Yu Chuanhui, Kastin Abba J, Pan Weihong
Pennington Biomedical Research Center, Baton Rouge, Louisiana 70808, USA.
J Cell Physiol. 2007 Oct;213(1):161-6. doi: 10.1002/jcp.21105.
To examine how the proinflammatory cytokine tumor necrosis factor alpha (TNF) modulates the response of cerebral microvessels to other cytokines, we used rat cerebral microvessel endothelial RBE4 cells to simulate the in vitro blood-brain barrier (BBB). The gp130 receptor, which is shared by the interleukin (IL)-6 family of cytokines, showed specific upregulation by TNF. TNF treatment (5 ng/ml for 30 min to 24 h) increased gp130 at both the levels of transcription and protein expression. The stability of gp130 protein was mediated by NFkappaB activity, as the inhibitors quinazoline and MG132 not only blocked the increase induced by 6 h of TNF treatment, but also reduced its basal level of expression. By contrast, the lysosomal inhibitor chloroquine and the extracellular regulated kinase inhibitor U0126 showed no effect. Despite the increase of gp130, TNF caused a significant reduction in the cell binding and endocytosis of leukemia inhibitory factor (LIF), another proinflammatory cytokine that binds to the gp130 co-receptor and its unique gp190 receptor. This is consistent with our previous findings that TNF reduces gp190 expression and Stat3 activation. Thus, TNF stimulation results in decreased responsiveness of RBE4 cells to LIF, indicating complex regulatory interactions of cytokines at the BBB.
为了研究促炎细胞因子肿瘤坏死因子α(TNF)如何调节脑微血管对其他细胞因子的反应,我们使用大鼠脑微血管内皮RBE4细胞来模拟体外血脑屏障(BBB)。白细胞介素(IL)-6细胞因子家族共有的gp130受体显示出被TNF特异性上调。TNF处理(5 ng/ml,处理30分钟至24小时)在转录和蛋白质表达水平上均增加了gp130。gp130蛋白的稳定性由NFκB活性介导,因为抑制剂喹唑啉和MG132不仅阻断了TNF处理6小时诱导的增加,还降低了其基础表达水平。相比之下,溶酶体抑制剂氯喹和细胞外调节激酶抑制剂U0126没有效果。尽管gp130增加,但TNF导致白血病抑制因子(LIF)的细胞结合和内吞作用显著降低,LIF是另一种与gp130共受体及其独特的gp190受体结合的促炎细胞因子。这与我们之前的发现一致,即TNF降低gp190表达和Stat3激活。因此,TNF刺激导致RBE4细胞对LIF的反应性降低,表明细胞因子在血脑屏障处存在复杂的调节相互作用。
