Your search keyword '"P Scott Hefty"' showing total 5 results

1. Chromosomal Recombination Targets in Chlamydia Interspecies Lateral Gene Transfer

Author

Yibing Wang, Robert J. Suchland, Debbie B. Kim, Kevin Hybiske, Zoe E. Dimond, Steven J. Carrell, P. Scott Hefty, and Daniel D. Rockey

Subjects

Transposable element, Chlamydia muridarum, Gene Transfer, Horizontal, Chlamydia trachomatis, Biology, medicine.disease_cause, Microbiology, Genome, law.invention, 03 medical and health sciences, Plasmid, law, medicine, Molecular Biology, Crosses, Genetic, 030304 developmental biology, Recombination, Genetic, Genetics, 0303 health sciences, Base Sequence, 030306 microbiology, Genetic transfer, Tetracycline Resistance, Chromosome, Gene Expression Regulation, Bacterial, Chromosomes, Bacterial, Tetracycline, Anti-Bacterial Agents, Horizontal gene transfer, DNA Transposable Elements, Recombinant DNA, Research Article, Plasmids

Abstract

Lateral gene transfer (LGT) among Chlamydia trachomatis strains is common, in both isolates generated in the laboratory and those examined directly from patients. In contrast, there are very few examples of recent acquisition of DNA by any Chlamydia spp. from any other species. Interspecies LGT in this system was analyzed using crosses of tetracycline (Tc)-resistant C. trachomatis L2/434 and chloramphenicol (Cam)-resistant C. muridarum VR-123. Parental C. muridarum strains were created using a plasmid-based Himar transposition system, which led to integration of the Camr marker randomly across the chromosome. Fragments encompassing 79% of the C. muridarum chromosome were introduced into a C. trachomatis background, with the total coverage contained on 142 independent recombinant clones. Genome sequence analysis of progeny strains identified candidate recombination hot spots, a property not consistent with in vitroC. trachomatis × C. trachomatis (intraspecies) crosses. In both interspecies and intraspecies crosses, there were examples of duplications, mosaic recombination endpoints, and recombined sequences that were not linked to the selection marker. Quantitative analysis of the distribution and constitution of inserted sequences indicated that there are different constraints on interspecies LGT than on intraspecies crosses. These constraints may help explain why there is so little evidence of interspecies genetic exchange in this system, which is in contrast to very widespread intraspecies exchange in C. trachomatis. IMPORTANCE Genome sequence analysis has demonstrated that there is widespread lateral gene transfer among strains within the species C. trachomatis and with other closely related Chlamydia species in laboratory experiments. This is in contrast to the complete absence of foreign DNA in the genomes of sequenced clinical C. trachomatis strains. There is no understanding of any mechanisms of genetic transfer in this important group of pathogens. In this report, we demonstrate that interspecies genetic exchange can occur but that the nature of the fragments exchanged is different than those observed in intraspecies crosses. We also generated a large hybrid strain library that can be exploited to examine important aspects of chlamydial disease.

Published

2019

2. Development of Transposon Mutagenesis for Chlamydia muridarum

Author

Scott D. LaBrie, Yibing Wang, Zoe E. Dimond, Robert J. Suchland, Forrest Kwong, P. Scott Hefty, Kevin Hybiske, Steven J. Carrell, and Daniel D. Rockey

Subjects

Transposable element, Chlamydia muridarum, Mutant, Microbiology, Genome, 03 medical and health sciences, Mice, Open Reading Frames, Bacterial Proteins, Animals, ORFS, Molecular Biology, Gene, 030304 developmental biology, Gene Library, Genetics, 0303 health sciences, biology, Base Sequence, Whole Genome Sequencing, 030306 microbiology, Chlamydia Infections, Chromosomes, Bacterial, biology.organism_classification, Phenotype, Anti-Bacterial Agents, Clone Cells, Chloramphenicol, Mutagenesis, Mutation, DNA Transposable Elements, Transposon mutagenesis, Plasmids, Research Article

