稳定敲低MYH10基因细胞株的建立

目的 构建稳定敲低MYH10基因的COS-7细胞株。方法 在293TX细胞中进行病毒的包装,用获得的高效价慢病毒感染COS-7细胞,通过免疫印迹和荧光显微镜,检测病毒感染后COS-7细胞MYH10蛋白表达的变化。结果 在构建的两种重组质粒中,MYH10-lentiviral shRNA-2在转染后表现出明显的干扰作用,感染后能明显下调COS-7细胞的MYH10蛋白表达。结论 病毒感染的COS-7细胞可明显抑制COS-7细胞内源MYH10的表达,说明了稳定敲低MYH10基因的COS-7细胞株的建立,为进一步研究MYH10在相关疾病中的功能奠定了基础。

Establishment of Stable COS-7 Cell Strain with MYH10-knock-down.

Objective To establish COS-7 cell strain stable knockdown of MYH10 gene. Methods The lentiviral plasmids were transfected into 293TX cells to package into lentiviral particles. Then COS-7 cells was transduced with the lentiviral particles. Western blot and fluorescence microscope were carried out to analyze the suppression of MYH10 in COS-7 Cells. Results In the construction of two recombinant plasmid, MYH10-lentiviral shRNA-2 showed significant interference after transfection, and can obviously reduced expression of MYH10 in COS-7 cells. Conclusion Infected COS-7 cells can inhibit the expression of the MYH10 COS-7 cells, indicating that a stable COS-7 cell strain has been successively established.