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Coordinated DNA dynamics during the human telomerase catalytic cycle

机译:人类端粒酶催化循环中协调的DNA动力学

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The human telomerase reverse transcriptase ( hTERT ) utilizes a template within the integral RNA subunit ( hTR ) to direct extension of telomeres. Telomerase exhibits repeat addition processivity (RAP) and must therefore translocate the nascent DNA product into a new RNA:DNA hybrid register to prime each round of telomere repeat synthesis. Here, we use single-molecule FRET and nuclease protection assays to monitor telomere DNA structure and dynamics during the telomerase catalytic cycle. DNA translocation during RAP proceeds through a previously uncharacterized kinetic substep during which the 3′-end of the DNA substrate base pairs downstream within the hTR template. The rate constant for DNA primer realignment reveals this step is not rate limiting for RAP, suggesting a second slow conformational change repositions the RNA:DNA hybrid into the telomerase active site and drives the extrusion of the 5′-end of the DNA primer out of the enzyme complex.
机译:人类端粒酶逆转录酶(hTERT)利用整合RNA亚基(hTR)中的模板指导端粒的延伸。端粒酶表现出重复添加持续性(RAP),因此必须将新生的DNA产物转移到新的RNA:DNA杂合寄存器中,以引发端粒重复合成的每一轮。在这里,我们使用单分子FRET和核酸酶保护试验来监测端粒酶催化循环过程中的端粒DNA结构和动力学。 RAP过程中的DNA易位通过先前未描述的动力学子步骤进行,在此子过程中,DNA底物的3'端碱基对在hTR模板的下游配对。 DNA引物重新排列的速率常数表明该步骤对RAP的速率没有限制,表明第二个缓慢的构象变化将RNA:DNA杂种重新定位到端粒酶活性位点,并驱使DNA引物的5'端挤出酶复合物。

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