Abstract

Functional genetic analysis of Chlamydia has been a challenge due to the historical genetic intractability of Chlamydia, although recent advances in chlamydial genetic manipulation have begun to remove these barriers. Here, we report the development of the Himar C9 transposon system for Chlamydia muridarum, a mouse-adapted Chlamydia species that is widely used in Chlamydia infection models. We demonstrate the generation and characterization of an initial library of 33 chloramphenicol (Cam)-resistant, green fluorescent protein (GFP)-expressing C. muridarum transposon mutants. The majority of the mutants contained single transposon insertions spread throughout the C. muridarum chromosome. In all, the library contained 31 transposon insertions in coding open reading frames (ORFs) and 7 insertions in intergenic regions. Whole-genome sequencing analysis of 17 mutant clones confirmed the chromosomal locations of the insertions. Four mutants with transposon insertions in glgB, pmpI, pmpA, and pmpD were investigated further for in vitro and in vivo phenotypes, including growth, inclusion morphology, and attachment to host cells. The glgB mutant was shown to be incapable of complete glycogen biosynthesis and accumulation in the lumen of mutant inclusions. Of the 3 pmp mutants, pmpI was shown to have the most pronounced growth attenuation defect. This initial library demonstrates the utility and efficacy of stable, isogenic transposon mutants for C. muridarum. The generation of a complete library of C. muridarum mutants will ultimately enable comprehensive identification of the functional genetic requirements for Chlamydia infection in vivo. IMPORTANCE Historical issues with genetic manipulation of Chlamydia have prevented rigorous functional genetic characterization of the ∼1,000 genes in chlamydial genomes. Here, we report the development of a transposon mutagenesis system for C. muridarum, a mouse-adapted Chlamydia species that is widely used for in vivo investigations of chlamydial pathogenesis. This advance builds on the pioneering development of this system for C. trachomatis. We demonstrate the generation of an initial library of 33 mutants containing stable single or double transposon insertions. Using these mutant clones, we characterized in vitro phenotypes associated with genetic disruptions in glycogen biosynthesis and three polymorphic outer membrane proteins.

Published

2019

3. Interrogating Genes That Mediate Chlamydia trachomatis Survival in Cell Culture Using Conditional Mutants and Recombination

Author

P. Scott Hefty, Michael L. Barta, Evelyn Toh, Julie A. Brothwell, Daniel D. Rockey, Matthew K. Muramatsu, Timothy E. Putman, David E. Nelson, and Robert J. Suchland

Subjects

0301 basic medicine, Sexually transmitted disease, Genotype, 030106 microbiology, Mutant, Population, Chlamydia trachomatis, Biology, medicine.disease_cause, Microbiology, Genome, 03 medical and health sciences, medicine, Humans, education, Molecular Biology, Gene, Alleles, Recombination, Genetic, Genetics, education.field_of_study, Temperature, Gene Expression Regulation, Bacterial, Articles, Phenotype, Mutation, Genome, Bacterial, HeLa Cells, Genetic screen

Abstract

Intracellular bacterial pathogens in the family Chlamydiaceae are causes of human blindness, sexually transmitted disease, and pneumonia. Genetic dissection of the mechanisms of chlamydial pathogenicity has been hindered by multiple limitations, including the inability to inactivate genes that would prevent the production of elementary bodies. Many genes are also Chlamydia -specific genes, and chlamydial genomes have undergone extensive reductive evolution, so functions often cannot be inferred from homologs in other organisms. Conditional mutants have been used to study essential genes of many microorganisms, so we screened a library of 4,184 ethyl methanesulfonate-mutagenized Chlamydia trachomatis isolates for temperature-sensitive (TS) mutants that developed normally at physiological temperature (37°C) but not at nonphysiological temperatures. Heat-sensitive TS mutants were identified at a high frequency, while cold-sensitive mutants were less common. Twelve TS mutants were mapped using a novel markerless recombination approach, PCR, and genome sequencing. TS alleles of genes that play essential roles in other bacteria and chlamydia-specific open reading frames (ORFs) of unknown function were identified. Temperature-shift assays determined that phenotypes of the mutants manifested at distinct points in the developmental cycle. Genome sequencing of a larger population of TS mutants also revealed that the screen had not reached saturation. In summary, we describe the first approach for studying essential chlamydial genes and broadly applicable strategies for genetic mapping in Chlamydia spp. and mutants that both define checkpoints and provide insights into the biology of the chlamydial developmental cycle. IMPORTANCE Study of the pathogenesis of Chlamydia spp. has historically been hampered by a lack of genetic tools. Although there has been recent progress in chlamydial genetics, the existing approaches have limitations for the study of the genes that mediate growth of these organisms in cell culture. We used a genetic screen to identify conditional Chlamydia mutants and then mapped these alleles using a broadly applicable recombination strategy. Phenotypes of the mutants provide fundamental insights into unexplored areas of chlamydial pathogenesis and intracellular biology. Finally, the reagents and approaches we describe are powerful resources for the investigation of these organisms.

