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Infectious Disorders - Drug Targets
(Formerly 'Current Drug Targets - Infectious Disorders')
ISSN: 1871-5265
Infectious Disorders
– Drug Targets
Volume 6, Number 3, September 2006
Contents
Differentially Regulated Genes to Understand Microbial
Pathogenesis and for the Development of New Vaccine, Diagnostic
and Antibiotherapy Strategies
Guest Editor: Dr. Martin Handfield
Editorial Pp.
205-206
Development and Application of In Vivo
Expression Technology (IVET) for Analysing Microbial Gene
Expression in Complex Environments Pp. 207-240
R. W. Jackson and S. R. Giddens
[Abstract]
High-Throughput Identification of Conditionally
Essential Genes in Bacteria: From STM to TSM Pp.
241-262
J. T. Bossé, L. Zhou, J. S. Kroll and P. R. Langford
[Abstract]
DNA Microarrays - An Armory for Combating Infectious
Diseases in the New Century Pp. 263-279
T. Chen
[Abstract]
Serial Analysis of Gene Expression in Eukaryotic
Pathogens Pp. 281-297
James W. Kronstad
[Abstract]
Microarray Analysis of Human Epithelial Cell Responses
to Bacterial Interaction Pp. 299-309
Jeffrey J. Mans, Richard J. Lamont and Martin Handfield
[Abstract]
Mass Spectrometry-Based Proteomics and its Application
to Studies of Porphyromonas gingivalis Invasion and
Pathogenicity Pp. 311-325
Richard J. Lamont, Marina Meila, Qiangwei Xia and Murray
Hackett
[Abstract]
In Vivo Induced Antigen Technology (IVIAT)
and Change Mediated Antigen Technology (CMAT) Pp.
327-334
Martin Handfield and Jeffrey D. Hillman
[Abstract]
Abstracts
[Back to top]
Editorial
Microbiologists have realized that it is unlikely that
all virulence determinants of a human pathogen could be identified
simply by studying the pathogen in the laboratory since it
is technically impossible to determine and mimic all of the
complex and changing environmental stimuli that occur at the
site of an infection. This shortcoming hampers our complete
understanding of the virulence mechanisms employed by human
pathogens, which is reflected in the relatively small number
of effective vaccines that are currently available to combat
the myriad of infections that afflict mankind. To overcome
this problem, a number of investigators have designed methods
to identify genes of pathogens that are specifically expressed
during infection. The advent of in vivo expression
technology (IVET) in 1993 triggered a concerted effort in
various fields of microbiology to seek for differentially-expressed
and/or in vivo induced genes. These genes were originally
proposed as likely targets for the development of new vaccine,
diagnostic and antibiotherapy strategies in the medical field.
In counterpart, other non-human systems quickly followed the
trend and included the development of methods particularly
suited to study plant and animal pathogens in vivo.
This Special Edition of Infectious Disorders-Drug Targets
reviews some of the latest and outstanding developments accomplished
using a number of methods that focus on differentially expressed
genes to further our understanding of molecular microbial
pathogenesis. A plethora of reviews have exhaustively covered
many aspects of the novel techniques that led to the identification
of numerous differentially expressed microbial genes. The
present overview focuses on those methods that show substantial
promise for—or have already led to—novel approaches
for diagnosing, preventing or treating microbial diseases.
In the first two papers, methods based on in vivo
screens and selection will be presented. Jackson and Giddens
(Development and Application of In Vivo Expression
Technology (IVET) for Analysing Microbial Gene Expression
in Complex Environments) will describe IVET and its
various spin-offs as tools for analyzing microbial gene expression
in complex environments and providing new targets for biotechnological
development. Bossé et al. (High-Throughput
Identification of Conditionally Essential
Genes in Bacteria: From STM to TSM) will next depict
the latest development obtained with signature-tagged mutagenesis
(STM) and transposon screen by microarray (TSM), which combine
the negative-selection principle of STM with the genome-wide
screening strength of DNA microarrays.
