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具有增强细胞浸润和增殖能力的双重孔隙蛋白支架。

Dual Porosity Protein-based Scaffolds with Enhanced Cell Infiltration and Proliferation.

机构信息

Marquette University School of Dentistry, Milwaukee, WI, USA.

Division of Pharmaceutical Sciences, School of Pharmacy, University of Wisconsin-Madison, Madison, WI, USA.

出版信息

Sci Rep. 2018 Oct 5;8(1):14889. doi: 10.1038/s41598-018-33245-w.

Abstract

3D dual porosity protein-based scaffolds have been developed using the combination of foaming and freeze-drying. The suggested approach leads to the production of large, highly porous scaffolds with negligible shrinkage and deformation compared to the conventional freeze-drying method. Scanning electron microscopy, standard histological processing and mercury intrusion porosimetry confirmed the formation of a dual network in the form of big primary pores (243 ± 14 µm) embracing smaller secondary pores (42 ± 3 µm) opened onto their surface, resembling a vascular network. High interconnectivity of the pores, confirmed by micro-CT, is shown to improve diffusion kinetics and support a relatively uniform distribution of isolated human dental pulp stem cells within the scaffold compared to conventional scaffolds. Dual network scaffolds indicate more than three times as high cell proliferation capability as conventional scaffolds in 14 days.

摘要

3D 双重孔隙蛋白基支架采用发泡和冷冻干燥相结合的方法开发。与传统的冷冻干燥方法相比,所提出的方法可生产出大尺寸、高多孔的支架,几乎没有收缩和变形。扫描电子显微镜、标准组织学处理和压汞法证实了双重网络的形成,其形式为大的初级孔(243±14μm),包含较小的次级孔(42±3μm),表面开放,类似于血管网络。通过微 CT 证实了孔的高连通性,这有利于改善扩散动力学,并与传统支架相比,支持分离的人牙髓干细胞在支架内相对均匀地分布。双重网络支架在 14 天内的细胞增殖能力比传统支架高三倍以上。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0c9f/6173780/89c2d761a50c/41598_2018_33245_Fig1_HTML.jpg

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