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用于3D打印组织工程支架内生物墨水生物打印的纤维雕刻

Fiber engraving for bioink bioprinting within 3D printed tissue engineering scaffolds.

作者信息

Diaz-Gomez Luis, Elizondo Maryam E, Koons Gerry L, Diba Mani, Chim Letitia K, Cosgriff-Hernandez Elizabeth, Melchiorri Anthony J, Mikos Antonios G

机构信息

Department of Bioengineering, Rice University, 6500 Main Street, Houston, TX, 77030, USA.

Biomaterials Lab, Rice University, 6500 Main Street, Houston, TX, 77030, USA.

出版信息

Bioprinting. 2020 Jun;18. doi: 10.1016/j.bprint.2020.e00076. Epub 2020 Jan 10.

Abstract

In this work, we describe a new 3D printing methodology for the fabrication of multimaterial scaffolds involving the combination of thermoplastic extrusion and low temperature extrusion of bioinks. A fiber engraving technique was used to create a groove on the surface of a thermoplastic printed fiber using a commercial 3D printer and a low viscosity bioink was deposited into this groove. In contrast to traditional extrusion bioinks that rely on increased viscosity to prevent lateral spreading, this groove creates a defined space for bioink deposition. By physically constraining bioink spreading, a broader range of viscosities can be used. As proof-of-concept, we fabricated and characterized a multimaterial scaffold containing poly(ε-caprolactone) (PCL) as the thermoplastic polymer and a gelatin-based bioink. A 7.5 w/v% gelatin methacryloyl (GelMA) bioink loaded with either 5 w/v% poly(lactic-co-glycolic acid) (PLGA) microparticles containing fluorescent albumin or mouse fibroblasts (1 × 10 cell/mL) was printed at 24 °C. The structure of the composite scaffolds had no significant decrease in porosity or mechanical properties as compared to the PCL control scaffolds, demonstrating the engraving technique did not significantly compromise the mechanical or structural integrity of the scaffold. The encapsulated PLGA microparticles were homogeneously distributed in the GelMA and remained in the scaffolds after incubation in PBS for 24 h at 37 °C. In addition, the viability of the fibroblasts encapsulated in the GelMA bioink and printed in the grooves of the PCL scaffolds was confirmed after 24 h of incubation. Overall, this work provides a new methodology for the preparation of 3D printed scaffolds containing a robust thermoplastic structure in combination with low viscosity bioinks.

摘要

在这项工作中,我们描述了一种用于制造多材料支架的新型3D打印方法,该方法涉及热塑性挤出和生物墨水低温挤出的结合。使用纤维雕刻技术,通过商用3D打印机在热塑性打印纤维的表面创建一个凹槽,并将低粘度生物墨水沉积到该凹槽中。与传统的依靠增加粘度来防止横向扩散的挤出生物墨水不同,这个凹槽为生物墨水的沉积创造了一个特定的空间。通过物理限制生物墨水的扩散,可以使用更广泛的粘度范围。作为概念验证,我们制备并表征了一种多材料支架,该支架包含聚(ε-己内酯)(PCL)作为热塑性聚合物和基于明胶的生物墨水。一种含有5 w/v%负载荧光白蛋白的聚(乳酸-共-乙醇酸)(PLGA)微粒或小鼠成纤维细胞(1×10细胞/mL)的7.5 w/v%甲基丙烯酰化明胶(GelMA)生物墨水在24°C下进行打印。与PCL对照支架相比,复合支架的结构在孔隙率或机械性能方面没有显著降低,这表明雕刻技术没有显著损害支架的机械或结构完整性。封装的PLGA微粒均匀分布在GelMA中,并在37°C下于PBS中孵育24小时后仍保留在支架中。此外,在孵育24小时后,证实了封装在GelMA生物墨水中并打印在PCL支架凹槽中的成纤维细胞的活力。总体而言,这项工作为制备结合了坚固热塑性结构和低粘度生物墨水的3D打印支架提供了一种新方法。

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