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Ig Sγ3 DNA 处依赖核因子κB p50的体内足迹与μ向γ3转换重组相关。

NF-kappa B p50-dependent in vivo footprints at Ig S gamma 3 DNA are correlated with mu-->gamma 3 switch recombination.

作者信息

Wuerffel R A, Ma L, Kenter A L

机构信息

Department of Microbiology and Immunology, University of Illinois College of Medicine, Chicago, IL 60680, USA.

出版信息

J Immunol. 2001 Apr 1;166(7):4552-9. doi: 10.4049/jimmunol.166.7.4552.

Abstract

NF-kappa B has been demonstrated to play critical roles in multiple aspects of immune responses including Ig H chain isotype switching. To better define the specific roles the p50 subunit of NF-kappa B plays in mu-->gamma 3 switch recombination (SR), we systematically evaluated p50-deficient B cells for activities that are strongly correlated with SR. B cell activation with LPS plus anti-IgD-dextran plus IL-5 plus IL-4 plus TGF-beta produced normal levels of proliferation and gamma3 germline transcripts in p50-deficient B cells, but mu-->gamma 3 SR was impaired. In vitro binding studies previously showed that NF-kappa B p50 homodimer binds the switch nuclear B-site protein (SNIP) of the S gamma 3 tandem repeat. Ligation-mediated PCR in vivo footprint analysis demonstrates that the region spanning the SNIP and switch nuclear A-site protein (SNAP) binding sites of the S gamma 3 region are contacted by protein in normal resting splenic B cells. B cells that are homozygous for the targeted disruption of the gene encoding p50 (-/-) show strong aberrant footprints, whereas heterozygous cells (+/-) reveal a partial effect in S gamma 3 DNA. These studies provide evidence of nucleoprotein interactions at switch DNA in vivo and suggest a direct interaction of p50 with S gamma 3 DNA that is strongly correlated with SR competence.

摘要

核因子-κB(NF-κB)已被证明在免疫反应的多个方面发挥关键作用,包括Ig重链同种型转换。为了更好地确定NF-κB的p50亚基在μ→γ3转换重组(SR)中所起的具体作用,我们系统地评估了p50缺陷型B细胞中与SR密切相关的活性。用脂多糖(LPS)加抗IgD-葡聚糖加白细胞介素-5(IL-5)加白细胞介素-4(IL-4)加转化生长因子-β(TGF-β)激活p50缺陷型B细胞,其增殖水平和γ3种系转录本正常,但μ→γ3 SR受损。体外结合研究先前表明,NF-κB p50同二聚体与Sγ3串联重复序列的转换核B位点蛋白(SNIP)结合。体内连接介导的PCR足迹分析表明,在正常静息脾B细胞中,蛋白质可与跨越Sγ3区域的SNIP和转换核A位点蛋白(SNAP)结合位点的区域发生接触。编码p50的基因靶向破坏的纯合B细胞(-/-)显示出强烈的异常足迹,而异合子细胞(+/-)在Sγ3 DNA中显示出部分效应。这些研究提供了体内转换DNA处核蛋白相互作用的证据,并表明p50与Sγ3 DNA的直接相互作用与SR能力密切相关。

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