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与新大草履虫端粒酶RNA互补的寡核苷酸描绘了模板结构域并揭示了一种新的引物利用模式。

Oligonucleotides complementary to the Oxytricha nova telomerase RNA delineate the template domain and uncover a novel mode of primer utilization.

作者信息

Melek M, Davis B T, Shippen D E

机构信息

Department of Biochemistry and Biophysics, Texas A&M University, College Station 77843-2128.

出版信息

Mol Cell Biol. 1994 Dec;14(12):7827-38. doi: 10.1128/mcb.14.12.7827-7838.1994.

Abstract

The telomerase reverse transcriptase uses an essential RNA subunit as a template to direct telomeric DNA synthesis. The 190-nucleotide Oxytricha nova telomerase RNA was identified by using an oligonucleotide probe complementary to the predicted CCCCAAAA template. This RNA displays extensive sequence similarity to the Euplotes crassus telomerase RNA and carries the same 5' CAAAACCCCAAAACC 3' telomeric domain. Antisense oligonucleotides were used to map the boundaries of the functional template and to investigate the mechanism of primer recognition and elongation. On the basis of their ability to inhibit or to prime telomerase, oligonucleotides were classified into three categories. Category 1 oligonucleotides, which extended 5' of residue 42 in the RNA, abolished elongation of (T4G4)3 and (G4T4)3 primers in vitro. In contrast, oligonucleotides terminating between residues 42 and 50 (categories 2 and 3), served as efficient telomerase primers. We conclude that the O. nova template comprises residues 42 to 50 in the 190-nucleotide RNA, a different set of nucleotides than are used by the E. crassus enzyme. Category 2 primer reactions amassed short products, and their abundance could be decreased by altering the 5' sequence of the primer, consistent with the two-primer-binding-site model for telomerase. Category 3 primers generated a bimodal distribution of short and long products, each having a unique elongation profile. The long-product profile is inconsistent with sequence-specific primer alignment. Rather, each primer was extended by the same register of TTTTGGGG repeats, suggesting shuttling to a default position within the template. The parallels between telomerase and RNA polymerase elongation mechanisms are discussed.

摘要

端粒酶逆转录酶以一个必需的RNA亚基作为模板来指导端粒DNA的合成。通过使用与预测的CCCCAAAA模板互补的寡核苷酸探针,鉴定出了190个核苷酸的嗜热四膜虫端粒酶RNA。该RNA与粗壮真核游仆虫端粒酶RNA显示出广泛的序列相似性,并携带相同的5' CAAAACCCCAAAACC 3'端粒结构域。反义寡核苷酸被用于绘制功能性模板的边界,并研究引物识别和延伸的机制。根据它们抑制或引发端粒酶的能力,寡核苷酸被分为三类。第1类寡核苷酸延伸到RNA中第42位残基的5'端,在体外消除了(T4G4)3和(G4T4)3引物的延伸。相反,在第42位和第50位残基之间终止的寡核苷酸(第2类和第3类)作为有效的端粒酶引物。我们得出结论,嗜热四膜虫模板由190个核苷酸RNA中的第42位至第50位残基组成,这与粗壮真核游仆虫酶所使用的核苷酸不同。第2类引物反应积累了短产物,并且通过改变引物的5'序列可以降低它们的丰度,这与端粒酶的双引物结合位点模型一致。第3类引物产生了短产物和长产物双峰分布,每种产物都有独特的延伸谱。长产物谱与序列特异性引物比对不一致。相反,每个引物都由相同的TTTTGGGG重复序列延伸,表明穿梭到模板内的默认位置。文中讨论了端粒酶与RNA聚合酶延伸机制之间的相似之处。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5b22/359322/eabe1adc0858/molcellb00012-0161-a.jpg

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