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Applied and Environmental Microbiology, October 2001, p. 4454-4457, Vol. 67, No. 10
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.10.4454-4457.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Role of 
B in Heat, Ethanol, Acid,
and Oxidative Stress Resistance and during Carbon Starvation in
Listeria monocytogenes
Adriana
Ferreira,1
Conor P.
O'Byrne,2 and
Kathryn J.
Boor1,*
Department of Food Science, Cornell
University, Ithaca, New York 14853,1 and
Department of Molecular and Cell Biology, Institute of
Medical Sciences, University of Aberdeen, Foresterhill, Aberdeen
AB25 2ZD, Scotland, United Kingdom2
Received 16 April 2001/Accepted 16 July 2001
 |
ABSTRACT |
To determine the contribution of sigma B (
B) to
survival of stationary-phase Listeria monocytogenes
cells following exposure to environmental stresses, we compared the
viability of strain 10403S with that of an isogenic nonpolar
sigB null mutant strain after exposure to heat (50°C),
ethanol (16.5%), or acid (pH 2.5). Strain viabilities were also
determined under the same conditions in cultures that had been
previously exposed to sublethal levels of the same stresses (45°C,
5% ethanol, or pH 4.5). The 
sigB and wild-type
strains had similar viabilities following exposure to ethanol and heat,
but the sigB strain was almost 10,000-fold more
susceptible to lethal acid stress than its parent strain. However, a
1-h preexposure to pH 4.5 yielded a 1,000-fold improvement in viability
for the sigB strain. These results suggest the
existence in L. monocytogenes of both a
B-dependent mechanism and a pH-dependent mechanism for
acid resistance in the stationary phase. B contributed
to resistance to both oxidative stress and carbon starvation in
L. monocytogenes. The sigB strain was
100-fold more sensitive to 13.8 mM cumene hydroperoxide than the
wild-type strain. Following glucose depletion, the
sigB strain lost viability more rapidly than the
parent strain. B contributions to viability during
carbon starvation and to acid resistance and oxidative stress
resistance support the hypothesis that B plays a role in
protecting L. monocytogenes against environmental adversities.
| |
INTRODUCTION |
Listeria monocytogenes is
a gram-positive bacterial pathogen that can cause severe food-borne
disease. This organism is responsible for approximately 2,500 illnesses
and 500 deaths annually in the United States (18).
L. monocytogenes is a common food contaminant, at least in
part due to its ubiquitous existence in the environment. This
organism's ability to persist and thrive under very different conditions suggests that it is capable of efficiently responding to
environmental stress challenges.
In bacteria, the association of appropriate alternative sigma factors
with core RNA polymerase provides a mechanism for cellular responses
that are mediated through redirection of transcription initiation. In
both gram-negative and gram-positive organisms, the alternative sigma
factors, RpoS and sigma B (B), respectively,
regulate expression of numerous genes under environmental stress
conditions and upon entry into the stationary phase. The role of RpoS
in regulation of genes involved in stress protection has been
characterized for various gram-negative bacteria, including Escherichia coli, Salmonella, and
Yersinia spp. RpoS has been shown to influence cellular
resistance to heat, acid, and high osmolarity in the pathogenic
organism E. coli O157:H7 (10) and in
Yersinia enterocolitica (4). RpoS also has been
shown to contribute to Salmonella virulence. For example,
the Salmonella enterica serovar Typhi Ty21 strain used as a
live oral vaccine has been shown to have an rpoS mutation
that has been demonstrated to contribute to the environmental stress
susceptibility of this virulence-attenuated organism (20).
Furthermore, in a mouse model system, an S. enterica serovar
Typhimurium RpoS mutant has been shown to have potential for use as a
live oral vaccine (11).
B regulates expression of a large general
stress operon in Bacillus subtilis, contributing to
transcription of more than 100 genes involved in heat, acid, ethanol,
salt, and oxidative stress resistance (2, 3, 14, 22).
B also has been shown to contribute to heat,
acid, and oxidative stress resistance in Staphylococcus
aureus (9) and in osmotolerance (5) and
acid stress resistance (23) in L. monocytogenes. Becker et al. (5) demonstrated that
there is increased L. monocytogenes sigB transcription,
which implies that there is increased B
activity, following exposure of exponentially growing cells to acid,
ethanol, osmotic, heat, and oxidative stresses, as well as upon entry
into the stationary phase. Furthermore, B has
been demonstrated to contribute to the ability of stationary-phase L. monocytogenes cells to adapt to and resume growth at
reduced temperatures (6). Although sigB and
rpoS do not exhibit significant sequence identity beyond
that required for conserved functions among sigma factors and while the
activities of these transcription factors are regulated in very
different ways, the proteins appear to contribute to physiologically
similar cellular needs. Furthermore, the B. subtilis
B and E. coli RpoS regulons share a
subset of genes, including genes for nonspecific DNA binding proteins
(dps) and catalases (katE) (15).
Taken together, these results suggest the possibility that
B and RpoS have parallel roles in the general
stress responses of gram-positive and gram-negative organisms, respectively.
