Virulence gene expression in vivo

Samuel A. Shelburne; James M. Musser

doi:10.1016/j.mib.2004.04.013

Virulence gene expression in vivo

Samuel A. Shelburne, James M. Musser

Research output: Contribution to journal › Review article › peer-review

21 Scopus citations

Abstract

The ability to identify and isolate bacterial RNA from animals or humans with infections has markedly advanced the capacity to examine microbial gene expression in vivo. This advance has been coupled with the development of quantitative real-time reverse transcription polymerase chain reaction and expression microarrays to allow investigators to accurately measure how organisms are manipulating their genetic expression during actual infections. Though the full ramifications of these technologies have yet to be realized, they promise to open new avenues of therapeutics for a broad range of infectious diseases by allowing researchers to focus on in vivo expressed genes. These developments provide a framework for efficient utilization of the vast amount of information being generated by the accelerating pace of genomic sequencing of microbes.

Original language	English (US)
Pages (from-to)	283-289
Number of pages	7
Journal	Current Opinion in Microbiology
Volume	7
Issue number	3
DOIs	https://doi.org/10.1016/j.mib.2004.04.013
State	Published - Jun 2004
Externally published	Yes

Keywords

DECAL
GAS
IVET
OspA
QRT-PCR
RT-PCR
differential expression analysis using a custom-amplified library
gfp
green fluorescent protein
group A Streptococcus
in vitro expression technology
outer surface protein A
quantitative RT-PCR

ASJC Scopus subject areas

Microbiology
Microbiology (medical)
Infectious Diseases

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10.1016/j.mib.2004.04.013

Cite this

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title = "Virulence gene expression in vivo",

abstract = "The ability to identify and isolate bacterial RNA from animals or humans with infections has markedly advanced the capacity to examine microbial gene expression in vivo. This advance has been coupled with the development of quantitative real-time reverse transcription polymerase chain reaction and expression microarrays to allow investigators to accurately measure how organisms are manipulating their genetic expression during actual infections. Though the full ramifications of these technologies have yet to be realized, they promise to open new avenues of therapeutics for a broad range of infectious diseases by allowing researchers to focus on in vivo expressed genes. These developments provide a framework for efficient utilization of the vast amount of information being generated by the accelerating pace of genomic sequencing of microbes.",

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AU - Shelburne, Samuel A.

AU - Musser, James M.

PY - 2004/6

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N2 - The ability to identify and isolate bacterial RNA from animals or humans with infections has markedly advanced the capacity to examine microbial gene expression in vivo. This advance has been coupled with the development of quantitative real-time reverse transcription polymerase chain reaction and expression microarrays to allow investigators to accurately measure how organisms are manipulating their genetic expression during actual infections. Though the full ramifications of these technologies have yet to be realized, they promise to open new avenues of therapeutics for a broad range of infectious diseases by allowing researchers to focus on in vivo expressed genes. These developments provide a framework for efficient utilization of the vast amount of information being generated by the accelerating pace of genomic sequencing of microbes.

AB - The ability to identify and isolate bacterial RNA from animals or humans with infections has markedly advanced the capacity to examine microbial gene expression in vivo. This advance has been coupled with the development of quantitative real-time reverse transcription polymerase chain reaction and expression microarrays to allow investigators to accurately measure how organisms are manipulating their genetic expression during actual infections. Though the full ramifications of these technologies have yet to be realized, they promise to open new avenues of therapeutics for a broad range of infectious diseases by allowing researchers to focus on in vivo expressed genes. These developments provide a framework for efficient utilization of the vast amount of information being generated by the accelerating pace of genomic sequencing of microbes.

KW - DECAL

KW - GAS

KW - IVET

KW - OspA

KW - QRT-PCR

KW - RT-PCR

KW - differential expression analysis using a custom-amplified library

KW - gfp

KW - green fluorescent protein

KW - group A Streptococcus

KW - in vitro expression technology

KW - outer surface protein A

KW - quantitative RT-PCR

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JO - Current Opinion in Microbiology

JF - Current Opinion in Microbiology

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ER -

Virulence gene expression in vivo

Abstract

Keywords

ASJC Scopus subject areas

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