Rotundo Robert F, Curtis Theresa M, Shah Melissa D, Gao Baochong, Mastrangelo Anthony, LaFlamme Susan E, Saba Thomas M
Department of Physiology and Cell Biology, Neil Hellman Medical Research Building, Albany Medical College, Albany, New York 12208, USA.
Am J Physiol Lung Cell Mol Physiol. 2002 Feb;282(2):L316-29. doi: 10.1152/ajplung.00145.2000.
Tumor necrosis factor-alpha (TNF-alpha) causes an increase in transendothelial protein permeability of confluent monolayers of calf pulmonary artery endothelial (CPAE) cells, and the addition of plasma fibronectin (pFn) to the culture medium can attenuate this increase in permeability. We determined if reduced integrin function had a role in decreased endothelial cell adhesion to immobilized Fn after exposure of the endothelial monolayers to TNF-alpha. TNF-alpha also causes a reorganization of the subendothelial Fn rich matrix and a significant loss in RGD-dependent adhesion of TNF-alpha treated CPAE cells to pFn coated surfaces. However, flow cytometry revealed no decrease in alpha(5)beta(1) or total beta(1) integrin expression on the surface of the CPAE cells after TNF-alpha. Reduced CPAE adhesion to immobilized Fn was, in part, due to a loss of beta(1)-integrin function since the beta(1)-integrin blocking antibody mAb 13 significantly (P < 0.05) prevented the adhesion of normal control CPAE cells but did not further reduce the adhesion of TNF-alpha-treated cells. In addition, antibodies which activate beta(1) integrins restored (P < 0.05) adhesion of TNF-alpha-treated cells to immobilized pFn but did not alter the adhesion of control cells. Despite reduced ability to adhere to immobilized Fn, TNF-alpha-treated CPAE monolayers demonstrated increased binding and incorporation of fluid-phase pFn into the subendothelial extracellular matrix (ECM) as measured by the analysis of the deoxycholate (DOC) detergent insoluble pool of (125)I-Fn in the cell layer. In contrast to the RGD-mediated adhesion of CPAE cells to matrix Fn, the increased binding of soluble pFn after TNF-alpha was not inhibited by RGD peptides or mAb 13. Thus reduced integrin-dependent adhesion of the CPAE cells to matrix Fn as well as disruption of the Fn matrix may contribute to the increased protein permeability of previously confluent endothelial monolayer after TNF-alpha. In addition, increased ability for the monolayer to incorporate fluid-phase Fn into the ECM after TNF-alpha via a non-beta(1)- integrin dependent mechanism may be a compensatory response to stabilize the Fn matrix and the endothelial barrier.
肿瘤坏死因子-α(TNF-α)可导致小牛肺动脉内皮(CPAE)细胞汇合单层的跨内皮蛋白通透性增加,而向培养基中添加血浆纤连蛋白(pFn)可减弱这种通透性增加。我们确定在内皮单层暴露于TNF-α后,整合素功能降低是否在减少内皮细胞对固定化Fn的黏附中起作用。TNF-α还会导致内皮下富含Fn的基质发生重组,并且TNF-α处理的CPAE细胞对pFn包被表面的RGD依赖性黏附显著丧失。然而,流式细胞术显示TNF-α处理后CPAE细胞表面的α(5)β(1)或总β(1)整合素表达没有降低。CPAE对固定化Fn的黏附减少部分是由于β(1)-整合素功能丧失,因为β(1)-整合素阻断抗体mAb 13显著(P < 0.05)阻止了正常对照CPAE细胞的黏附,但并未进一步降低TNF-α处理细胞的黏附。此外,激活β(1)整合素的抗体可恢复(P < 0.05)TNF-α处理细胞对固定化pFn的黏附,但不改变对照细胞的黏附。尽管黏附固定化Fn的能力降低,但通过分析细胞层中脱氧胆酸盐(DOC)去污剂不溶性池中的(125)I-Fn,发现TNF-α处理的CPAE单层显示出液相pFn与内皮下细胞外基质(ECM)的结合和掺入增加。与CPAE细胞对基质Fn的RGD介导黏附相反,TNF-α处理后可溶性pFn结合的增加不受RGD肽或mAb 13的抑制。因此,CPAE细胞对基质Fn的整合素依赖性黏附减少以及Fn基质的破坏可能导致TNF-α处理后先前汇合的内皮单层蛋白通透性增加。此外,TNF-α处理后单层通过非β(1)-整合素依赖性机制将液相Fn掺入ECM的能力增加可能是一种补偿反应,以稳定Fn基质和内皮屏障。
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