L. monocytogenes (17) and B. subtilis (22) have been shown to display enhanced
resistance to lethal stresses following preexposure to sublethal levels
of the same stresses. In B. subtilis, this stress adaptation
response appears to be B dependent
(22). Pretreatment with mild heat (48°C) or mild salt
(4%) stress was shown to enhance survival of the B. subtilis wild-type strain but not a sigB strain when
cultures were exposed to a more severe level of the same stress (54°C
or 10% ethanol). Furthermore, B activation in
the absence of specific stresses was also shown to confer enhanced
resistance to subsequent exposure to lethal stress (22).
Specifically, sigB was placed under control of the
isopropyl-
-D-thiogalactopyranoside-inducible
promoter Pspac in a B. subtilis strain carrying a null mutation in rsbW, the primary negative regulator of B activity.
Addition of isopropyl--D-thiogalactopyranoside
prior to heat or salt treatment enhanced cell survival following
exposure to stress, leading to the conclusion that activation of
B expression alone may protect cells from
subsequent stresses.
In this study, we characterized the survival phenotypes of L. monocytogenes sigB null mutant stationary-phase cells under multiple stress conditions, including heat, ethanol, acid, and oxidative stresses. We also examined the role of
B in the L. monocytogenes
stationary-phase stress adaptation response.
| |
MATERIALS AND METHODS |
Bacterial strains.
L. monocytogenes 10403S
(8) and FSL A1-254 (23) were used throughout
this study. L. monocytogenes 10403S, a serotype 1/2a strain,
was obtained from D. Portnoy (University of California, Berkeley).
L. monocytogenes FSL A1-254 was generated by creating a
600-bp sigB fragment with an in-frame 297-bp deletion
between nucleotides 1490 and 1788 of the sigB operon in
10403S (GenBank accession no. AF032446 [20]). Stock
cultures were stored at 
80°C in brain heart infusion (BHI) broth
(Difco, Sparks, Md.) with 15% glycerol and streaked onto BHI agar
plates prior to inoculation of the working cultures.
Resistance to ethanol, heat, and acid following
preadaptation.
Strains were tested as described by Lou and Yousef
(17), with the following modifications. Briefly, 5 ml of
BHI broth was inoculated from an isolated colony of L. monocytogenes 10403S or FSL A1-254, and the culture was grown to
the stationary phase (12 h) at 37°C with rotary shaking (250 rpm) in
a series 25 incubator-shaker (New Brunswick Scientific, Edison, N. J.). Such cultures were used to inoculate fresh tubes containing 5 ml
of BHI broth (1:100), which were then incubated with shaking at 37°C
for another 12 h. The resulting stationary-phase cultures were
centrifuged at 4,000 × g for 5 min. The pellets were
resuspended in 5 ml of either BHI broth containing 5% ethanol or BHI
broth acidified to pH 4.5 and then incubated for 1 h at 37°C.
For heat preadaptation, cells harvested in the stationary phase were
resuspended in 5 ml of BHI broth as described above and incubated at
45°C for 1 h. Following 1-h adaptation periods in 5% ethanol
and at pH 4.5, cells were harvested, and the pellets exposed to
sublethal conditions were resuspended in BHI broth with 16.5% ethanol
and in BHI broth (pH 2.5), respectively, and then incubated at 37°C
for 3 h. In both cases, the broth media had been prewarmed to
37°C. The pellets from cultures preadapted at 45°C were resuspended
in BHI broth (prewarmed to 50°C) and incubated at 50°C for up to
8 h. Nonadapted stationary-phase cell pellets were resuspended
directly under the following lethal conditions: BHI broth with 16%
ethanol, BHI broth (pH 2.5), and BHI broth at 50°C. These control
cultures were incubated in parallel with the preadapted samples.
Aliquots were removed for viable cell determination at suitable
intervals. Serial dilutions in phosphate-buffered saline were plated in
duplicate onto BHI agar plates and then incubated at 37°C for 48 h. Colonies were enumerated, and the results are presented below as
percentages of cell survival. Experiments were performed in duplicate
and repeated independently at least two times.
Resistance to carbon starvation.
Cultures of L. monocytogenes 10403S and FSL A1-254 were grown from isolated
colonies in a defined medium (1) supplemented with a
limiting level of glucose (0.04%, wt/vol). Culture density was
monitored by determining optical density at 600 nm
(OD600), and cell viability was measured by
standard plate counting using samples taken at various times for up to
12 h after cultures had stopped growing due to carbon limitation
(OD600, ~0.2).
Resistance to oxidative stress.
Oxidative resistance
responses of the mutant and wild-type cultures were assessed by using
the oxidative agent cumene hydroperoxide (CHP) (Sigma, St. Louis, Mo.).
CHP survival assays were conducted as described by Antelmann et al.
