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Sox-9 促进脂肪组织来源的干细胞在体外向软骨细胞样表型分化。

Sox-9 facilitates differentiation of adipose tissue-derived stem cells into a chondrocyte-like phenotype in vitro.

机构信息

Department of Anesthesiology, University of Miami Miller School of Medicine, Miami, Florida 33136, USA.

出版信息

J Orthop Res. 2011 Aug;29(8):1291-7. doi: 10.1002/jor.21336. Epub 2011 Mar 11.

Abstract

The purpose of this study is to test whether ectopic expression of Sox-9 can induce adipose tissue-derived stem cells (ASCs) to function as real nucleus pulposus (NP) cells in vitro. Adenoviral vectors expressing Sox-9 were reported to infect the chondroblastic and human disc cells, which resulted in increased Sox-9 and type II collagen production. ASCs were isolated from rat inguinal adipose pad, characterized, and transduced in vitro with a retroviral vector encoding the Sox-9 gene. Sox-9-engineered ASCs (ASCs/Sox-9) were induced for the chondrocyte-like cell differentiation by 3D cultured in alginate beads and TGF-β3 for 2 weeks. Expression of exogenous Sox-9 protein was detected. Type II collagen and Aggrecan gene expressions of induced ASCs/Sox-9 were measured using real-time PCR; proteoglycans expressions were measured by checking the glycosaminoglycan content and type II collagen production by enzyme-linked immunosorbent assay. Isolated ASCs were CD 29(+) /CD44(+) /C-Kit(-) /Lin(-) /CD34(-) /CD45(-) . ASCs/Sox-9 expressed marked increase in exogenous Sox-9 protein. After induction, type II collagen gene expression was sevenfold higher in mRNA levels, with an approximately twofold increase in protein levels of ASCs/Sox-9 compared to ASCs. Type II collagen and proteoglycan productions were significantly increased in the ASCs/Sox-9 compared to the ASCs. In addition, co-culture of induced ASCs/Sox-9 with matured NP cells resulted in enhanced increase in proteoglycan and type II collagen production. Constitutive retroviral expression of Sox-9 could efficiently induce ASCs differentiation into chondrocyte-like cells. This novel approach may provide a practicable system for a simple and rapid differentiation of ASCs into chondrocyte-like cells which may be potentially used as a stem cell-based therapeutic tool for the treatment of degenerative disc diseases.

摘要

本研究旨在测试 Sox-9 的异位表达是否能使脂肪组织来源的干细胞(ASCs)在体外表现为真正的髓核(NP)细胞。已有报道称,腺病毒载体表达 Sox-9 能感染软骨细胞和人类椎间盘细胞,从而增加 Sox-9 和 II 型胶原的产生。ASCs 从大鼠腹股沟脂肪垫中分离出来,进行特征鉴定,然后用编码 Sox-9 基因的逆转录病毒载体进行体外转导。通过在藻酸盐珠中 3D 培养并添加 TGF-β3 诱导 Sox-9 工程化 ASCs(ASCs/Sox-9)向软骨细胞样细胞分化 2 周。检测外源性 Sox-9 蛋白的表达。使用实时 PCR 测量诱导的 ASCs/Sox-9 的 II 型胶原和 Aggrecan 基因表达;通过检查糖胺聚糖含量和酶联免疫吸附试验中的 II 型胶原产生来测量蛋白聚糖的表达。分离的 ASCs 为 CD29(+) / CD44(+) / C-Kit(-) / Lin(-) / CD34(-) / CD45(-) 。ASCs/Sox-9 表达明显增加的外源性 Sox-9 蛋白。诱导后,II 型胶原基因表达在 mRNA 水平上提高了 7 倍,与 ASCs 相比,ASCs/Sox-9 的蛋白水平提高了约 2 倍。与 ASCs 相比,ASCs/Sox-9 的 II 型胶原和蛋白聚糖产生明显增加。此外,诱导的 ASCs/Sox-9 与成熟 NP 细胞的共培养导致蛋白聚糖和 II 型胶原产生的增强增加。Sox-9 的组成型逆转录病毒表达能有效地诱导 ASCs 分化为软骨细胞样细胞。这种新方法可能为 ASCs 向软骨细胞样细胞的简单快速分化提供一种可行的系统,可能作为一种基于干细胞的治疗退行性椎间盘疾病的治疗工具。

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