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本文引用的文献

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Long-range interactions between three transcriptional enhancers, active Vkappa gene promoters, and a 3' boundary sequence spanning 46 kilobases.三个转录增强子、活跃的Vκ基因启动子与一个跨越46千碱基的3'边界序列之间的长程相互作用。
Mol Cell Biol. 2005 Apr;25(8):3220-31. doi: 10.1128/MCB.25.8.3220-3231.2005.
2
Important roles for E protein binding sites within the immunoglobulin kappa chain intronic enhancer in activating Vkappa Jkappa rearrangement.免疫球蛋白κ链内含子增强子内的E蛋白结合位点在激活VκJκ重排中起重要作用。
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Differential functions for the transcription factor E2A in positive and negative gene regulation in pre-B lymphocytes.转录因子E2A在pre-B淋巴细胞基因正负调控中的差异功能
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Variegated transcriptional activation of the immunoglobulin kappa locus in pre-b cells contributes to the allelic exclusion of light-chain expression.前B细胞中免疫球蛋白κ基因座的多样化转录激活有助于轻链表达的等位基因排斥。
Cell. 2004 Jul 9;118(1):19-29. doi: 10.1016/j.cell.2004.06.019.
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Regulation of activation and recombination of the murine Igkappa locus.小鼠Igκ基因座激活与重排的调控
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Regulation of E2A gene expression in B-lymphocyte development.B淋巴细胞发育过程中E2A基因表达的调控。
Mol Immunol. 2004 Mar;40(16):1165-77. doi: 10.1016/j.molimm.2003.11.031.
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Receptor editing and marginal zone B cell development are regulated by the helix-loop-helix protein, E2A.受体编辑和边缘区B细胞发育受螺旋-环-螺旋蛋白E2A调控。
J Exp Med. 2004 Apr 19;199(8):1101-12. doi: 10.1084/jem.20031180. Epub 2004 Apr 12.
8
Analysis of gene expression and Ig transcription in PU.1/Spi-B-deficient progenitor B cell lines.PU.1/Spi-B 缺陷祖 B 细胞系中的基因表达及 Ig 转录分析
J Immunol. 2004 Jan 1;172(1):144-54. doi: 10.4049/jimmunol.172.1.144.
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A conserved transcriptional enhancer regulates RAG gene expression in developing B cells.一个保守的转录增强子在发育中的B细胞中调节RAG基因的表达。
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10
IRF-4,8 orchestrate the pre-B-to-B transition in lymphocyte development.IRF-4、8在淋巴细胞发育过程中协调前B细胞到B细胞的转变。
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E2A和IRF-4/Pip促进前B细胞中免疫球蛋白κ基因座的染色质修饰和转录。

E2A and IRF-4/Pip promote chromatin modification and transcription of the immunoglobulin kappa locus in pre-B cells.

作者信息

Lazorchak Adam S, Schlissel Mark S, Zhuang Yuan

机构信息

Department of Immunology, Duke University Medical Center, Box 3010, 328 Jones Building, Research Drive, Durham, NC 27710, USA.

出版信息

Mol Cell Biol. 2006 Feb;26(3):810-21. doi: 10.1128/MCB.26.3.810-821.2006.

DOI:10.1128/MCB.26.3.810-821.2006
PMID:16428437
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1347029/
Abstract

The immunoglobulin kappa light chain (Igkappa) locus is regulated in a lineage- and stage-specific manner during B-cell development. The highly restricted timing of V to J gene recombination at the pre-B-cell stage is under the control of two enhancers, the intronic enhancer (kappaEi) and the 3' enhancer (kappaE3'), flanking the constant exon. E2A transcription factors have been indicated to be directly involved in the regulation of Igkappa locus activation. In this study, we utilize E2A-deficient pre-B cells to directly investigate the mechanism of E2A-mediated Igkappa activation. We demonstrate that Igkappa germ line transcription is severely impaired and recombination is blocked in the absence of E2A. Reconstitution of E2A-/- pre-B cells with inducible human E2A (E47R) is sufficient to promote chromatin modification of Igkappa and rescue Igkappa germ line transcription and Jkappa gene recombinase accessibility. Furthermore, we show that increased E2A recruitment to kappaEi and kappaE3' correlates with activation of Igkappa in pre-B cells and that recruitment of E2A to kappaE3' is in part dependent on the transcription factor IRF-4. Inhibition of IRF-4 expression in pre-B cells leads to a significant reduction of Igkappa germ line transcription and enhancer acetylation. In the absence of E2A, increased IRF-4 expression is not sufficient to promote Igkappa enhancer chromatin modification or transcription, suggesting that the sequential involvement of IRF-4 and E2A is necessary for the activation of the Igkappa locus. Finally, we provide genetic evidence in the mouse that E2A gene dosage can influence the development of pre-B cells during the phase of Igkappa gene activation.

摘要

免疫球蛋白κ轻链(Igκ)基因座在B细胞发育过程中以谱系和阶段特异性方式受到调控。前B细胞阶段V到J基因重组的高度受限时间受两个增强子控制,即内含子增强子(κEi)和3'增强子(κE3'),它们位于恒定外显子两侧。E2A转录因子已被表明直接参与Igκ基因座激活的调控。在本研究中,我们利用E2A缺陷的前B细胞直接研究E2A介导的Igκ激活机制。我们证明,在没有E2A的情况下,Igκ种系转录严重受损且重组被阻断。用可诱导的人E2A(E47R)重建E2A-/-前B细胞足以促进Igκ的染色质修饰并挽救Igκ种系转录和Jκ基因重组酶可及性。此外,我们表明E2A在前B细胞中向κEi和κE3'募集的增加与Igκ的激活相关,并且E2A向κE3'的募集部分依赖于转录因子IRF-4。在前B细胞中抑制IRF-4表达会导致Igκ种系转录和增强子乙酰化显著降低。在没有E2A的情况下,IRF-4表达的增加不足以促进Igκ增强子染色质修饰或转录,这表明IRF-4和E2A的顺序参与对于Igκ基因座的激活是必要的。最后,我们在小鼠中提供了遗传学证据,表明E2A基因剂量可以在Igκ基因激活阶段影响前B细胞的发育。