Laura Sampson scite author profile

SummaryBacteria of the spirochaete genus Borrelia have linear chromosomes about 950 kbp in size. We report here that these linear chromosomes have covalently closed hairpin structures at their termini that are similar but not identical to those reported for linear plasmids carried by these organisms. Nucleotide sequence analysis of the chromosomal telomeric regions indicates that unique, apparently functional genes lie within a few hundred bp of each of the telomeres, and that there is an imperfect 26 bp inverted repeat at the two telomeres. In addition, we characterize a major chromosomal length polymorphism within the right telomeric regions of various Borrelia isolates, and show that sequences similar to those near the right telomere are often found on linear plasmids in B. burgdorferi (sensu stricto) isolates from nature. Sequences similar to a number of other regions of the chromosome, including those near the left telomere, were not found on B. burgdorferi plasmids. These observations suggest that there has been historical exchange of genetic information between the linear plasmids and the right end of the linear chromosome.

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Molecular Genetics of Bacteriophage P22 Scaffolding Protein's Functional Domains

Weigele

Sampson

Winn-Stapley

et al. 2005

Journal of Molecular Biology

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The DNA site utilized by bacteriophage P22 for initiation of DNA packaging

Sampson

Parr

et al. 2002

Molecular Microbiology

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SummaryVirion proteins recognize their cognate nucleic acid for encapsidation into virions through recognition of a specific nucleotide sequence contained within that nucleic acid. Viruses like bacteriophage P22, which have partially circularly permuted, double-stranded virion DNAs, encapsidate DNA through processive series of packaging events in which DNA is recognized for packaging only once at the beginning of the series. Thus a single DNA recognition event programmes the encapsidation of multiple virion chromosomes. The protein product of P22 gene 3 , a terminase component, is thought to be responsible for this recognition. The site on the P22 genome that is recognized by the gene 3 protein to initiate packaging series is called the pac site. We report here a strategy for assaying pac site activity in vivo , and the utilization of this system to identify and characterize the site genetically. It is an asymmetric site that spans 22 basepairs and is located near the centre of P22 gene 3 .

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Bacteriophage P22 portal protein is part of the gauge that regulates packing density of intravirion DNA

Casjens¹,

Wyckoff²,

Hayden³

et al. 1992

Journal of Molecular Biology

106

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A helical coat protein recognition domain of the bacteriophage P22 scaffolding protein

Tůma

Parker

Weigele

et al. 1998

Journal of Molecular Biology

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Laura Sampson

Telomeres of the linear chromosomes of Lyme disease spirochaetes: nucleotide sequence and possible exchange with linear plasmid telomeres

Molecular Genetics of Bacteriophage P22 Scaffolding Protein's Functional Domains

The DNA site utilized by bacteriophage P22 for initiation of DNA packaging

Bacteriophage P22 portal protein is part of the gauge that regulates packing density of intravirion DNA

A helical coat protein recognition domain of the bacteriophage P22 scaffolding protein

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