Preparation and characterization of laser microporous acellular osteochondral scaffolds

Xue-jian Liu; Shi-chen Liu; Bai-chuan Sun; Kai-hong Zhang; Hao-ye Meng; Yu Wang; Shao-dai Huang; Chang-feng LU; Chong Wang; Wen YU; Xiao-guang Jing; Yue Zhao; Jian-hua Yang; Jiang Peng

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Preparation and characterization of laser microporous acellular osteochondral scaffolds

VernacularTitle:激光微孔化脱细胞骨软骨支架的制备及表征
Author: Xue-Jian LIU ¹ ; Shi-Chen LIU ; Bai-Chuan SUN ; Kai-Hong ZHANG ; Hao-Ye MENG ; Yu WANG ; Shao-Dai HUANG ; Chang-Feng LU ; Chong WANG ; Wen YU ; Xiao-Guang JING ; Yue ZHAO ; Jian-Hua YANG ; Jiang PENG
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1. 佳木斯大学
From: Chinese Journal of Tissue Engineering Research 2018;22(18):2836-2842
CountryChina
Language:Chinese
Abstract: BACKGROUND: Preparing a scaffold with cartilage derived components and good initial mechanical strength is the direction of tissue engineering cartilage research. OBJECTIVE: To prepare porous acellular osteochondral scaffolds, and to explore their mechanical properties and cell compatibility. METHODS: Osteochondral bone from the porcine knee joint was taken, and then porous osteochondral scaffolds were made by laser microporation technology. Subsequently, the scaffolds were decellularized chemical methods. Scaffold structure was observed by scanning electron microscopy, and the compression modulus of the scaffolds was determined. Bone marrow mesenchymal stem cells were cultured in L-DMEM containing 10% fetal bovine serum (control group) and cultured in the medium extract of porous acellular osteochondral scaffolds (experimental group), respectively. Cell proliferation was detected by cell counting kit-8 method within 5 days of culture. Bone marrow mesenchymal stem cells were seeded on the porous acellular osteochondral scaffolds, and within 28 days of co-culture, cell growth was observed by hematoxylin-eosin staining and toluidine blue staining. RESULTS AND CONCLUSION: (1) Observation under scanning electron microscopy: The porous acellular osteochondral scaffolds had the smooth surface with evenly distributed pores. The pores of the scaffold extended longitudinally into the subchondral bone. (2) Mechanical properties: The average compressive modulus of porous acellular osteochondral scaffolds was 0.77 MPa, which was close to the compression modulus of the normal cartilage (1.15 MPa). (3) Cell counting kit-8 test: There were no differences in cell proliferation between the control and experimental groups at 1, 2, 3, 4 and 5 days of culture. (4) Cell-scaffold co-culture: A large amount of bone marrow mesenchymal stem cells were observed to be adherent to the scaffold after 1 day of culture through hematoxylin-eosin and toluidine blue staining. However, as time went on, a few cells adhered to the pore wall or grew into the pores at 7 and 21 days of culture. There were also some adherent cells but a large amount of cell masses formed in the pores at 28 days of culture. To conclude, the porous acellular osteochondral scaffold has good mechanical properties and cell compatibility.