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用于开发用于生物打印的稳健墨水的实验设计方法。

Design of experiments approach to developing a robust ink for bioprinting.

作者信息

Hegab Rachel, Van Volkenburg Tessa, Ohiri Korine, Sebeck Natalie, Bessling Seneca, Theodore Mellisa, Rossick Katelyn, Pellicore Matthew, Benkoski Jason, Patrone Julia

机构信息

The Johns Hopkins Applied Physics Laboratory, Laurel, MD, United States of America.

出版信息

Biomed Phys Eng Express. 2022 Mar 24;8(3). doi: 10.1088/2057-1976/ac5de1.

Abstract

Despite advancements in tissue engineering, the methods used to generate three-dimensional (3D)models for rapid screening and characterization studies remain time and labor intensive. Bioprinting offers an opportunity to offset these limitations by providing a scalable, high-throughput method with precise control over biomaterial scaffold and cellular deposition. However, the process of formulating bioinks can be complex in terms of balancing the mechanical integrity of a bioscaffold and viability of cells. One key factor, especially in alginate-based bioinks, is the rate of bioscaffold dissolution. It must allow cells to replace the bioscaffold with extracellular matrix (ECM), yet remain durable during extended tissue culture. This study uses a Design of Experiments (DoE) approach to understand the dependencies of multiple variables involved in the formulation and processing of an alginate-based bioink. The focus of the DoE was to understand the effects of hydrogel composition on bioink durability while maintaining cell viability. Three ingredients were varied in all: alginate, nanocellulose, and fibrinogen. Their effects on the bioink were then measured with respect to extrudability, strength, and stiffness as determined by dynamic mechanical analysis (DMA). The DoE demonstrated that mechanical integrity increased with increasing alginate concentration. In contrast, fibrinogen and nanofibril concentration had no statistically significant effect. The optimized ink containing fibroblasts was printable using multiple nozzle sizes while also supporting fibroblast cell viability. DMA characterization further showed that the composition of the cell culture medium did not modulate the degradation rate of the hydrogel. Ultimately, the study outlines a methodology for formulating a bioink that will result in robust bioscaffolds formodel development.

摘要

尽管组织工程取得了进展,但用于生成三维(3D)模型以进行快速筛选和表征研究的方法仍然耗时且费力。生物打印提供了一个机会来弥补这些局限性,它提供了一种可扩展的、高通量的方法,能够精确控制生物材料支架和细胞沉积。然而,就平衡生物支架的机械完整性和细胞活力而言,生物墨水的配制过程可能很复杂。一个关键因素,尤其是在基于藻酸盐的生物墨水中,是生物支架的溶解速率。它必须允许细胞用细胞外基质(ECM)取代生物支架,但在长时间的组织培养过程中仍保持耐用性。本研究采用实验设计(DoE)方法来了解基于藻酸盐的生物墨水配制和加工过程中涉及的多个变量之间的依赖性。DoE的重点是了解水凝胶组成对生物墨水耐久性的影响,同时保持细胞活力。总共改变了三种成分:藻酸盐、纳米纤维素和纤维蛋白原。然后通过动态力学分析(DMA)测定它们对生物墨水的挤出性、强度和刚度的影响。DoE表明,机械完整性随着藻酸盐浓度的增加而提高。相比之下,纤维蛋白原和纳米纤维浓度没有统计学上的显著影响。含有成纤维细胞的优化墨水可以使用多种喷嘴尺寸进行打印,同时还能支持成纤维细胞的活力。DMA表征进一步表明,细胞培养基的组成不会调节水凝胶的降解速率。最终,该研究概述了一种配制生物墨水的方法,该方法将产生用于模型开发的坚固生物支架。

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