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Regulation of relB in dendritic cells by means of modulated association of vitamin D receptor and histone deacetylase 3 with the promoter

机译:通过维生素D受体和组蛋白脱乙酰基酶3与启动子的调节结合,调节树突状细胞中relB的表达

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摘要

The NF-κB component RelB is essential for dendritic cell (DC) differentiation and maturation. The vitamin D receptor (VDR) is a nuclear receptor that mediates inhibition of DC maturation and transcriptional repression of relB after engagement of its ligand, 1α,25-dihydroxyvitamin D3, or related analogs (D3 analogs). Ligand-dependent relB suppression was abolished by a histone deacetylase (HDAC) inhibitor. Constitutive association of VDR with the relB promoter was demonstrated in DCs by chromatin immunoprecipitation. Promoter binding by VDR was enhanced by ligand and reduced by LPS. Association of HDAC3 and HDAC1 with the relB VDR-binding site was observed, but only HDAC3 was reciprocally modulated by D3 analog and LPS. Overexpression of HDAC3 caused relB promoter suppression, increased sensitivity to D3 analog, and resistance to LPS. Depletion of HDAC3 attenuated relB suppression by D3 analog. In vivo, D3 analog resulted in reduced RelB in DCs from VDR WT mice but not VDR knockout mice. Other NF-lation of RelB and c-Rel in control animals. We conclude that vitamin D-regulated relB transcription in DCs is controlled by chromatin remodeling by means of recruitment of complexes including HDAC3.
机译:NF-κB成分RelB对于树突状细胞(DC)分化和成熟至关重要。维生素D受体(VDR)是一种核受体,在其配体,1α,25-二羟基维生素D3或相关类似物(D3类似物)接合后,介导DC成熟的抑制和relB的转录抑制。组蛋白脱乙酰基酶(HDAC)抑制剂取消了依赖配体的relB抑制。通过染色质免疫沉淀在DC中证实了VDR与relB启动子的组成性缔合。 VDR启动子结合被配体增强而被LPS降低。观察到HDAC3和HDAC1与relB VDR结合位点的关联,但只有HDAC3被D3类似物和LPS相互调节。 HDAC3的过表达引起relB启动子抑制,对D3类似物的敏感性增加以及对LPS的抗性。通过D3模拟耗尽HDAC3的relB抑制衰减。在体内,D3类似物导致VDR WT小鼠的DC中的RelB减少,但VDR敲除小鼠的DC中的RelB减少。对照动物中RelB和c-Rel的其他NF-化。我们得出的结论是,DC中维生素D调节的relB转录受染色质重塑的控制,该染色质重塑是通过募集包括HDAC3在内的复合物来实现的。

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