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大肠杆菌K-12基因组中λ样原噬菌体元件e14的分析。

Analysis of the lambdoid prophage element e14 in the E. coli K-12 genome.

作者信息

Mehta Preeti, Casjens Sherwood, Krishnaswamy Sankaran

机构信息

Bioinformatics Centre, School of Biotechnology, Madurai Kamaraj University, Madurai-625021, India.

出版信息

BMC Microbiol. 2004 Jan 20;4:4. doi: 10.1186/1471-2180-4-4.

Abstract

BACKGROUND

Many sequenced bacterial genomes harbor phage-like elements or cryptic prophages. These elements have been implicated in pathogenesis, serotype conversion and phage immunity. The e14 element is a defective lambdoid prophage element present at 25 min in the E. coli K-12 genome. This prophage encodes important functional genes such as lit (T4 exclusion), mcrA (modified cytosine restriction activity) and pin (recombinase).

RESULTS

Bioinformatic analysis of the e14 prophage sequence shows the modular nature of the e14 element which shares a large part of its sequence with the Shigella flexneri phage SfV. Based on this similarity, the regulatory region including the repressor and Cro proteins and their binding sites were identified. The protein product of b1149 was found to be a fusion of a replication protein and a terminase. The genes b1143, b1151 and b1152 were identified as putative pseudogenes. A number of duplications of the stfE tail fibre gene of the e14 are seen in plasmid p15B. A protein based comparative approach using the COG database as a starting point helped detect lambdoid prophage like elements in a representative set of completely sequenced genomes.

CONCLUSIONS

The e14 element was characterized for the function of its encoded genes, the regulatory regions, replication origin and homology with other phage and bacterial sequences. Comparative analysis at nucleotide and protein levels suggest that a number of important phage related functions are missing in the e14 genome including parts of the early left operon, early right operon and late operon. The loss of these genes is the result of at least three major deletions that have occurred on e14 since its integration. A comparative protein level approach using the COG database can be effectively used to detect defective lambdoid prophage like elements in bacterial genomes.

摘要

背景

许多已测序的细菌基因组中含有噬菌体样元件或隐匿性原噬菌体。这些元件与发病机制、血清型转换及噬菌体免疫有关。e14元件是存在于大肠杆菌K-12基因组25分钟处的一个缺陷性λ样原噬菌体元件。该原噬菌体编码重要的功能基因,如lit(T4排除)、mcrA(修饰胞嘧啶限制活性)和pin(重组酶)。

结果

对e14原噬菌体序列的生物信息学分析显示了e14元件的模块化性质,其序列的很大一部分与福氏志贺氏菌噬菌体SfV相同。基于这种相似性,鉴定出了包括阻遏蛋白和Cro蛋白及其结合位点的调控区域。发现b1149的蛋白质产物是一种复制蛋白和一种末端酶的融合体。基因b1143、b1151和b1152被鉴定为假定的假基因。在质粒p15B中可见e14的stfE尾丝基因的多个重复。以COG数据库为起点的基于蛋白质的比较方法有助于在一组代表性的完全测序基因组中检测λ样原噬菌体样元件。

结论

对e14元件的编码基因功能、调控区域、复制起点以及与其他噬菌体和细菌序列的同源性进行了表征。核苷酸和蛋白质水平的比较分析表明,e14基因组中缺少许多重要的噬菌体相关功能,包括早期左操纵子、早期右操纵子和晚期操纵子的部分区域。这些基因的缺失是e14自整合以来至少发生三次主要缺失的结果。使用COG数据库的比较蛋白质水平方法可有效用于检测细菌基因组中的缺陷性λ样原噬菌体样元件。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9359/331406/aa1a86b2d872/1471-2180-4-4-1.jpg

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