小鼠肾脏足细胞的原代培养和鉴定

doi:10.13481/j.1671-587x.20170137

Abstract

Abstract:

Objective: To establish a good operability, simple and efficient mouse kidney cell separation and primary culture model, and to lay the foundation for further study.Methods: The murine kidney tissues were collected and the glomeruli with different size combination of screening were obtained. The isolated glomeruli were suspensioned in KI-3T3 medium, then subsided in the medium cell with rat tail collagen. The glomeruli were refreshed 4 d after cultivation. 7 d after cultivation, the glomeruli were resolved by trypsin and the podocyts were cultured. The podocytes were generated at 5-7 d. The podocytes were analyzed after 2-3 generations. The morphology of podocytes of kidney tissue of the mice was observed by inverted phase contract microscope.The expressions of nephrin,podocin and P-cadherin in the podocytes of kidney tissue of the mice were detected by PCR.Results: The podocytes began to remove from the planted glomeruli at the 3th day. After 7 d of generation, the cultured podocytes showed microvilli and process.The PCR results showed that the podocytes expressed nephrin,podocin, and P-cadherin.Conclusion: The difference sifting technology combined with enzyme digestion could successfully isolate and culture the C57/BL6J mouse podocytes in vitro.

Key words: kidney, podocyte, primary culture

CLC Number:

Q813.11

GAO Xia, LEI Xiaoyan, LIU Shurao, SUO Yanhong, CAO Xiaofeng, GAO Mingdong. Primary culture and identification of mouse kidney cells[J].Journal of Jilin University Medicine Edition, 2017, 43(01): 186-189.

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Primary culture and identification of mouse kidney cells

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