The next three papers will focus on transcriptomic approaches
that have been used to dissect host-pathogen interactions.
A review on the recent and ongoing developments obtained with
bacterial microarrays will first be presented by Chen (DNA
Microarrays - An Armory for Combating Infectious Diseases
in the New Century). Besides describing exciting
progress in microarray technology applied to the study of
microbial pathogenesis, drug response, vaccine development
and disease agent identification, Chen will address certain
issues and challenges in the analysis, management and interpretation
of microarray data. Kronstad (Serial Analysis of Gene
Expression in Eukaryotic Pathogens) will then present
SAGE as an alternative technique to microarrays to obtain
information on transcript abundance and differential RNA expression,
particularly with eukaryotic systems such as Saccharomyces
cerevisiae and Caenorhabditis elegans. Finally,
Mans et al. (Microarray Analysis of Human
Epithelial Cell Responses to Bacterial Interaction)
will present how the host transcriptional responses have been
recently used to infer the function of virulence determinants
of bacterial pathogens that are interacting with the epithelial
mucosa during disease.
In the last two papers, particular emphasis will be granted
to the use of proteomic approaches leading to understanding
of microbial pathogenesis and development of new vaccine,
diagnostic and antibiotherapy tools. Lamont et al.
(Mass Spectrometry-Based Proteomics and Its Application
to Studies of Porphyromonas gingivalis Invasion and
Pathogenicity) will depict the recent advances in
proteomic methods based on multidimensional capillary HPLC
and tandem mass spectrometry, which allow the acquisition
of comprehensive protein expression datasets. These datasets
are comparable with spotted cDNA arrays in terms of coverage
and quantitative precision. Finally, Handfield and Hillman
(In Vivo Induced Antigen Technology (IVIAT)
and Change Mediated Antigen Technology (CMAT)) will
review recent applications of IVIAT and CMAT to various human
and plant pathogens.
Martin Handfield, MSc, PhD.
Center for Molecular Microbiology and
Department of Oral Biology,
Box 100424 JHMHSC,
University of Florida College of Dentistry,
Gainesville FL 32610-0424,
USA
E-mail: MHANDFIELD@dental.ufl.edu
[Back to top]
Development and Application of In Vivo
Expression Technology (IVET) for Analysing Microbial Gene
Expression in Complex Environments
R. W. Jackson and S. R. Giddens
Establishing the mechanisms by which microbes interact with
their environment, including eukaryotic hosts, is a major
challenge that is essential for the economic utilisation of
microbes and their products. Techniques for determining global
gene expression profiles of microbes, such as microarray analyses,
are often hampered by methodological restraints, particularly
the recovery of bacterial transcripts (RNA) from complex mixtures
and rapid degradation of RNA. A pioneering technology that
avoids this problem is In Vivo Expression Technology
(IVET). IVET is a ‘promoter-trapping’ methodology
that can be used to capture nearly all bacterial promoters
(genes) upregulated during a microbe-environment interaction.
IVET is especially useful because there is virtually no limit
to the type of environment used (examples to date include
soil, oomycete, a host plant or animal) to select for active
microbial promoters. Furthermore, IVET provides a powerful
method to identify genes that are often overlooked during
genomic annotation, and has proven to be a flexible technology
that can provide even more information than identification
of gene expression profiles. A derivative of IVET, termed
resolvase-IVET (RIVET), can be used to provide spatio-temporal
information about environment-specific gene expression. More
recently, niche-specific genes captured during an IVET screen
have been exploited to identify the regulatory mechanisms
controlling their expression. Overall, IVET and its various
spin-offs have proven to be a valuable and robust set of tools
for analysing microbial gene expression in complex environments
and providing new targets for biotechnological development.
