The effects of inflammatory cytokines on lymphatic endothelial barrier function

被引:109
作者
Cromer, Walter E. [1 ]
Zawieja, Scott D. [1 ]
Tharakan, Binu [2 ]
Childs, Ed W. [3 ]
Newell, M. Karen [2 ]
Zawieja, David C. [1 ]
机构
[1] Texas A&M HSC, Dept Syst Biol & Translat Med, College Stn, TX 77843 USA
[2] Texas A&M HSC, Scott & White, Dept Surg, Temple, TX USA
[3] Morehouse Sch Med, Dept Surg, Atlanta, GA 30310 USA
关键词
Lymphatic; Endothelial; Permeability; Cytokines; Barrier; NITRIC-OXIDE; IN-VITRO; BETA-CATENIN; VASCULAR-PERMEABILITY; MOLECULAR CONTROL; CELL; VEGF; NO; DYSFUNCTION; EXPRESSION;
D O I
10.1007/s10456-013-9393-2
中图分类号
R6 [外科学];
学科分类号
1002 ; 100210 ;
摘要
Proper lymphatic function is necessary for the transport of fluids, macromolecules, antigens and immune cells out of the interstitium. The lymphatic endothelium plays important roles in the modulation of lymphatic contractile activity and lymph transport, but it's role as a barrier between the lymph and interstitial compartments is less well understood. Alterations in lymphatic function have long been associated with edema and inflammation although the integrity of the lymphatic endothelial barrier during inflammation is not well-defined. In this paper we evaluated the integrity of the lymphatic barrier in response to inflammatory stimuli commonly associated with increased blood endothelial permeability. We utilized in vitro assays of lymphatic endothelial cell (LEC) monolayer barrier function after treatment with different inflammatory cytokines and signaling molecules including TNF-alpha, IL-6, IL-1 beta, IFN-gamma and LPS. Moderate increases in an index of monolayer barrier dysfunction were noted with all treatments (20-60 % increase) except IFN-gamma which caused a greater than 2.5-fold increase. Cytokine-induced barrier dysfunction was blocked or reduced by the addition of LNAME, except for IL-1 beta and LPS treatments, suggesting a regulatory role for nitric oxide. The decreased LEC barrier was associated with modulation of both intercellular adhesion and intracellular cytoskeletal activation. Cytokine treatments reduced the expression of VE-cadherin and increased scavenging of beta-catenin in the LECs and this was partially reversed by LNAME. Likewise the phosphorylation of myosin light chain 20 at the regulatory serine 19 site, which accompanied the elevated monolayer barrier dysfunction in response to cytokine treatment, was also blunted by LNAME application. This suggests that the lymphatic barrier is regulated during inflammation and that certain inflammatory signals may induce large increases in permeability.
引用
收藏
页码:395 / 406
页数:12
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