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Sequence-dependent dynamics of synthetic and endogenous RSSs in V(D)J recombination

机译:v(d)j重组中的合成和内源性RSS的序列依赖性动态

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Developing lymphocytes of jawed vertebrates cleave and combine distinct gene segments to assemble antigen-receptor genes. This process called V(D)J recombination that involves the RAG recombinase binding and cutting recombination signal sequences (RSSs) composed of conserved heptamer and non-amer sequences flanking less well-conserved 12-or 23-bp spacers. Little quantitative information is known about the contributions of individual RSS positions over the course of the RAG-RSS interaction. We employ a single-molecule method known as tethered particle motion to track the formation, lifetime and cleavage of individual RAG-12RSS-23RSS paired complexes (PCs) for numerous synthetic and endogenous 12RSSs. We reveal that single-bp changes, including in the 12RSS spacer, can significantly and selectively alter PC formation or the probability of RAG-mediated cleavage in the PC. We find that some rarely used endogenous gene segments can be mapped directly to poor RAG binding on their adjacent 12RSSs. Finally, we find that while abrogating RSS nicking with Ca2+ leads to substantially shorter PC lifetimes, analysis of the complete lifetime distributions of any 12RSS even on this reduced system reveals that the process of exiting the PC involves unidentified molecular details whose involvement in RAG-RSS dynamics are crucial to quantitatively capture kinetics in V(D)J recombination.
机译:显影脊椎动物的淋巴细胞切割,并将不同的基因段与组合抗原受体基因组合。该过程称为V(d)J重组,其涉及由保守的七肽和非Amer序列组成的rag重组酶结合和切割重组信号序列(RSS),并且非AMER序列侧翼较低的较低保守的12-或23bp间隔物。关于在RAG-RS相互作用的过程中,对单个RSS位置的贡献知之甚少。我们采用称为系环颗粒运动的单分子方法,以跟踪各个rag-12rss-23rs对多种合成和内源12rss的形成,寿命和裂解的单个RAG-12RSS-23RS对复合物(PC)。我们揭示了在12次间隔物中的单胞胎变化,包括在12RS间隔物中,可以显着且选择性地改变PC在PC中的rag介导的裂解的概率或缺陷的裂解。我们发现一些很少使用的内源基因段可以直接映射到其相邻的12rs上的差的覆盖物结合。最后,我们发现,同时用CA2 +发出rss的​​RSS,即使在这种减少的系统上也越短的PC寿命,也可以分析任何12RS的完整寿命分布,揭示了退出PC的过程涉及未识别的分子细节,其参与RAG-RS的未识别的分子细节动态对于定量捕获V(d)J重组的动力学是至关重要的。

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