[Back to top]
High-Throughput Identification of Conditionally
Essential Genes in Bacteria: From STM to TSM
J. T. Bossé, L. Zhou, J. S. Kroll and P. R. Langford
Signature-tagged mutagenesis (STM) provided the first widely
applicable high-throughput method for detecting conditionally
essential genes in bacteria by using negative selection to
screen large pools of transposon (Tn) mutants. STM requires
no prior knowledge of the bacterium’s genome sequence,
and has been used to study a large number of Gram-positive
and Gram-negative species, greatly expanding the repertoires
of known virulence factors for these organisms. Originally,
hybridization of radiolabelled probes to colony or dot blots
was used to detect differences in populations of tagged mutants
before and after growth under a selective condition. Modifications
of the tag detection method involving polymerase chain reaction
(PCR) amplification and visualisation by gel electrophoresis
have been developed and can be automated through the use of
robotics. Genetic footprinting is another negative selection
technique that uses PCR amplification to detect loss of mutants
from a pool. Unlike PCR-STM, this technique allows direct
amplification of Tn-flanking sequences. However, it requires
the bacterium’s whole genome sequence in order to design
specific primers for every gene of interest. More recently,
a number of techniques have been described that combine the
negative-selection principle of STM and genetic footprinting
with the genome-wide screening power of DNA microarrays. These
techniques, although also requiring whole genome sequences,
use either a form of linker-mediated or semi-random PCR to
amplify and label Tn-flanking regions for hybridization to
microarrays. The superior sensitivity microarray detection
allows greater numbers of mutants to be screened per pool,
as well as determination of the coverage/distribution of insertions
in the library prior to screening, two significant advantages
over STM.
[Back to top]
DNA Microarrays - An Armory for Combating Infectious
Diseases in the New Century
T. Chen
DNA microarrays are high-throughput platforms that take advantage
of the vast amount of sequence information and allow scientists
to perform gene expression profiling or genotyping studies
on a "global" or "genome-wide" scale.
The global monitoring of gene expression in hosts and pathogens,
either separately or interactively, has given us systemic
views of the disease mechanisms. Ongoing improvements in DNA
sequencing and microarray technologies continue to open up
new opportunities for better understanding and developing
more effective approaches in diagnosis, treatments, and preventions
of infectious diseases. This review focuses on the latest
developments and applications of the DNA microarray technologies
designed for studying pathogens in the areas of pathogenesis,
host-pathogen interaction, drug response, vaccine development,
and disease agent identification. Issues and challenges in
the analysis, management and interpretation of microarray
data are also addressed.
[Back to top]
Serial Analysis of Gene Expression in Eukaryotic
Pathogens
James W. Kronstad
The tag-based method of serial analysis of gene expression
(SAGE) has been used to measure mRNA abundance and differential
expression in a variety of organisms including several parasites
and fungal pathogens. SAGE is based on the collection of short
sequence tags as a measure of transcript abundance and the
method provides an alternative, and in some instances, complementary
approach to array-based methods of measuring differential
gene expression. These methods are being used to improve our
molecular understanding of the pathogenesis of eukaryotic
microbes and SAGE in particular presents valuable opportunities
for gene discovery and genome annotation. For eukaryotic pathogens,
the SAGE method has been employed for the parasites Plasmodium
falciparum, Toxoplasma gondii and Giardia lamblia,
as well as fungal pathogens of plants (Magnaporthe grisea,
Blumeria graminis, Ustilago maydis) and humans (Cryptococcus
neoformans, Coccidiodes posadasii, Trichophyton rubrum).
The accumulating information promises to speed the identification
of key pathogen functions for virulence and proliferation
in the host with the hope that some of these will represent
important targets for drug and vaccine development.
[Back to top]
Microarray Analysis of Human Epithelial Cell Responses
to Bacterial Interaction
Jeffrey J. Mans, Richard J. Lamont and Martin Handfield
Host-pathogen interactions are inherently complex and dynamic.
