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将生物打印与3D细胞培养相结合,以增强打印合成构建物中的组织形成。

Synergizing bioprinting and 3D cell culture to enhance tissue formation in printed synthetic constructs.

作者信息

Günther Daniel, Bergerbit Cédric, Marsee Ary, Vedaraman Sitara, Pueyo Moliner Alba, Bastard Céline, Eelen Guy, Gerardo Nava José Luis, Dewerchin Mieke, Carmeliet Peter, Kramann Rafael, Schneeberger Kerstin, Spee Bart, De Laporte Laura

机构信息

DWI-Leibniz Institute for Interactive Materials, Aachen, Germany.

Institute of Technical and Macromolecular Chemistry, Advanced Materials for Biomedicine (AMB), RWTH Aachen University, Aachen, Germany.

出版信息

Biofabrication. 2025 Feb 14;17(2). doi: 10.1088/1758-5090/adae37.

Abstract

Bioprinting is currently the most promising method to biofabricate complex tissueswith the potential to transform the future of organ transplantation and drug discovery. Efforts to create such tissues are, however, almost exclusively based on animal-derived materials, such as gelatin methacryloyl, which have demonstrated efficacy in bioprinting of complex tissues. While these materials are already used in clinical applications, uncertainty about their safety still remains due to their animal origin. Alternatively, synthetic bioinks have been developed that match the printability of natural bioinks but lack their biological complexity, and thereby often fail to support cell growth and facilitate tissue formation. Additionally, most synthetic materials do not meet the mechanical demands of bioprint stable constructs while providing a suitable environment for cells to grow, limiting the number of available bioinks. To bridge this gap and synergize bioprinting and 3D cell culture, we developed a polyethylene glycol-based bioink system to promote the growth and spreading of cell spheroids that consist of human primary endothelial cells and fibroblasts. The 3D bioprinted centimeter-scale constructs have a high shape fidelity and accelerated softening to provide sufficient space for cells to grow. Adjusting the rate of degradability, induced by the integration of ester-functionalized crosslinkers in addition to protease cleavable crosslinkers into the hydrogel network, improves the growth of spheroids in larger printed hydrogel constructs containing an interconnected channel structure. The perfusable constructs enable extensive spheroid sprouting and the formation of a cellular network upon fusion of sprouts as initial steps toward tissue formation with the potential for clinical translation.

摘要

生物打印是目前生物制造复杂组织最具前景的方法,具有改变器官移植和药物研发未来的潜力。然而,制造此类组织的努力几乎完全基于动物源材料,如甲基丙烯酰化明胶,这些材料已在复杂组织的生物打印中证明了其有效性。虽然这些材料已用于临床应用,但由于其动物来源,其安全性仍存在不确定性。另外,已开发出合成生物墨水,其打印性能与天然生物墨水相当,但缺乏生物复杂性,因此常常无法支持细胞生长和促进组织形成。此外,大多数合成材料在为细胞生长提供合适环境的同时,无法满足生物打印稳定结构的机械要求,限制了可用生物墨水的数量。为了弥合这一差距并使生物打印与3D细胞培养协同作用,我们开发了一种基于聚乙二醇的生物墨水系统,以促进由人原代内皮细胞和成纤维细胞组成的细胞球状体的生长和扩散。3D生物打印的厘米级构建体具有高形状保真度和加速软化,为细胞生长提供了足够的空间。通过在水凝胶网络中除了整合蛋白酶可裂解交联剂之外还整合酯官能化交联剂来调节降解速率,可改善在含有相互连接通道结构的较大打印水凝胶构建体中球状体的生长。可灌注的构建体能够实现广泛的球状体发芽,并在芽融合时形成细胞网络,这是组织形成的初始步骤,具有临床转化的潜力。

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