Literature DB >> 16109950

Gene organization and transcriptional analysis of the tprJ, tprI, tprG, and tprF loci in Treponema pallidum strains Nichols and Sea 81-4.

Lorenzo Giacani1, Karin Hevner, Arturo Centurion-Lara.   

Abstract

The tpr gene family of Treponema pallidum subsp. pallidum, the causative agent of syphilis, has recently become the focus of intensive investigation. TprF and TprI sequences are highly conserved among different isolates and are the targets of strong humoral and cellular immune responses of the host, and immunization with a recombinant peptide from the amino terminus of these antigens has been shown to alter significantly lesion development following homologous challenge. This indicates that these antigens are expressed during infection and strongly suggests a key functionality. tprF and tprI are located immediately downstream of the tprG and tprJ genes, respectively, separated by very short intergenic spacers (55 nucleotides for G-F and 56 nucleotides for J-I). Preliminary analysis using gene-specific primers failed to amplify tprJ in the Sea 81-4 isolate. In this study, sequence and transcriptional analysis of these loci showed a similar gene organization in the Nichols and Sea 81-4 strains, a complex pattern of transcription, and the presence of G homopolymeric repeats of variable lengths upstream of the tprF, tprI, tprG, and tprJ transcriptional start sites. However, distinctive features were also identified in the Sea 81-4 isolate, including a tprG-like open reading frame in the tprJ locus, a frameshift and a premature termination in the tprG coding sequence, a longer tprG-tprF intergenic spacer, and absence of cotranscription of the tprG-tprF genes.

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Year:  2005        PMID: 16109950      PMCID: PMC1196134          DOI: 10.1128/JB.187.17.6084-6093.2005

Source DB:  PubMed          Journal:  J Bacteriol        ISSN: 0021-9193            Impact factor:   3.490


  21 in total

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4.  Expression in Escherichia coli of the 37-kilodalton endoflagellar sheath protein of Treponema pallidum by use of the polymerase chain reaction and a T7 expression system.

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5.  Compilation of E. coli mRNA promoter sequences.

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  16 in total

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2.  Length of guanosine homopolymeric repeats modulates promoter activity of subfamily II tpr genes of Treponema pallidum ssp. pallidum.

Authors:  Lorenzo Giacani; Sheila Lukehart; Arturo Centurion-Lara
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Review 3.  The endemic treponematoses.

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4.  Quantitative analysis of tpr gene expression in Treponema pallidum isolates: Differences among isolates and correlation with T-cell responsiveness in experimental syphilis.

Authors:  Lorenzo Giacani; Barbara Molini; Charmie Godornes; Lynn Barrett; Wesley Van Voorhis; Arturo Centurion-Lara; Sheila A Lukehart
Journal:  Infect Immun       Date:  2006-10-09       Impact factor: 3.441

5.  Antigenic variation in Treponema pallidum: TprK sequence diversity accumulates in response to immune pressure during experimental syphilis.

Authors:  Lorenzo Giacani; Barbara J Molini; Eric Y Kim; B Charmie Godornes; B Troy Leader; Lauren C Tantalo; Arturo Centurion-Lara; Sheila A Lukehart
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6.  Transcription of TP0126, Treponema pallidum putative OmpW homolog, is regulated by the length of a homopolymeric guanosine repeat.

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7.  Identification of the Treponema pallidum subsp. pallidum TP0092 (RpoE) regulon and its implications for pathogen persistence in the host and syphilis pathogenesis.

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8.  Treponema pallidum, the stealth pathogen, changes, but how?

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10.  Genetic engineering of Treponema pallidum subsp. pallidum, the Syphilis Spirochete.

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