[肠毒素超抗原通过上调淋巴细胞趋化因子受体5诱导肺动脉内皮损伤]
[Induction of injury to endothelium of pulmonary artery due to entero superantigen by up regulation of lymphocyte chemokine receptor 5].
作者信息
Wu Li-Xiang, Xiao Zheng-Lun, Kong Tian-Han
机构信息
Intensive Care Unit, the First Affiliated Hospital of Jinan University, Guangzhou 510620, Guangdong, China.
出版信息
Zhongguo Wei Zhong Bing Ji Jiu Yi Xue. 2011 Apr;23(4):208-12.
OBJECTIVE
To observe the injurious effect of T cell activated by Staphylococcus enterotoxin B (SEB) on human pulmonary artery endothelial cell (HPAEC) and explore its possible mechanism.
METHODS
HPAEC was cocultured with SEB-activated T cells supernatant, and the secretion of chemotactic factors from HPAEC was examined. The Transwell inserts was used in chemoattraction assays. After HPAECs were cocultured with T cells and 10 ng/ml SEB for 3 days, HPAEC damage was monitored by microscopy and the terminal deoxynucleotidyl transferase mediated dUTP nick end labeling (TUNEL) assay.
RESULTS
Three kinds of tested chemokines showed a time dependent increase in all supernatant of HPAEC incubated with different concentrations of T cells. After 72 hours, the monocyte chemoattractant protein 1 (MCP 1, ng/ml) in 1×10(-2) , 1×10(-1), 1×10(0) T cell supernatant groups was 1.240±0.103, 4.200±0.305, 6.500±0.500, respectively, macrophage inflammatory protein 1α (MIP 1α, ng/ml) was 0.210±0.015, 0.287±0.012, 0.531±0.037, respectively , and Rantes (ng/ml) was 1.420±0.074, 7.634±0.630, 15.700±1.300, respectively. Rantes presented a two phase secretion mode: in early 6 hours it increased swiftly, but relatively slow at 12, 24, 48, 72 hours. T cell adherent to polycarbonate membrane increased after SEB stimulation in superantigen group compared with control group without SEB stimulation (86.38±14.50 vs. 16.50±2.50, P<0.01). When 10 ng/ml SEB-activated T cell was cocultured with HPAEC, more of originally suspended cultured T cells adhered to HPAEC monolayer [(15.50±1.08)% vs. (1.60±0.22)%, PP<0.01], whereas the cell adhesion ratio decreased markedly in 1 μg/ml Met Rantes group [(4.39±0.66)%, PP<0.01). FACs test of HPAEC adherent T cell showed lymphocyte chemokine receptor 5 (CCR5)/CD4 and CCR5/CD8 increased over 2.5 folds and 2.8 folds compared with 100 ng/ml SEB-activated T cell. Cell death rate of HPAEC was increased when cocultured with SEB-activated T cell in superantigen group compared with HPAEC normal incubation group [(32.50±4.50)% vs. (3.50±0.50)%, P<0.01].
CONCLUSION
Increased chemoattraction and adherence of SEB-activated T cells to HPAEC could damage HPAEC; this effect was possibly due to up regulation of CCR5 on T cell.
目的
观察金黄色葡萄球菌肠毒素B(SEB)激活的T细胞对人肺动脉内皮细胞(HPAEC)的损伤作用,并探讨其可能机制。
方法
将HPAEC与SEB激活的T细胞上清共培养,检测HPAEC趋化因子的分泌情况。采用Transwell小室进行趋化实验。HPAEC与T细胞及10 ng/ml SEB共培养3天后,通过显微镜观察及末端脱氧核苷酸转移酶介导的dUTP缺口末端标记(TUNEL)法监测HPAEC损伤情况。
结果
三种检测的趋化因子在与不同浓度T细胞共培养的HPAEC所有上清中均呈时间依赖性增加。72小时后,1×10(-2)、1×10(-1)、1×10(0) T细胞上清组中的单核细胞趋化蛋白1(MCP 1,ng/ml)分别为1.240±0.103、4.200±0.305、6.500±0.500,巨噬细胞炎性蛋白1α(MIP 1α,ng/ml)分别为0.210±0.015、0.287±0.012、0.531±0.037,调节激活正常T细胞表达和分泌的因子(Rantes,ng/ml)分别为1.420±0.074、7.634±0.630、15.700±1.300。Rantes呈现双相分泌模式:在最初6小时迅速增加,但在12、24、48、72小时相对缓慢。与未用SEB刺激的对照组相比,超抗原组经SEB刺激后T细胞黏附于聚碳酸酯膜的数量增加(86.38±14.50对16.50±2.5, P<0.01)。当10 ng/ml SEB激活的T细胞与HPAEC共培养时,更多原本悬浮培养的T细胞黏附于HPAEC单层[(15.50±1.08)%对(1.60±0.22)%,P<0.01],而在1 μg/ml Met Rantes组细胞黏附率显著降低[(4.39±0.66)%,P<×0.01]。对HPAEC黏附T细胞的流式细胞术检测显示,与100 ng/ml SEB激活的T细胞相比,淋巴细胞趋化因子受体5(CCR5)/CD4和CCR5/CD8增加超过2.5倍和2.8倍。与HPAEC正常培养组相比,超抗原组中与SEB激活的T细胞共培养时HPAEC的细胞死亡率增加[(32.50±4.50)%对(3.50±0.50)%,P<0.01]。
结论
SEB激活的T细胞对HPAEC趋化性和黏附性增加可损伤HPAEC;这种作用可能是由于T细胞上CCR5上调所致。
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