Beeren I A O, Dos Santos G, Dijkstra P J, Mota C, Bauer J, Ferreira H, Reis Rui L, Neves N, Camarero-Espinosa S, Baker M B, Moroni L
Department of Complex Tissue Regeneration, MERLN Institute for Technology-Inspired Regenerative Medicine, Maastricht University, 6229 ER Maastricht, The Netherlands.
3B's Research Group, I3Bs - Research Institute on Biomaterials, Biodegradables and Biomimetics, Headquarters of the European Institute of Excellence on Tissue Engineering and Regenerative Medicine, University of Minho, AvePark, Zona Industrial da Gandra, 4805-017 Barco, Guimarães, Portugal.
Biodes Manuf. 2024;7(3):277-291. doi: 10.1007/s42242-024-00286-2. Epub 2024 May 20.
Melt extrusion-based additive manufacturing (ME-AM) is a promising technique to fabricate porous scaffolds for tissue engineering applications. However, most synthetic semicrystalline polymers do not possess the intrinsic biological activity required to control cell fate. Grafting of biomolecules on polymeric surfaces of AM scaffolds enhances the bioactivity of a construct; however, there are limited strategies available to control the surface density. Here, we report a strategy to tune the surface density of bioactive groups by blending a low molecular weight poly(ε-caprolactone) (PCL) containing orthogonally reactive azide groups with an unfunctionalized high molecular weight PCL at different ratios. Stable porous three-dimensional (3D) scaffolds were then fabricated using a high weight percentage (75 wt.%) of the low molecular weight PCL. As a proof-of-concept test, we prepared films of three different mass ratios of low and high molecular weight polymers with a thermopress and reacted with an alkynated fluorescent model compound on the surface, yielding a density of 201-561 pmol/cm. Subsequently, a bone morphogenetic protein 2 (BMP-2)-derived peptide was grafted onto the films comprising different blend compositions, and the effect of peptide surface density on the osteogenic differentiation of human mesenchymal stromal cells (hMSCs) was assessed. After two weeks of culturing in a basic medium, cells expressed higher levels of BMP receptor II (BMPRII) on films with the conjugated peptide. In addition, we found that alkaline phosphatase activity was only significantly enhanced on films containing the highest peptide density (i.e., 561 pmol/cm), indicating the importance of the surface density. Taken together, these results emphasize that the density of surface peptides on cell differentiation must be considered at the cell-material interface. Moreover, we have presented a viable strategy for ME-AM community that desires to tune the bulk and surface functionality via blending of (modified) polymers. Furthermore, the use of alkyne-azide "click" chemistry enables spatial control over bioconjugation of many tissue-specific moieties, making this approach a versatile strategy for tissue engineering applications.
The online version contains supplementary material available at 10.1007/s42242-024-00286-2.
基于熔融挤出的增材制造(ME-AM)是一种用于制造组织工程应用多孔支架的有前途的技术。然而,大多数合成半结晶聚合物不具备控制细胞命运所需的内在生物活性。在增材制造支架的聚合物表面接枝生物分子可增强构建体的生物活性;然而,控制表面密度的策略有限。在此,我们报告一种策略,通过将含有正交反应性叠氮基团的低分子量聚(ε-己内酯)(PCL)与未官能化的高分子量PCL以不同比例混合来调节生物活性基团的表面密度。然后使用高重量百分比(75 wt.%)的低分子量PCL制造稳定的多孔三维(3D)支架。作为概念验证测试,我们用热压机制备了三种不同质量比的低分子量和高分子量聚合物的薄膜,并使其与表面的炔基化荧光模型化合物反应,得到的密度为201 - 561 pmol/cm。随后,将骨形态发生蛋白2(BMP-2)衍生的肽接枝到包含不同共混组成的薄膜上,并评估肽表面密度对人间充质基质细胞(hMSCs)成骨分化的影响。在基础培养基中培养两周后,细胞在含有共轭肽的薄膜上表达更高水平的BMP受体II(BMPRII)。此外,我们发现碱性磷酸酶活性仅在含有最高肽密度(即561 pmol/cm)的薄膜上显著增强,表明表面密度的重要性。综上所述,这些结果强调在细胞 - 材料界面必须考虑表面肽密度对细胞分化的影响。此外,我们为希望通过(改性)聚合物共混来调节本体和表面功能的ME-AM领域提出了一种可行的策略。此外,炔基 - 叠氮“点击”化学的使用能够对许多组织特异性部分的生物共轭进行空间控制,使这种方法成为组织工程应用的通用策略。
在线版本包含可在10.1007/s42242-024-00286-2获取的补充材料。
Zotero 插件
