Effect of TRPC6 knockdown on puromycin aminonucleoside-induced podocyte injury.
10.1007/s11596-012-0059-x
- Author:
Xifeng SUN
1
;
Yongli CHU
;
Chun ZHANG
;
Xiyun DU
;
Fangfang HE
;
Shan CHEN
;
Pan GAO
;
Jianshe LIU
;
Zhonghua ZHU
;
Xianfang MENG
Author Information
1. Department of Nephrology, Huangzhong University of Science and Technology, Wuhan, China. sxfgh-1976@163.com
- Publication Type:Journal Article
- MeSH:
Animals;
Cell Membrane Permeability;
drug effects;
physiology;
Cell Survival;
drug effects;
physiology;
Cells, Cultured;
Gene Knockdown Techniques;
Mice;
Mice, Knockout;
Podocytes;
drug effects;
physiology;
Puromycin Aminonucleoside;
pharmacology;
TRPC Cation Channels;
genetics;
metabolism
- From:
Journal of Huazhong University of Science and Technology (Medical Sciences)
2012;32(3):340-345
- CountryChina
- Language:English
-
Abstract:
This study was aimed to construct eukaryotic expression vectors carrying the small hairpin RNA (shRNA) targeting TRPC6 gene and investigate the effect of TRPC6 knockdown on puromucin aminonucleoside (PAN)-induced podocyte injury. Two DNA sequences containing the small hairpin structure targeting TRPC6 were designed, synthesized and then inserted into the green fluorescence protein (GFP)-contained plasmids (pGC) to establish the plasmids pGCsi-TRPC6A and pGCsi-TRPC6B. Plasmids expressing scrambled shRNA were used as negative control and named pGCsi-NC. These plasmids were transfected into a conditionally immortalized murine podocyte cell line by using liposome. Flow cytometry was used to examine the transfection efficiency. TRPC6 mRNA and protein expression levels were detected by RT-PCR and Western blotting. Cultured podocytes were divided into four groups: control group, PAN treatment group, PAN+TRPC6 shRNA transfected group and PAN+scrambled shRNA transfected group. The paracelluar permeability to BSA was evaluated by Millicell-PCF Inserts and cell viability was measured by the trypan blue assay. Immunofluorescent assay was used to observe the distribution of α-actinin-4 and α-tubulin. The results showed that the transfection efficiency of the shRNA expression vector was about 45%. Expression levels of TRPC6 mRNA and protein were downregulated after transfection with pGCsi-TRPC6A and pGCsi-TRPC6B. Knocking down TRPC6 gene could effectively reverse the PAN-induced increase in the paracelluar permeability to BSA. The distribution of α-actinin-4 and α-tubulin was disrupted after treatment with PAN, which was reversed by knocking down TRPC6 gene. It was concluded that knocking down TRPC6 gene could effectively prevent podocytes from the permeability increase induced by PAN, which may be related to the regulation of podocyte cytoskeleton.
