›› 2009, Vol. 40 ›› Issue (1): 20-24.doi: 10.3969/j.issn.0529-1356.2009.01.004
• 肿瘤基础研究专题报道 • 上一篇 下一篇
孙璐; 陈晋峰 ;王嘉; 赵威; 杨跃*
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关键词: Thy-1, 肺癌, A549细胞, 细胞迁移, 载体构建, 基因芯片, Transwell, 反转录-聚合酶链式反应, 人
Abstract: Objective To investigate the function of Thy-1 gene, especially its possible roles in the migration of A549 cells as well as the possible mechanisms by which it works. Methods Construct recombinant expression plasmid vector of pcDNA3.0-Thy-1 and transfected it into A549 cells. These cell lines were further studied for the exogenous Thy-1 mRNA expression by RT-PCR and expression of endogenous Thy-1 protein by immunofluorescence assay. Then the transwell cell migrations were assayed. In order to study the possible mechanisms by which Thy-1 influences the invasiveness potential, microarray were used to screen out cell migrations associated genes. Results Eukaryotic expression vector pcDNA3.0-Thy-1 was constructed; Stable Thy-1 expressing cell line were established; Transwell assay showed that over expression of Thy-1 in A549 cell line resulted in reduced ability of cell migration (EM>P/EM><0.0001); and microarray suggested that the Thy-1 gene could influenced the expression level of 25 cell motility-related genes. In these genes, 11 genes expressions were up regulated, and 14 genes were down regulated. These results could be consistent when microarray and RT-PCR methods were used to detect the difference of gene expression.Conclusion Overexpression of Thy-1 leads to a less invasive phenotype of A549 cells and changes the expression level of many cell motility-related genes. This suggested that Thy-1 expression patterns in lung cancer tissue may be associated with the invasiveness of non-small cell lung cancer.
Key words: Thy-1, Lung cancer, A549 cell, Cell motility, Construction of vector, Microarray, Transwell, RT-PCR, Human
中图分类号:
R734
孙璐;陈晋峰;王嘉;赵威;杨跃. Thy-1表达水平对肺腺癌细胞A549迁移性及部分相关基因表达的影响[J]. , 2009, 40(1): 20-24.
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链接本文: https://jpxb.bjmu.edu.cn/CN/10.3969/j.issn.0529-1356.2009.01.004
https://jpxb.bjmu.edu.cn/CN/Y2009/V40/I1/20
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