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Dive into the research topics where Janelle M. Hare is active.

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Featured researches published by Janelle M. Hare.


Molecular Microbiology | 1999

Independent acquisition and insertion into different chromosomal locations of the same pathogenicity island in Yersinia pestis and Yersinia pseudotuberculosis

Janelle M. Hare; Alexandra K. Wagner; Kathleen A. McDonough

We show that Yersinia pestis and pesticin‐sensitive isolates of Y. pseudotuberculosis possess a common 34 kbp DNA region that has all the hallmarks of a pathogenicity island and is inserted into different asparaginyl tRNA genes at different chromosomal locations in each species. This pathogenicity island (YP‐HPI) is marked by IS100, has a G + C content different from its host, is flanked by 24 bp direct repeats, encodes a putative, P4‐like integrase and contains the iron uptake virulence genes from the pgm locus of Y. pestis. These findings indicate independent horizontal acquisition of this island by Y. pestis and Y. pseudotuberculosis. The two YP‐HPI locations and their possession of an integrase gene support a model of site‐specific integration of the YP‐HPI into these bacteria.


PLOS ONE | 2016

UmuDAb: An Error-Prone Polymerase Accessory Homolog Whose N-Terminal Domain Is Required for Repression of DNA Damage Inducible Gene Expression in Acinetobacter baylyi

Travis A. Witkowski; Alison N. Grice; DeAnna B. Stinnett; Whitney K. Wells; Megan A. Peterson; Janelle M. Hare

In many bacteria, the DNA damage response induces genes (SOS genes) that were repressed by LexA. LexA represses transcription by binding to SOS promoters via a helix-turn-helix motif in its N-terminal domain (NTD). Upon DNA damage, LexA cleaves itself and allows induction of transcription. In Acinetobacter baumannii and Acinetobacter baylyi, multiple genes are induced by DNA damage, and although the Acinetobacter genus lacks LexA, a homolog of the error-prone polymerase subunit UmuD, called UmuDAb, regulates some DNA damage-induced genes. The mechanism of UmuDAb regulation has not been determined. We constructed UmuDAb mutant strains of A. baylyi to test whether UmuDAb mediates gene regulation through LexA-like repressor actions consisting of relief of repression through self-cleavage after DNA damage. Real-time quantitative PCR experiments in both a null umuDAb mutant and an NTD mutant showed that the DNA damage-inducible, UmuDAb-regulated gene ddrR was highly expressed even in the absence of DNA damage. Protein modeling identified a potential LexA-like helix-turn-helix structure in the UmuDAb NTD, which when disrupted, also relieved ddrR and umuDAb repression under non-inducing conditions. Mutations in a putative SOS box in the shared umuDAb-ddrR promoter region similarly relieved these genes’ repression under non-inducing conditions. Conversely, cells possessing a cleavage-deficient UmuDAb were unable to induce gene expression after MMC-mediated DNA damage. This evidence of a UmuDAb repressor mechanism was contrasted with the failure of umuDAb to complement an Escherichia coli umuD mutant for UmuD error-prone DNA replication activity. Similarly, A. baumannii null umuDAb mutant cells did not have a reduced UmuDˊ2UmuC-mediated mutation rate after DNA damage, suggesting that although this UmuDAb protein may have evolved from a umuDC operon in this genus, it now performs a LexA-like repressor function for a sub-set of DNA damage-induced genes.


Archive | 2013

Sabouraud Agar for Fungal Growth

Janelle M. Hare

This article describes the history, theory, and use of Sabouraud agar for isolating and growing fungi. This includes an explanation of the role of each ingredient, the instructions for making this medium, variations upon the basic recipe, and the various recipes that are commercially available.


Proceedings of the National Academy of Sciences of the United States of America | 2005

Dissecting the PhoP regulatory network of Escherichia coli and Salmonella enterica

Igor Zwir; Dongwoo Shin; Akinori Kato; Kunihiko Nishino; Tammy Latifi; Felix Solomon; Janelle M. Hare; Henry V. Huang; Eduardo A. Groisman


Journal of Bacteriology | 1999

High-Frequency RecA-Dependent and -Independent Mechanisms of Congo Red Binding Mutations in Yersinia pestis

Janelle M. Hare; Kathleen A. McDonough


Journal of Bacteriology | 1997

Homology with a repeated Yersinia pestis DNA sequence IS100 correlates with pesticin sensitivity in Yersinia pseudotuberculosis.

Kathleen A. McDonough; Janelle M. Hare


Microbiology | 2012

Diverse responses to UV light exposure in Acinetobacter include the capacity for DNA damage-induced mutagenesis in the opportunistic pathogens Acinetobacter baumannii and Acinetobacter ursingii

Janelle M. Hare; James A. Bradley; Ching-li Lin; Tyler J. Elam


PLOS ONE | 2014

Prophage Induction and Differential RecA and UmuDAb Transcriptome Regulation in the DNA Damage Responses of Acinetobacter baumannii and Acinetobacter baylyi

Janelle M. Hare; Joshua C. Ferrell; Travis A. Witkowski; Alison N. Grice


Fems Microbiology Letters | 2012

The Acinetobacter regulatory UmuDAb protein cleaves in response to DNA damage with chimeric LexA/UmuD characteristics

Janelle M. Hare; Sabal Adhikari; Kasandra V. Lambert; Alexander E. Hare; Alison N. Grice


Archive | 2008

Sabouraud Agar for Fungal Growth Protocols

Janelle M. Hare

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Alison N. Grice

Morehead State University

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Kathleen A. McDonough

New York State Department of Health

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Alexandra K. Wagner

New York State Department of Health

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Ching-li Lin

Morehead State University

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Dongwoo Shin

Washington University in St. Louis

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Felix Solomon

Washington University in St. Louis

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