The recent use of human microarrays has been invaluable to
monitor the effects of various bacterial and viral pathogens
upon host cell gene expression programs. This methodology
has allowed the host response transcriptome of several cell
lines to be studied on a global scale. To this point, the
great majority of reports have focused on the response of
immune cells, including macrophages and dendritic cells. These
studies revealed that the immune response to microbial pathogens
is tailored to different microbial challenges. Conversely,
the paradigm for epithelial cells has—until recently—held
that the epithelium mostly served as a relatively passive
physical barrier to infection. It is now generally accepted
that the epithelial barrier contributes more actively to signaling
events in the immune response. In light of this shift, this
review will compare transcriptional profiling data from studies
that involved host-pathogen interactions occurring with epithelial
cells. Experiments that defined both a common core response,
as well as pathogen-specific host responses will be discussed.
This review will also summarize the contributions that transcriptional
profiling analysis has made to our understanding of bacterial
physio-pathogensis of infection. This will include a discussion
of how host transcriptional responses can be used to infer
the function of virulence determinants from bacterial pathogens
interacting with epithelial mucosa. In particular, we will
expand upon the lessons that have been learned from gastro-intestinal
and oral pathogens, as well as from members of the commensal
flora.
[Back to top]
Mass Spectrometry-Based Proteomics and its Application
to Studies of Porphyromonas gingivalis Invasion and
Pathogenicity
Richard J. Lamont, Marina Meila, Qiangwei Xia and Murray
Hackett
Porphyromonas gingivalis is a Gram-negative anaerobe
that populates the subgingival crevice of the mouth. It is
known to undergo a transition from its commensal status in
healthy individuals to a highly invasive intracellular pathogen
in human patients suffering from periodontal disease, where
it is often the dominant species of pathogenic bacteria. The
application of mass spectrometry-based proteomics to the study
of P. gingivalis interactions with model host cell
systems, invasion and pathogenicity is reviewed. These studies
have evolved from qualitative identifications of small numbers
of secreted proteins, using traditional gel-based methods,
to quantitative whole cell proteomic studies using multiple
dimension capillary HPLC coupled with linear ion trap mass
spectrometry. It has become possible to generate a differential
readout of protein expression change over the entire P.
gingivalis proteome, in a manner analogous to whole genome
mRNA arrays. Different strategies have been employed for generating
protein level expression ratios from mass spectrometry data,
including stable isotope metabolic labeling and most recently,
spectral counting methods. A global view of changes in protein
modification status remains elusive due to the limitations
of existing computational tools for database searching and
data mining. Such a view would be desirable for purposes of
making global assessments of changes in gene regulation in
response to host interactions during the course of adhesion,
invasion and internalization. With a complete data matrix
consisting of changes in transcription, protein abundance
and protein modification during the course of invasion, the
search for new protein drug targets would benefit from a more
comprehensive understanding of these processes than what could
be achieved prior to the advent of systems biology.
[Back to top]
In Vivo Induced Antigen Technology (IVIAT)
and Change Mediated Antigen Technology (CMAT)
Martin Handfield and Jeffrey D. Hillman
In this chapter, an overview of in vivo induced antigen
technology (IVIAT) and change mediated antigen technology
(CMAT) will be presented, including a discussion of the advantages
and limitations of these methods. Over fifteen different microbial
pathogens have been or are known to be currently studied with
these methods. Salient data obtained from the application
of IVIAT and/or CMAT to a selection of human and plant pathogens
will be summarized. This includes recent reports on Streptococcus
pyogenes (Group A) in neurological disorders and invasive
diseases, Xylella fastidiosa in Pierce's disease,
Xanthomonas campestris in bean blight, Salmonella
enterica serovar typhi in typhoid fever and
Leishmania spp. related infections. Special emphasis
will be given to those targets that have been further investigated
for the development of novel vaccine, diagnostic and/or antibiotherapy
strategies. This encompasses a new point-of-care serological
diagnostic test for chronic periodontal diseases. Finally,
Mycobacterium tuberculosis in vivo induced products
will be described as providing a rational basis for differentiating
subjects with primary, dormant or secondary tuberculosis infections,
from control subjects who have or did not have prior vaccination
with BCG.
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