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染色质环化所造成的限制会在免疫球蛋白类别转换重组过程中限制重组靶向。

Constraints contributed by chromatin looping limit recombination targeting during Ig class switch recombination.

作者信息

Feldman Scott, Achour Ikbel, Wuerffel Robert, Kumar Satyendra, Gerasimova Tatiana, Sen Ranjan, Kenter Amy L

机构信息

Department of Microbiology and Immunology, University of Illinois College of Medicine, Chicago, IL 60612; and.

Gene Regulation Section, Laboratory of Cellular and Molecular Biology, National Institute on Aging/National Institutes of Health, Baltimore, MD 21224.

出版信息

J Immunol. 2015 Mar 1;194(5):2380-9. doi: 10.4049/jimmunol.1401170. Epub 2015 Jan 26.

Abstract

Engagement of promoters with distal elements in long-range looping interactions has been implicated in regulation of Ig class switch recombination (CSR). The principles determining the spatial and regulatory relationships among Igh transcriptional elements remain poorly defined. We examined the chromosome conformation of C region (CH) loci that are targeted for CSR in a cytokine-dependent fashion in mature B lymphocytes. Germline transcription (GLT) of the γ1 and ε CH loci is controlled by two transcription factors, IL-4-inducible STAT6 and LPS-activated NF-κB. We showed that although STAT6 deficiency triggered loss of GLT, deletion of NF-κB p50 abolished both GLT and γ1 locus:enhancer looping. Thus, chromatin looping between CH loci and Igh enhancers is independent of GLT production and STAT6, whereas the establishment and maintenance of these chromatin contacts requires NF-κB p50. Comparative analysis of the endogenous γ1 locus and a knock-in heterologous promoter in mice identified the promoter per se as the interactive looping element and showed that transcription elongation is dispensable for promoter/enhancer interactions. Interposition of the LPS-responsive heterologous promoter between the LPS-inducible γ3 and γ2b loci altered GLT expression and essentially abolished direct IgG2b switching while maintaining a sequential μ→γ3→γ2b format. Our study provides evidence that promoter/enhancer looping interactions can introduce negative constraints on distal promoters and affect their ability to engage in germline transcription and determine CSR targeting.

摘要

启动子与远距离环化相互作用中的远端元件结合,已被认为与免疫球蛋白类别转换重组(CSR)的调控有关。确定Igh转录元件之间空间和调控关系的原则仍不清楚。我们研究了成熟B淋巴细胞中以细胞因子依赖方式进行CSR靶向的C区(CH)基因座的染色体构象。γ1和ε CH基因座的胚系转录(GLT)由两种转录因子控制,即IL-4诱导的STAT6和LPS激活的NF-κB。我们发现,虽然STAT6缺陷导致GLT缺失,但NF-κB p50的缺失消除了GLT和γ1基因座:增强子环化。因此,CH基因座与Igh增强子之间的染色质环化独立于GLT产生和STAT6,而这些染色质接触的建立和维持需要NF-κB p50。对小鼠内源性γ1基因座和敲入的异源启动子的比较分析确定启动子本身为相互作用的环化元件,并表明转录延伸对于启动子/增强子相互作用是可有可无的。在LPS诱导的γ3和γ2b基因座之间插入LPS反应性异源启动子改变了GLT表达,并基本消除了直接的IgG2b转换,同时保持了μ→γ3→γ2b的顺序形式。我们的研究提供了证据,表明启动子/增强子环化相互作用可以对远端启动子施加负向限制,并影响它们参与胚系转录和确定CSR靶向的能力。

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