Eukaryotic gene invasion by a bacterial mobile insertion sequence element IS2 during cloning into a plasmid vector.

Q4 Biochemistry, Genetics and Molecular Biology Genome Integrity Pub Date : 2010-05-26 DOI:10.1186/2041-9414-1-2
Alireza G Senejani, Joann B Sweasy
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引用次数: 2

Abstract

Escherichia coli (E. coli) are commonly used as hosts for DNA cloning and sequencing. Upon transformation of E. coli with recombined vector carrying a gene of interest, the bacteria multiply the gene of interest while maintaining the integrity of its content. During the subcloning of a mouse genomic fragment into a plasmid vector, we noticed that the size of the insert increased significantly upon replication in E. coli. The sequence of the insert was determined and found to contain a novel DNA sequence within the mouse genomic insert. A BLAST search of GenBank revealed the novel sequence to be that of the Insertion Sequence 2 (IS2) element from E. coli that was likely inserted during replication in that organism. Importantly, a detailed search of GenBank shows that the IS2 is present within many eukaryotic nucleotide sequences, and in many cases, has been annotated as being part of the protein. The results of this study suggest that one must perform additional careful analysis of the sequence results using BLAST comparisons, and further verification of gene annotation before submission into the GenBank.

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细菌移动插入序列元件IS2在质粒载体克隆过程中的真核基因入侵。
大肠杆菌通常被用作DNA克隆和测序的宿主。在大肠杆菌与重组载体携带感兴趣的基因转化后,细菌繁殖感兴趣的基因,同时保持其内容的完整性。在将小鼠基因组片段亚克隆到质粒载体的过程中,我们注意到插入物的大小在大肠杆菌中复制后显着增加。该插入物的序列被确定并发现在小鼠基因组插入物中包含一个新的DNA序列。对GenBank进行BLAST搜索发现,该新序列是来自大肠杆菌的插入序列2 (IS2)元件,可能是在该生物体的复制过程中插入的。重要的是,对GenBank的详细搜索表明,IS2存在于许多真核生物核苷酸序列中,并且在许多情况下,已被注释为蛋白质的一部分。本研究的结果表明,在提交到GenBank之前,必须使用BLAST比较对序列结果进行额外的仔细分析,并进一步验证基因注释。
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Genome Integrity
Genome Integrity Biochemistry, Genetics and Molecular Biology-Genetics
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