建体,同时完全去除细胞DNA和RNA。去细胞化过程保留了通过组织学、电子显微镜和蛋白质组分析证实的超微结构ECM成分。通过对比计算机断层扫描确认了肝脏天然微血管网络和胆汁引流的解剖学特征。去细胞化的血管基质仍然适合正常缝合,未检测到主要组织相容性复合体分子,表明用于移植时不存在同种异体反应性。经过广泛冲洗后,去细胞化支架在重新接种人间充质基质或脐静脉内皮细胞后对细胞无毒。事实上,获得了血管内衬有效再细胞化的证据。总之,我们建立了一种从人类废弃全肝移植物中生成临床适用肝脏支架的有效方法,并证明了在支架中重新接种正常人细胞是可行的这一概念。这为未来可移植移植物的生物工程提供了新的机会。

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