Published

2016

4. Ab initio structural modeling of and experimental validation for Chlamydia trachomatis protein CT296 reveal structural similarity to Fe(II) 2-oxoglutarate-dependent enzymes

Author

P. Scott Hefty, Kyle Evan Kemege, Yang Zhang, John M. Hickey, Kevin P. Battaile, and Scott Lovell

Subjects

Models, Molecular, Structural similarity, Hypothetical protein, Molecular Sequence Data, Ab initio, Repressor, Chlamydia trachomatis, Biology, Crystallography, X-Ray, Microbiology, Open reading frame, Protein structure, Biochemistry, Bacterial Proteins, Structural Biology, Amino Acid Sequence, Molecular Biology, Root-mean-square deviation, Peptide sequence

Abstract

Chlamydia trachomatis is a medically important pathogen that encodes a relatively high percentage of proteins with unknown function. The three-dimensional structure of a protein can be very informative regarding the protein's functional characteristics; however, determining protein structures experimentally can be very challenging. Computational methods that model protein structures with sufficient accuracy to facilitate functional studies have had notable successes. To evaluate the accuracy and potential impact of computational protein structure modeling of hypothetical proteins encoded by Chlamydia, a successful computational method termed I-TASSER was utilized to model the three-dimensional structure of a hypothetical protein encoded by open reading frame (ORF) CT296. CT296 has been reported to exhibit functional properties of a divalent cation transcription repressor (DcrA), with similarity to the Escherichia coli iron-responsive transcriptional repressor, Fur. Unexpectedly, the I-TASSER model of CT296 exhibited no structural similarity to any DNA-interacting proteins or motifs. To validate the I-TASSER-generated model, the structure of CT296 was solved experimentally using X-ray crystallography. Impressively, the ab initio I-TASSER-generated model closely matched (2.72-Å C(α) root mean square deviation [RMSD]) the high-resolution (1.8-Å) crystal structure of CT296. Modeled and experimentally determined structures of CT296 share structural characteristics of non-heme Fe(II) 2-oxoglutarate-dependent enzymes, although key enzymatic residues are not conserved, suggesting a unique biochemical process is likely associated with CT296 function. Additionally, functional analyses did not support prior reports that CT296 has properties shared with divalent cation repressors such as Fur.

Published

2011

5. Chlamydial type III secretion system is encoded on ten operons preceded by sigma 70-like promoter elements

Author

P. Scott Hefty and Richard S. Stephens

Subjects

Genetics, Molecular Biology of Pathogens, Operon, Genetic Linkage, Virulence Factors, Repressor, Virulence, Chlamydia trachomatis, Sigma Factor, DNA-Directed RNA Polymerases, Biology, Microbiology, Type three secretion system, Bacterial Proteins, Sigma factor, Gene expression, Secretion, Transcription Initiation Site, Promoter Regions, Genetic, Molecular Biology, Gene

Abstract

Many gram-negative bacterial pathogens employ type III secretion systems for infectious processes. Chlamydiae are obligate intracellular bacteria that encode a conserved type III secretion system that is likely requisite for growth. Typically, genes encoding type III secretion systems are located in a single locus; however, for chlamydiae these genes are scattered throughout the genome. Little is known regarding the gene regulatory mechanisms for this essential virulence determinant. To facilitate identification of cis -acting transcriptional regulatory elements, the operon structure was determined. This analysis revealed 10 operons that contained 37 genes associated with the type III secretion system. Linkage within these operons suggests a role in type III secretion for each of these genes, including 13 genes encoding proteins with unknown function. The transcriptional start site for each operon was determined. In conjunction with promoter activity assays, this analysis revealed that the type III secretion system operons encode σ 70 -like promoter elements. Transcriptional initiation by a sigma factor responsible for constitutive gene expression indicates that undefined activators or repressors regulate developmental stage-specific expression of chlamydial type III secretion system genes.

Published

2006