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一个结构保守的人类和端粒酶催化核心。

A structurally conserved human and telomerase catalytic core.

机构信息

Department of Chemistry and Biochemistry, University of California, Los Angeles, CA 90095-1569.

Department of Chemistry and Biochemistry, University of California, Los Angeles, CA 90095-1569

出版信息

Proc Natl Acad Sci U S A. 2020 Dec 8;117(49):31078-31087. doi: 10.1073/pnas.2011684117. Epub 2020 Nov 23.

Abstract

Telomerase is a ribonucleoprotein complex that counteracts the shortening of chromosome ends due to incomplete replication. Telomerase contains a catalytic core of telomerase reverse transcriptase (TERT) and telomerase RNA (TER). However, what defines TERT and separates it from other reverse transcriptases remains a subject of debate. A recent cryoelectron microscopy map of telomerase revealed the structure of a previously uncharacterized TERT domain (TRAP) with unanticipated interactions with the telomerase essential N-terminal (TEN) domain and roles in telomerase activity. Both TEN and TRAP are absent in the putative TERT that has been used as a model for telomerase for over a decade. To investigate the conservation of TRAP and TEN across species, we performed multiple sequence alignments and statistical coupling analysis on all identified TERTs and find that TEN and TRAP have coevolved as telomerase-specific domains. Integrating the data from bioinformatic analysis and the structure of telomerase, we built a pseudoatomic model of human telomerase catalytic core that accounts for almost all of the cryoelectron microscopy density in a published map, including TRAP in previously unassigned density as well as telomerase RNA domains essential for activity. This more complete model of the human telomerase catalytic core illustrates how domains of TER and TERT, including the TEN-TRAP complex, can interact in a conserved manner to regulate telomere synthesis.

摘要

端粒酶是一种核糖核蛋白复合物,可抵消由于不完全复制而导致的染色体末端缩短。端粒酶包含端粒酶逆转录酶 ( TERT ) 和端粒酶 RNA ( TER ) 的催化核心。然而,定义 TERT 并将其与其他逆转录酶区分开来的是什么,仍然是一个争论的话题。最近的一项端粒酶低温电子显微镜图谱揭示了以前未被表征的 TERT 结构域 ( TRAP ) 的结构,该结构域与端粒酶必需的 N 端 ( TEN ) 结构域具有意想不到的相互作用,并在端粒酶活性中发挥作用。TEN 和 TRAP 都不存在于已经被用作端粒酶模型超过十年的假定 TERT 中。为了研究 TRAP 和 TEN 在物种间的保守性,我们对所有鉴定的 TERT 进行了多次序列比对和统计耦合分析,发现 TEN 和 TRAP 作为端粒酶特有的结构域共同进化。将生物信息学分析和端粒酶结构的数据整合在一起,我们构建了人端粒酶催化核心的伪原子模型,该模型解释了发表图谱中几乎所有低温电子显微镜密度,包括以前未分配密度的 TRAP 以及对活性至关重要的端粒酶 RNA 结构域。这个更完整的人端粒酶催化核心模型说明了 TER 和 TERT 的结构域,包括 TEN-TRAP 复合物,如何以保守的方式相互作用来调节端粒合成。

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Diagnostic utility of telomere length testing in a hospital-based setting.基于医院环境的端粒长度检测的诊断效用。
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