Li Yijin, Louzoun Yoram, Weigert Martin
Department of Molecular Biology, Princeton University, NJ 08544, USA.
J Exp Med. 2004 Feb 2;199(3):337-46. doi: 10.1084/jem.20031712.
Receptor editing is performed by replacement of Vkappa genes that contribute to autoreactivity. In addition, the Ckappa locus can be deleted by Vkappa rearrangement to intronic or 3' of Ckappa RS sequences (also referred to as kappa deletion elements). B cells that delete the Ckappa can then express lambda light chains. However, the lambda locus, either of man or mouse, does not allow V gene replacement. Nor does it appear to be deleted. Therefore, editing of autoreactive lambda B cells may require alternative pathways. We have found that in anti-DNA heavy chain transgenic mice (tgs) VH3H9/56R, B cells that express anti-DNA receptors comprised of lambda1 in association with an anti-DNA heavy chain often coexpress a kappa chain that prevents DNA binding. We speculate that such isotypically included cells may have low anti-DNA receptor densities, a feature that may lead to self-tolerance. Here we describe a mechanism of preventing DNA binding by expression of a rarely used member of the Vlambda family, Vlambdax. The lambdax B cells of the tgs also express CD25 and may represent B cells that have exhausted light chain editing possibilities.
受体编辑通过替换导致自身反应性的Vκ基因来进行。此外,Cκ基因座可通过Vκ重排至Cκ RS序列(也称为κ缺失元件)的内含子或3'端而被删除。删除Cκ的B细胞随后可表达λ轻链。然而,人类或小鼠的λ基因座均不允许V基因替换,似乎也不会被删除。因此,自身反应性λ B细胞的编辑可能需要其他途径。我们发现,在抗DNA重链转基因小鼠(tgs)VH3H9/56R中,表达由λ1与抗DNA重链组成的抗DNA受体的B细胞通常共表达一种κ链,该κ链可阻止DNA结合。我们推测,这类同型包含细胞的抗DNA受体密度可能较低,这一特征可能导致自身耐受。在此,我们描述了一种通过表达Vλ家族中很少使用的成员Vλx来阻止DNA结合的机制。tgs的λx B细胞也表达CD25,可能代表已经用尽轻链编辑可能性的B细胞。
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