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端粒酶将G-四链体和线性DNA识别为不同的底物。

Telomerase recognizes G-quadruplex and linear DNA as distinct substrates.

作者信息

Oganesian Liana, Graham Mark E, Robinson Phillip J, Bryan Tracy M

机构信息

Children's Medical Research Institute, 214 Hawkesbury Road, Westmead NSW 2145, Australia and University of Sydney, NSW 2006, Australia.

出版信息

Biochemistry. 2007 Oct 9;46(40):11279-90. doi: 10.1021/bi700993q. Epub 2007 Sep 18.

DOI:10.1021/bi700993q
PMID:17877374
Abstract

Telomeric DNA can assemble into a nonlinear, higher-order conformation known as a G-quadruplex. Here, we demonstrate by electrospray ionization mass spectrometry that the two repeat telomeric sequence d(TGGGGTTGGGGT) from Tetrahymena thermophila gives rise to a novel parallel four-stranded G-quadruplex in the presence of sodium. The G-quadruplex directly interacts with the catalytic subunit of Tetrahymena telomerase (TERT) with micromolar affinity, and the presence of telomerase RNA is not obligatory for this interaction. Both N- and C-terminal halves of TERT bind the G-quadruplex independently. This G-quadruplex is a robust substrate for both recombinant and cell extract-derived telomerase in vitro. Furthermore, the G-quadruplex weakens the affinity of wild-type telomerase for the incoming nucleotide (dTTP) and likely perturbs the nucleotide binding pocket of the enzyme. In agreement with this, a lysine to alanine substitution at amino acid 538 (K538A) within motif 1 of TERT dramatically reduces the ability of telomerase to extend G-quadruplex but not linear DNA. The K538A mutant retains binding affinity for the quadruplex. This suggests that telomerase undergoes changes in conformation in its active site to specifically accommodate binding and subsequent extension of G-quadruplex DNA. We propose that telomerase recognizes G-quadruplex DNA as a substrate that is distinct from linear DNA.

摘要

端粒DNA可以组装成一种非线性的高阶构象,即G-四链体。在此,我们通过电喷雾电离质谱证明,来自嗜热四膜虫的两个重复端粒序列d(TGGGGTTGGGGT)在有钠存在的情况下会形成一种新型的平行四链G-四链体。该G-四链体以微摩尔亲和力直接与嗜热四膜虫端粒酶(TERT)的催化亚基相互作用,并且这种相互作用并不需要端粒酶RNA的存在。TERT的N端和C端两半独立地结合G-四链体。这种G-四链体在体外是重组端粒酶和细胞提取物来源的端粒酶的强大底物。此外,G-四链体削弱了野生型端粒酶对进入的核苷酸(dTTP)的亲和力,并可能扰乱该酶的核苷酸结合口袋。与此一致的是,TERT基序1内氨基酸538处的赖氨酸到丙氨酸的取代(K538A)显著降低了端粒酶延伸G-四链体而不是线性DNA的能力。K538A突变体保留了对四链体的结合亲和力。这表明端粒酶在其活性位点发生构象变化,以特异性适应G-四链体DNA的结合和随后的延伸。我们提出,端粒酶将G-四链体DNA识别为一种不同于线性DNA的底物。

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Telomerase recognizes G-quadruplex and linear DNA as distinct substrates.端粒酶将G-四链体和线性DNA识别为不同的底物。
Biochemistry. 2007 Oct 9;46(40):11279-90. doi: 10.1021/bi700993q. Epub 2007 Sep 18.
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The different biological effects of telomestatin and TMPyP4 can be attributed to their selectivity for interaction with intramolecular or intermolecular G-quadruplex structures.端粒抑素和TMPyP4不同的生物学效应可归因于它们与分子内或分子间G-四链体结构相互作用的选择性。
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Combining Electrospray Mass Spectrometry (ESI-MS) and Computational Techniques in the Assessment of G-Quadruplex Ligands: A Hybrid Approach to Optimize Hit Discovery.结合电喷雾质谱(ESI-MS)和计算技术评估 G-四链体配体:一种优化命中发现的混合方法。
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Molecules. 2020 Aug 13;25(16):3686. doi: 10.3390/molecules25163686.
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A mechanism for the extension and unfolding of parallel telomeric G-quadruplexes by human telomerase at single-molecule resolution.人类端粒酶在单分子分辨率下延伸和展开平行端粒 G-四链体的机制。
Elife. 2020 Jul 29;9:e56428. doi: 10.7554/eLife.56428.
5
GNG Motifs Can Replace a GGG Stretch during G-Quadruplex Formation in a Context Dependent Manner.GNG模体可以在依赖于上下文的方式下,在G-四链体形成过程中取代一段GGG序列。
PLoS One. 2016 Jul 14;11(7):e0158794. doi: 10.1371/journal.pone.0158794. eCollection 2016.
6
Telomeric G-quadruplexes are a substrate and site of localization for human telomerase.端粒G-四链体是人类端粒酶的一个底物和定位位点。
Nat Commun. 2015 Jul 9;6:7643. doi: 10.1038/ncomms8643.
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Telomere maintenance mechanisms in cancer: clinical implications.癌症中的端粒维持机制:临床意义
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