Literature DB >> 27146086

Function, expression, specificity, diversity and incompatibility of actinobacteriophage parABS systems.

Rebekah M Dedrick1, Travis N Mavrich1, Wei L Ng1, Juan C Cervantes Reyes1, Matthew R Olm1, Rachael E Rush1, Deborah Jacobs-Sera1, Daniel A Russell1, Graham F Hatfull1.   

Abstract

More than 180 individual phages infecting hosts in the phylum Actinobacteria have been sequenced and grouped into Cluster A because of their similar overall nucleotide sequences and genome architectures. These Cluster A phages are either temperate or derivatives of temperate parents, and most have an integration cassette near the centre of the genome containing an integrase gene and attP. However, about 20% of the phages lack an integration cassette, which is replaced by a 1.4 kbp segment with predicted partitioning functions, including plasmid-like parA and parB genes. Phage RedRock forms stable lysogens in Mycobacterium smegmatis in which the prophage replicates at 2.4 copies/chromosome and the partitioning system confers prophage maintenance. The parAB genes are expressed upon RedRock infection of M. smegmatis, but are downregulated once lysogeny is established by binding of RedRock ParB to parS-L, one of two centromere-like sites flanking the parAB genes. The RedRock parS-L and parS-R sites are composed of eight directly repeated copies of an 8 bp motif that is recognized by ParB. The actinobacteriophage parABS cassettes span considerable sequence diversity and specificity, providing a suite of tools for use in mycobacterial genetics.
© 2016 John Wiley & Sons Ltd.

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Year:  2016        PMID: 27146086      PMCID: PMC4998052          DOI: 10.1111/mmi.13414

Source DB:  PubMed          Journal:  Mol Microbiol        ISSN: 0950-382X            Impact factor:   3.501


  70 in total

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Review 5.  Chromosome replication and segregation in bacteria.

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8.  Evolution of Superinfection Immunity in Cluster A Mycobacteriophages.

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