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在丝素海绵和搅拌室中培养的同种异体软骨细胞移植以促进软骨再生。

Transplantation of allogeneic chondrocytes cultured in fibroin sponge and stirring chamber to promote cartilage regeneration.

作者信息

Shangkai Chueh, Naohide Tomita, Koji Yamamoto, Yasuji Harada, Masaaki Nakajima, Tomohiro Terao, Yasushi Tamada

机构信息

Graduate School of Medicine, Kyoto University, Yoshida-Konoe-cho, Sakyo-ku, Kyoto, Japan.

出版信息

Tissue Eng. 2007 Mar;13(3):483-92. doi: 10.1089/ten.2006.0181.

Abstract

Cartilage regeneration using a fibroin sponge and a stirring chamber was investigated to improve the potential of articular cartilage tissue engineering. Chondrocytes seeded on the fibroin-sponge scaffolds were cultured in the stirring chamber (a bioreactor facilitating mechanical stimulation) for up to 3 weeks. Changes in DNA content, glycosaminoglycan (GAG) amount, integrin subunits alpha5 and beta1 fluorescence intensity, and morphologic appearance, were studied to evaluate tissue maturity. Seeded scaffolds subjected to the stirring chamber demonstrated significant increases in both DNA content (38.9%) and GAG content (54.3%) at day 21 compared to the control group. In addition, the stirring chamber system facilitated a maturation of cartilage tissue showed by histologic examination, after a staining of proteoglycan and type II collagen. Clinical feasibility of the fibroin and stirring chamber system was evaluated using rabbit models with cartilage defect. Large defects on rabbit knee joints were repaired with regenerated cartilage, which resembles hyaline cartilage at 12 weeks after operation. These studies demonstrated the potential of such mechanically stimulated scaffold/cell constructs to support chondrogenesis in vivo.

摘要

为提高关节软骨组织工程的潜能,对使用丝素海绵和搅拌室进行软骨再生展开了研究。接种在丝素海绵支架上的软骨细胞在搅拌室(一种便于机械刺激的生物反应器)中培养长达3周。研究了DNA含量、糖胺聚糖(GAG)量、整合素亚基α5和β1荧光强度以及形态外观的变化,以评估组织成熟度。与对照组相比,置于搅拌室的接种支架在第21天时DNA含量(38.9%)和GAG含量(54.3%)均显著增加。此外,经蛋白聚糖和II型胶原染色后的组织学检查显示,搅拌室系统促进了软骨组织的成熟。使用兔软骨缺损模型评估了丝素和搅拌室系统的临床可行性。兔膝关节的大缺损用再生软骨修复,术后12周时再生软骨类似于透明软骨。这些研究证明了这种经机械刺激的支架/细胞构建体在体内支持软骨形成的潜能。

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