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Fluorescence Resonance Energy Transfer Analysis of Recombination Signal Sequence Configuration in the RAG1/2 Synaptic Complex

机译:RAG1 / 2突触复合物中重组信号序列构型的荧光共振能量转移分析

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A critical step in V(D)J recombination is the synapsis of complementary (12/23) recombination signal sequences (RSSs) by the RAG1 and RAG2 proteins to generate the paired complex (PC). Using a facilitated ligation assay and substrates that vary the helical phasing of the RSSs, we provide evidence that one particular geometric configuration of the RSSs is favored in the PC. To investigate this configuration further, we used fluorescent resonance energy transfer (FRET) to detect the synapsis of fluorescently labeled RSS oligonucleotides. FRET requires an appropriate 12/23 RSS pair, a divalent metal ion, and high-mobility-group protein HMGB1 or HMGB2. Energy transfer between the RSSs was detected with all 12/23 RSS end positions of the fluorescent probes but was not detected when probes were placed on the two ends of the same RSS. Energy transfer was confirmed to originate from the PC by using an in-gel FRET assay. The results argue against a unique planar configuration of the RSSs in the PC and are most easily accommodated by models in which synapsed 12- and 23-RSSs are bent and cross one another, with implications for the organization of the RAG proteins and the DNA substrates at the time of cleavage.
机译:V(D)J重组的关键步骤是RAG1和RAG2蛋白对互补(12/23)重组信号序列(RSS)的突触,以生成配对的复合物(PC)。使用便利的连接测定法和可改变RSS螺旋相位的底物,我们提供了PC偏爱RSS的一种特殊几何构型的证据。为了进一步研究此配置,我们使用了荧光共振能量转移(FRET)来检测荧光标记的RSS寡核苷酸的突触。 FRET需要适当的12/23 RSS对,二价金属离子和高迁移率基团蛋白HMGB1或HMGB2。使用荧光探针的所有12/23 RSS末端位置都可以检测到RSS之间的能量转移,但是当将探针放在同一RSS的两端时,则无法检测到能量转移。通过使用凝胶内FRET分析,证实了能量转移源自PC。结果与PC中RSS的独特平面构型相抵触,并且最容易被以下模型容纳:突触的12-RSS和23-RSS弯曲并彼此交叉,这对RAG蛋白质和DNA底物的组织有影响分裂时。

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