World Journal of Emergency Medicine ›› 2014, Vol. 5 ›› Issue (2): 122-127.doi: 10.5847/wjem.j.issn.1920-8642.2014.02.008
• Original Articles • Previous Articles Next Articles
Pei-ren Shan, Wei-wei Xu, Zhou-qing Huang, Jun Pu, Wei-jian Huang()
Received:
2013-10-11
Accepted:
2014-03-06
Online:
2014-06-15
Published:
2014-06-15
Contact:
Wei-jian Huang
E-mail:weijianhuang69@126.com
Pei-ren Shan, Wei-wei Xu, Zhou-qing Huang, Jun Pu, Wei-jian Huang. Protective role of retinoid X receptor in H9c2 cardiomyocytes from hypoxia/reoxygenation injury in rats[J]. World Journal of Emergency Medicine, 2014, 5(2): 122-127.
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URL: http://wjem.com.cn//EN/10.5847/wjem.j.issn.1920-8642.2014.02.008
Figure 1.
Activating RXR suppressed H/R-induced myocardial cell apoptosis by flow cytometric analysis with JC-1 assay (n=6, mean±SD). A: The percentage of apoptotic cells was determined by calculating the ratio of JC-1 green-stained cells (LR) to total cells. B: All data were expressed by the bar graph showing means±standard deviation (n=6); compared with the control group, *P<0.01; compared with the H/R group, #P<0.01; compared with the RA group, ΔP<0.01.
Figure 2.
Activation of RXR stabled H/R injury-induced ΔΨm in myocardial cells. A: The cells were stained with JC-1 and visualized by a fluorescence microscope. The regions of high mitochondrial membrane polarization are indicated by red fluorescence due to J-aggregate formation by concentrated dye. The regions of reduced polarization are indicated by the green fluorescence of JC-1 monomers. B: ΔΨm was monitored using JC-1, by flow cytometry. The excitation wave length was 488 nm. The emission fluorescence was monitored at 530 nm with green fluorescence (left panel) and 585 nm with red fluorescence (right panel). C: Mitochondrial transmembrane potential was expressed as red/green fluorescence intensity ratio (n=6); compared with the control group, *P<0.01; compared with the H/R group, #P<0.01; compared with the RA group, ΔP<0.01.
Figure 3.
Activation of RXR inhibited the H/R-induced mitochondrial apoptosis pathway (n=3, x- ±s). A: Western blot analysis of Bcl-2/Bax and cleaved caspase 9 protein was performed in cultured rat H9c2 cardiomyocytes. B: Scanning densitometry was used for semiquantitative analysis of the expression level of Bcl-2/Bax and cleaved caspase 9 protein; compared with the control group, *P<0.01; compared with the H/R group, #P<0.01; compared with the RA group, ΔP<0.01.
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