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| 真核表达人Wnt7b基因建立软骨细胞退变模型 | |
| 引用本文: | 王小军,张浩,郑杰,庞坚,曹月龙,詹红生,丁道芳.真核表达人Wnt7b基因建立软骨细胞退变模型[J].南方医科大学学报,2015,35(3):370-374. |
| 作者姓名: | 王小军 张浩 郑杰 庞坚 曹月龙 詹红生 丁道芳 |
| 作者单位: | 浙江中医药大学附属湖州市中医院;上海吉凯基因化学技术有限公司;上海中医药大学附属曙光医院石氏伤科医学中心;上海市中医药研究院骨伤科研究所 |
| 基金项目: | 国家自然科学基金(81073114,81072830);上海市教委创新项目(11YZ64);上海市高校青年教师培养资助计划(ZZszy12017)~~ |
| 摘 要: | 目的在真核细胞中表达人Wnt7b基因并且观察对大鼠原代软骨细胞的退变作用。方法取出生24 h SD大鼠关节处软 骨,Ⅱ型胶原酶多次消化后获得原代软骨细胞,取P1 代细胞进行实验。扩增人Wnt7b 基因及克隆至PCDH-GFP 上,转染 PCDH-GFP和PCDH-Wnt7b 至293ft 细胞中,48 h 后收集细胞上清及转染细胞,Western blot 鉴定Wnt7b 在293ft 细胞中的表 达。收集的上清分别稀释10倍和50倍培养大鼠软骨细胞,24 h后观察细胞形态并收集细胞蛋白和抽提RNA,Western blot和定 量PCR检测软骨退变指标MMP13、MMP3、Ⅱ型胶原、A-can、ADAMTS5、ColⅩ和SOX9的表达。结果成功克隆人Wnt7b基 因至PCDH-GFP载体上且在293ft细胞中得到有效表达。含Wnt7b培养基干预软骨细胞24 h后,软骨细胞形态由原来的多角形 变成长梭形,Wnt7b处理组软骨细胞MMP13和MMP3表达显著上调,Ⅱ型胶原的表达下调。PCR结果表明A-can和Sox9表达 下降,ColⅩ和ADAMTS5表达增强。结论有效在真核细胞中表达Wnt7b基因并且促进大鼠软骨细胞退变,建立软骨细胞退变 的体外模型。 |
| 关 键 词: | Wnt7b基因 293ft细胞 软骨细胞 转染 细胞退变 |
Establishment of a chondrocyte degeneration model by over-expression of human Wnt7bgene in 293ft cell line |
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| WANG Xiaojun;ZHANG Hao;ZHENG jie;ZHENG yuxin;CAO Yuelong;ZHAN Hongsheng;SHI Yinyu;DING Daofang.Establishment of a chondrocyte degeneration model by over-expression of human Wnt7bgene in 293ft cell line[J].Journal of Southern Medical University,2015,35(3):370-374. | |
| Authors: | WANG Xiaojun;ZHANG Hao;ZHENG jie;ZHENG yuxin;CAO Yuelong;ZHAN Hongsheng;SHI Yinyu;DING Daofang |
| Institution: | WANG Xiaojun;ZHANG Hao;ZHENG jie;ZHENG yuxin;CAO Yuelong;ZHAN Hongsheng;SHI Yinyu;DING Daofang;Huzhou Hospital of TCM Affiliated to Zhejing Chinese Medical University;Shanghai Genechem Co.Ltd;Shi’s Center of Orthopedics and Traumatology, Shuguang Hospital Affiliated to Shanghai University of TCM;Institute of Traumatology and Orthopedics, Shanghai Academy of Traditional Chinese Medicine; |
| Abstract: | Objective To investigate the role of human Wnt7b gene in rat chondrocyte degeneration. Methods Wnt7b gene obtained by PCR was cloned to PCDH-GFP. 293ft cell line was transfected with PCDH-GFP and PCDH-Wnt7b, and the supernatant and transfected cells were collected. The expression level of Wnt7b in 293ft cells was detected by Western blotting. The first passage of chondrocytes were isolated from articular cartilages of newborn born (within 24 h) SD rats were cultured in the supernatants from the transfected cells (at 10- and 50-fold dilutions). The cell morphology of the rat chondrocytes was observed under inverted microscope, and the protein expressions of MMP13, MMP3 and type II collagen and mRNA expressions of A-can, ADAMTS5, Col X and Sox9 were examined by Western blotting or real-time PCR. Results Human Wnt7b gene cloned to PCDH-GFP was expressed efficiently in 293ft cell line. Rat chndrocytes cultured for 24 h in the supernatants from PCDH-Wnt7b-transfected 293ft cells underwent changes from a polygonal to a spindle-shaped morphology. The protein expression levels of MMP13 and MMP3 increased while type II collagen decreased significantly, and the mRNA levels of A-can and Sox9 were down-regulated while Col X and ADMATS5 up-regulated in ratchondrocytes after incubation in supernatants from PCDH-Wnt7b-transfected 293ft cells. Conclusion Human Wnt7b gene can be expressed efficiently in 293ft cell line and can induce rat chondrocyte degeneration in vitro. |
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