共 48 条
Molecular regulation of MHC class I chain-related protein A expression after HDAC-inhibitor treatment of Jurkat T cells
被引:50
作者:

Andresen, Lars
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机构:
Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark

Jensen, Helle
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Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark

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Hansen, Karen A.
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Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark

Skov, Soren
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Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark
机构:
[1] Univ Copenhagen, Dept Immunol, Inst Int Hlth Immunol & Microbiol, DK-1168 Copenhagen, Denmark
关键词:
D O I:
10.4049/jimmunol.179.12.8235
中图分类号:
R392 [医学免疫学];
Q939.91 [免疫学];
学科分类号:
100102 ;
摘要:
In this study, we characterize the molecular signal pathways that lead to MHC class I chain-related protein A (MICA) expression after histone deacetylase (HDAC)-inhibitor (HDAC-i) treatment of Jurkat T cells. Chelating calcium with BAPTA-AM or EGTA potently inhibited HDAC- and CMV-mediated MICA/B expression. It was further observed that endoplasmic reticulum calcium stores were depleted after HDAC treatment. NF-kappa B activity can be induced by HDAC treatment. However, nuclear translocation of NF-kappa B p65 was not observed after HDAC treatment of Jurkat T cells and even though we could effectively inhibit p65 expression by siRNA, it did not modify MICA/B expression. To identify important elements in MICA regulation, we made a promoter construct consisting of similar to 3 kb of the proximal MICA promoter in front of GFP. Deletion analysis showed that a germinal center-box containing a putative Sp1 site from position -113 to -93 relative to the mRNA start site was important for HDAC and CMV-induced promoter activity. Sp1 was subsequently shown to be important, as targeted mutation of the Sp1 binding sequence or siRNA mediated down modulation of Sp1-inhibited MICA promoter activity and surface-expression.
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页码:8235 / 8242
页数:8
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