Aluminum-induced impairment in primary cultured rat choroid plexus epithelial cells
10.3760/cma.j.issn.1001-9391.2016.04.012
- VernacularTitle:铝对大鼠原代脉络丛上皮细胞的损伤作用
- Author:
Yaxian PANG
1
;
Xiaohong WU
;
Jianping CHEN
;
Hengying QIU
;
Qiao NIU
;
Qinli ZHANG
Author Information
1. 山西医科大学公共卫生学院劳动卫生教研室
- Keywords:
Rats;
Choroid plexus;
Epithelial cells;
Reactive oxygen species;
Superoxide dismutase
- From:
Chinese Journal of Industrial Hygiene and Occupational Diseases
2016;34(4):286-290
- CountryChina
- Language:Chinese
-
Abstract:
Objective To investigate the impairment in primary cultured rat choroid plexus epithelial cells (CPECs) induced by aluminum.Methods The choroid plexus isolated from Sprague-Dawley rats 14 days old was cut into pieces and digested by trypsin in the sterile area.The obtained single cells were cultured in DMEM with 1% epidermal growth factor and 20% fetal calf serum.Five days later,immunohistochemistry with anti-transthyretin antibody was used to identify the purity of cultured cells.The well-grown cells were treated with aluminum lactate at different concentrations (0,100,400,and 1 600 μmol/L for control,low-dose,medium-dose,and high-dose groups).Forty-eight hours later,the cell viability,apoptotic rate,level of reactive oxygen species (ROS),and activity of superoxide dismutase (SOD) were measured in each group to evaluate the impairment in primary cultured rat CPECs by aluminum.Results More than 95% of the cultured cells were identified as CPECs.The medium-and high-dose groups had significantly lower cell viability than the control group (86.74%±4.03% vs 100%,P<0.01;81.90%±9.17% vs 100%,P<0.01).The high-dose group had significantly lower cell viability than the low-dose group (81.90%±9.17% vs 92.92%±8.81%,P<0.01).The medium-and high-dose groups had significantly higher apoptotic rates than the control group (7.26%±0.99% vs 1.29%±0.03%,P<0.01;22.25%±1.55% vs 1.29%±0.03%,P<0.01) and the low-dose group (7.26%±0.99% vs 1.68%±0.27%,P<0.01;22.25%±1.55% vs 1.68%±0.27%,P<0.01).The high-dose group had a significantly higher apoptotic rate than the medium-dose group(22.25%±1.55% vs 7.26%±0.99%,P<0.01).The medium-and high-dose groups had significantly higher fluorescence intensity of ROS than the control group (22.23%±0.41% vs 17.24%±0.09%,P<0.05;25.10%±1.13% vs 17.24%±0.09%,P<0.05) and the low-dose group (22.23%± 0.41% vs 18.31%±0.21%,P<0.05;25.10%±1.13% vs 18.31%±0.21%,P<0.05).The high-dose group had significantly higher fluorescence intensity of ROS than the medium-dose group (25.10%±1.13% vs 22.23%± 0.41%,P<0.05).The low-,medium-and high-dose groups had significantly lower SOD activity than the control group[(28.65±0.74) U/g Hb vs (37.35±1.05) U/g Hb,P<0.05;(22.75±1.94) U/g Hb vs (37.35±1.05) U/g Hb,P<0.05;(13.29 ±0.64) U/g Hb vs (37.35 ± 1.05) U/g Hb,P<0.05].The medium-and high-dose groups had significantly lower SOD activity than the low-dose group [(22.75±1.94) U/g Hb vs (28.65±0.74) U/g Hb,P< 0.05;(13.29±0.64) U/g Hb vs (28.65±0.74) U/g Hb,P<0.05],while the high-dose group had had significantly lower SOD activity than the medium-dose group[(13.29±0.64) U/g Hb vs (22.75±1.94) U/g Hb,P<0.05].There were no significant differences in cell viability,apoptotic rate,level of ROS,or activity of SOD between any other two groups (P>0.05).Conclusion Aluminum lactate may induce impairment in primary cultured rat CPECs.It reduces the cell viability,elevates the apoptotic rate,and causes oxidative stress.
