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框架:基因组测序错误的检测

Frame: detection of genomic sequencing errors.

作者信息

Brown N P, Sander C, Bork P

机构信息

1European Bioinformatics Institute (EMBL-EBI), Wellcome Genome Campus, Cambridge, CB10 1SD, UK.

出版信息

Bioinformatics. 1998;14(4):367-71. doi: 10.1093/bioinformatics/14.4.367.

Abstract

MOTIVATION

The underlying error rate for genomic sequencing sometimes results in the introduction of artificial frameshifts and in-frame stop codons into putative protein encoding genes. Severe errors are then introduced into the inferred transcripts through mis-translation or premature termination.

RESULTS

We describe a system for screening segments of DNA for frameshift and in-frame stop errors in coding regions. The method is based on homology matching using blastx to compare all six reading frames of the query nucleotide sequence against selected protein sequence databases. Fragments of protein matching neighbouring regions of the query DNA are united and extended laterally to define candidate open reading frames, within which, frameshifts and stops are identified. Suitable targets include prokaryotic or other intron-free genomic sequence and complementary DNAs. As an example of its use, we report here two frameshifted ORFs that deviate from the original TIGR sequence annotations for the recently released Helicobacter pylori genome.

AVAILABILITY

The tool is accessible via the URL http://www.sander.ebi.ac.uk/frame/.

CONTACT

brown@ebi.ac.uk.

摘要

动机

基因组测序的潜在错误率有时会导致在假定的蛋白质编码基因中引入人为的移码突变和框内终止密码子。然后,通过错误翻译或提前终止,严重错误会被引入到推断的转录本中。

结果

我们描述了一种用于筛选DNA片段中编码区移码突变和框内终止错误的系统。该方法基于使用blastx进行同源匹配,将查询核苷酸序列的所有六个阅读框与选定的蛋白质序列数据库进行比较。与查询DNA相邻区域匹配的蛋白质片段被合并并横向扩展,以定义候选开放阅读框,在其中识别移码突变和终止密码子。合适的目标包括原核生物或其他无内含子的基因组序列以及互补DNA。作为其应用的一个例子,我们在此报告了两个移码的开放阅读框,它们与最近发布的幽门螺杆菌基因组的原始TIGR序列注释不同。

可用性

该工具可通过网址http://www.sander.ebi.ac.uk/frame/访问。

联系方式

brown@ebi.ac.uk

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