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酵母中端粒酶丰度较低:对端粒酶单倍剂量不足的影响。

Low abundance of telomerase in yeast: implications for telomerase haploinsufficiency.

作者信息

Mozdy Amy D, Cech Thomas R

机构信息

Howard Hughes Medical Institute, Department of Chemistry and Biochemistry, University of Colorado, Boulder, Colorado 80309-0215, USA.

出版信息

RNA. 2006 Sep;12(9):1721-37. doi: 10.1261/rna.134706. Epub 2006 Aug 7.

Abstract

Telomerase is an RNA-dependent reverse transcriptase that maintains telomeric DNA at a species-specific equilibrium length. To determine an upper limit for the number of telomerase molecules in a Saccharomyces cerevisiae cell, we have established real-time RT-PCR assays to quantify the noncoding telomerase RNA, TLC1. We find that the number of TLC1 molecules in a haploid yeast cell is approximately 29, less than the number of chromosome ends (64) in late S-phase. Wild-type diploid cells contain approximately 37 telomerase RNAs, while diploids heterozygous for a null tlc1 allele have half the wild-type amount, approximately 19 TLC1 molecules. For comparison, there are approximately 480 molecules of the U2 snRNA per haploid cell. We show that a biological consequence of this low level of telomerase is haploinsufficiency: A TLC1/tlc1Delta heterozygote maintains shorter telomeres. A dominant-negative telomerase RNA, with a deletion of the template for telomeric DNA synthesis, further demonstrates that yeast telomere length is sensitive to telomerase dosage. Sixfold overexpression of tlc1Deltatemplate establishes a new telomere length set point, approximately 160 bp shorter than wild type. Removing telomerase protein-interaction sites from the tlc1Deltatemplate RNA mitigates the dominant-negative effect, suggesting that the tlc1Deltatemplate RNA competes with wild-type TLC1 for a limited supply of telomerase proteins or for telomeres. Because yeast telomerase is tethered at chromosome ends, the finding that it may be outnumbered by its telomeric DNA substrates provides a new perspective for interpreting the results of telomere maintenance studies.

摘要

端粒酶是一种依赖RNA的逆转录酶,可将端粒DNA维持在物种特异性的平衡长度。为了确定酿酒酵母细胞中端粒酶分子数量的上限,我们建立了实时RT-PCR检测方法来定量非编码端粒酶RNA,即TLC1。我们发现,单倍体酵母细胞中TLC1分子的数量约为29个,少于S期后期染色体末端的数量(64个)。野生型二倍体细胞含有约37个端粒酶RNA,而tlc1无效等位基因杂合的二倍体细胞的端粒酶RNA数量是野生型的一半,约为19个TLC1分子。作为比较,每个单倍体细胞中约有480个U2 snRNA分子。我们表明,这种低水平端粒酶的生物学后果是单倍体不足:TLC1/tlc1Delta杂合子维持较短的端粒。一种缺失端粒DNA合成模板的显性负性端粒酶RNA进一步证明,酵母端粒长度对端粒酶剂量敏感。tlc1Deltatemplate的六倍过表达建立了一个新的端粒长度设定点,比野生型短约160 bp。从tlc1Deltatemplate RNA中去除端粒酶蛋白相互作用位点可减轻显性负性效应,这表明tlc1Deltatemplate RNA与野生型TLC1竞争有限的端粒酶蛋白供应或端粒。由于酵母端粒酶定位于染色体末端,其数量可能少于其端粒DNA底物这一发现为解释端粒维持研究结果提供了新的视角。

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