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酵母中端粒DNA周转的动力学

Dynamics of telomeric DNA turnover in yeast.

作者信息

McEachern Michael J, Underwood Dana Hager, Blackburn Elizabeth H

机构信息

Department of Genetics, Life Sciences Building, University of Georgia, Athens, Georgia 30602-7223, USA.

出版信息

Genetics. 2002 Jan;160(1):63-73. doi: 10.1093/genetics/160.1.63.

DOI:10.1093/genetics/160.1.63
PMID:11805045
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1461958/
Abstract

Telomerase adds telomeric DNA repeats to telomeric termini using a sequence within its RNA subunit as a template. We characterized two mutations in the Kluyveromyces lactis telomerase RNA gene (TER1) template. Each initially produced normally regulated telomeres. One mutation, ter1-AA, had a cryptic defect in length regulation that was apparent only if the mutant gene was transformed into a TER1 deletion strain to permit extensive replacement of basal wild-type repeats with mutant repeats. This mutant differs from previously studied delayed elongation mutants in a number of properties. The second mutation, TER1-Bcl, which generates a BclI restriction site in newly synthesized telomeric repeats, was indistinguishable from wild type in all phenotypes assayed: cell growth, telomere length, and in vivo telomerase fidelity. TER1-Bcl cells demonstrated that the outer halves of the telomeric repeat tracts turn over within a few hundred cell divisions, while the innermost few repeats typically resisted turnover for at least 3000 cell divisions. Similarly deep but incomplete turnover was also observed in two other TER1 template mutants with highly elongated telomeres. These results indicate that most DNA turnover in functionally normal telomeres is due to gradual replicative sequence loss and additions by telomerase but that there are other processes that also contribute to turnover.

摘要

端粒酶利用其RNA亚基内的序列作为模板,将端粒DNA重复序列添加到端粒末端。我们对乳酸克鲁维酵母端粒酶RNA基因(TER1)模板中的两个突变进行了表征。每个突变最初产生的端粒调控正常。其中一个突变,ter1-AA,在长度调控方面存在隐性缺陷,只有当突变基因被转化到TER1缺失菌株中,以允许大量用突变重复序列替代基础野生型重复序列时,这种缺陷才会显现出来。该突变体在许多特性上与先前研究的延迟延伸突变体不同。第二个突变,TER1-Bcl,在新合成的端粒重复序列中产生一个BclI限制性位点,在所有检测的表型中:细胞生长、端粒长度和体内端粒酶保真度方面,与野生型没有区别。TER1-Bcl细胞表明,端粒重复序列束的外半部分在几百次细胞分裂内发生更替,而最里面的少数重复序列通常至少在3000次细胞分裂中抵抗更替。在另外两个具有高度延长端粒的TER1模板突变体中也观察到了类似深度但不完全的更替。这些结果表明,功能正常的端粒中的大多数DNA更替是由于端粒酶导致的逐渐复制性序列丢失和添加,但也有其他过程导致了更替。

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1
Dynamics of telomeric DNA turnover in yeast.酵母中端粒DNA周转的动力学
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2
Genetic dissection of the Kluyveromyces lactis telomere and evidence for telomere capping defects in TER1 mutants with long telomeres.乳酸克鲁维酵母端粒的遗传剖析以及具有长端粒的TER1突变体中端粒封端缺陷的证据。
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3
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Mutant telomeric repeats in yeast can disrupt the negative regulation of recombination-mediated telomere maintenance and create an alternative lengthening of telomeres-like phenotype.酵母中的突变端粒重复序列可破坏重组介导的端粒维持的负调控,并产生类似端粒替代延长的表型。
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Rap1 protein regulates telomere turnover in yeast.Rap1蛋白调控酵母中的端粒周转。
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Control of telomere growth by interactions of RAP1 with the most distal telomeric repeats.通过RAP1与最远端端粒重复序列的相互作用来控制端粒生长。
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Recombination at long mutant telomeres produces tiny single- and double-stranded telomeric circles.在长的突变端粒处发生的重组会产生微小的单链和双链端粒环。
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引用本文的文献

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PLoS Genet. 2012;8(11):e1003017. doi: 10.1371/journal.pgen.1003017. Epub 2012 Nov 1.
2
Recombination can cause telomere elongations as well as truncations deep within telomeres in wild-type Kluyveromyces lactis cells.在野生型乳酸克鲁维酵母细胞中,重组可导致端粒延长以及端粒内部深处的截短。
Eukaryot Cell. 2011 Feb;10(2):226-36. doi: 10.1128/EC.00209-10. Epub 2010 Dec 10.
3
Evidence for an additional base-pairing element between the telomeric repeat and the telomerase RNA template in Kluyveromyces lactis and other yeasts.乳酸克鲁维酵母和其他酵母中端粒重复序列与端粒酶RNA模板之间存在额外碱基配对元件的证据。
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4
Mutant telomeric repeats in yeast can disrupt the negative regulation of recombination-mediated telomere maintenance and create an alternative lengthening of telomeres-like phenotype.酵母中的突变端粒重复序列可破坏重组介导的端粒维持的负调控,并产生类似端粒替代延长的表型。
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5
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本文引用的文献

1
Totally mutant telomeres: single-step mutagenesis of tandem repeat DNA sequences.完全突变的端粒:串联重复DNA序列的单步诱变
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Telomeres and their control.端粒及其调控
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Specific telomerase RNA residues distant from the template are essential for telomerase function.远离模板的特定端粒酶RNA残基对于端粒酶功能至关重要。
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