Regulation of p38MAPK-mediated dendritic cell functions by the deubiquitylase otubain 1

被引:8
|
作者
Nguyen Thi Xuan [1 ,2 ]
Do Minh Trung [3 ]
Nghiem Ngoc Minh [1 ,2 ]
Vu Xuan Nghia [4 ]
Nguyen Van Giang [5 ]
Nguyen Xuan Canh [5 ]
Nguyen Linh Toan [4 ]
Truong Dinh Cam [6 ]
Nguyen Thanh Nga [1 ]
Tran Viet Tien [7 ]
Nguyen Huy Hoang [1 ,2 ]
机构
[1] Vietnam Acad Sci & Technol, Inst Genome Res, 18 Hoang Quoc Viet, Hanoi, Vietnam
[2] Grad Univ Sci & Technol, Vietnam Acad Sci & Technol, Hanoi, Vietnam
[3] Vietnam Mil Med Univ, Inst Biomed & Pharm, Hanoi, Vietnam
[4] Vietnam Mil Med Univ, Dept Pathophysiol, Hanoi, Vietnam
[5] Vietnam Natl Univ Agr, Fac Biotechnol, Hanoi, Vietnam
[6] 175 Mil Med Hosp, Dept Cardiol, Ho Chi Minh, Vietnam
[7] Vietnam Mil Med Univ, Hosp 103, Dept Infect Dis, Hanoi, Vietnam
关键词
dendritic cells; LPS; p38MAPK and otubain 1; EXPRESSION; PROLIFERATION; ACTIVATION; INCREASES; MIGRATION;
D O I
10.1111/tan.13534
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Dendritic cells (DCs) are professional antigen presenting cells (APCs) that represent the essential link between innate and acquired immunity. Otubain (OTUB) 1 is shown to deubiquitinate TRAFs to suppress virus-induced inflammatory response. MAPK, a downstream molecule of TRAFs, is involved in regulating LPS-induced immune reactions and its activation is sensitive to the presence of OTUB1. Little is known about contributions of OTUB1 to changes in biological properties of DCs. The present study, therefore, explored whether DC functions are influenced by OTUB1. To this end, DCs were isolated and cultured with GM-CSF to attain bone marrow-derived DCs (BMDCs) and followed by treatment with lipopolysaccharide (LPS) in the presence or absence of OTUB1 siRNA. Expression of markers of cellular maturation and proliferation were analyzed by flow cytometry, and secretion of inflammatory cytokines and ability to stimulate CD4(+) T-cells in allogenic mixed leukocyte reaction (allo-MLR) by ELISA, cell migration by a transwell migration assay and phagocytic capacity by FITC-dextran uptake measurement. As a result, treatment of the cells with OTUB1 siRNA prolonged activation of p38MAPK, increased CD54 expression and IL-6 release and reduced FITC-dextran uptake. Moreover, cytokine release produced from CD4(+) T-cells in allo-MLR was different. The enhanced level of IFN-gamma, but not other cytokine production was observed in the presence of siRNA OTUB1. All the effects were completely abolished when the cells were exposed with p38MAPK inhibitor SB203580. In conclusion, OTUB1 prevents the prolonged activation of p38MAPK, which in turn compromises DC functions.
引用
收藏
页码:462 / 470
页数:9
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