(2), with the following modifications. Briefly, cell
cultures that had been grown to the stationary phase at 37°C with
shaking (250 rpm) for 12 h were inoculated into 5 ml of BHI broth
(1:100). Following 12 h of incubation at 37°C, 900-µl portions
of the cultures were transferred to tubes containing 100 µl of 138 mM
CHP diluted in dimethyl sulfoxide (Fisher Scientific, Fair Lawn,
N.J.), which yielded a final CHP concentration of 13.8 mM. Control
cultures were transferred to tubes containing 100 µl of dimethyl
sulfoxide. All tubes, including the controls, were then incubated for
15 min at 37°C with shaking. Cell viability was assessed by standard
plate counting on BHI agar plates that had been incubated at 37°C.
The results described below reflect the data from two independent
experiments, each performed in triplicate.
| |
RESULTS AND DISCUSSION |
Role of B in resistance to heat, ethanol, and acid
stress.
The survival of the L. monocytogenes 10403S
wild-type strain was compared with that of an isogenic nonpolar
sigB null mutant strain following exposure to lethal levels
of heat (50°C), ethanol (16.5%), and acid (pH 2.5). To investigate
the role of B in L. monocytogenes
stress adaptation, we also compared strain survival under these lethal
environmental stress conditions following a 1-h preexposure to
sublethal levels of the same stresses (45°C, 5% ethanol, and pH
4.5). B-dependent survival phenotypes were
assessed in stationary-phase cells as (i) B
activity increases upon entry into the stationary phase
(5) and (ii) B previously has
been shown to contribute to L. monocytogenes acid stress
survival under these conditions (23).
Heat stress resistance and ethanol stress resistance were found to be
at least partially B independent in L. monocytogenes under the conditions used in this study. Similar
culture viabilities were observed for both the L. monocytogenes sigB and wild-type strains when they
were exposed to either 50°C (Fig. 1A)
or 16.5% ethanol (Fig. 1B). Preadaptation to reduced heat stress
(45°C) did not enhance survival of either strain following exposure
to a more lethal level of heat stress (50°C) (Fig. 1A). However,
preadaptation to a sublethal level of ethanol (5%) enhanced cell
survival by 10- to 100-fold in the presence of a more lethal level of
ethanol (16.5%) for both the sigB and wild-type strains.
The ethanol adaptation response mechanism in L. monocytogenes appears to be B independent
as the sigB and wild-type strains exhibited similar recoveries from exposure to 16% ethanol following preadaptation in 5%
ethanol (Fig. 1B). Although heat and ethanol have been shown to induce
sigB transcription in exponentially growing L. monocytogenes cells (5), our results suggest that
stationary-phase resistance to heat and ethanol stresses is at least
partially B independent in this organism.
These results parallel those obtained with S. aureus, in
which cellular exposure to ethanol or NaCl enhanced production of a
sigB transcript but did not differentially affect survival
of the B mutant and its wild-type counterpart
(9). Similarly, in preliminary experiments, the levels of
survival of the L. monocytogenes 10403S wild-type strain and
the sigB mutant were identical after 24 h of
exposure to up to 25% NaCl in BHI broth (incubated at 37°C with
shaking) (data not shown) despite the previous observation that there
was increased sigB transcription in the presence of 4% NaCl
(5). We speculate that the environmental stress conditions used in our study, as well as those used by Chan et al.
(9), may have been sufficiently lethal to have overwhelmed
possible B contributions to cellular survival.
Alternatively, it is possible that although B
activity is induced during exposure to ethanol or salt
(5), the resulting general stress response does not
provide appropriate cellular defenses against these specific stresses.
This hypothesis is supported, at least in part, by the observation that
preexposure to 5% ethanol enhances L. monocytogenes
survival in the presence of 16.5% ethanol in a
B-independent manner. The specific
mechanism(s) responsible for this adaptive response is currently
unknown.
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FIG. 1.
Percent viabilities of L. monocytogenes
sigB (circles) and wild-type (WT) (squares)
stationary-phase cultures during exposure to lethal stresses, including
heat (50°C) (A), ethanol (16.5%) (B), and acid (pH 2.5) (C), with
(AD) (solid symbols) and without (NA) (open symbols) preadaptation for
1 h at 45°C, in the presence of 5% ethanol, and at pH 4.5, respectively. The results are averages based on at least two
repetitions, each performed in duplicate. The error bars indicate
standard deviations.
|
|
As shown in Fig.
1C, acid resistance in
L. monocytogenes
stationary-phase cells exposed to pH 2.5 appears to be at least
partially
B dependent. The percent survival of
the
L. monocytogenes sigB strain was almost
10,000-fold lower than that of its parent strain
after 3 h of
exposure to pH 2.5. However, a 1-h preexposure to
a sublethal level of
acid stress (pH 4.5) improved
sigB strain
viability by
more than 1,000-fold following exposure to pH 2.5,
suggesting that
L. monocytogenes stationary-phase acid tolerance
can be
induced by exposure to reduced pH in a
B-independent
manner.
Previous work has shown that
L. monocytogenes possesses a
pH-dependent log-phase acid tolerance response (ATR), as well as
a
stationary-phase-dependent ATR (
12). Our data suggest that
stationary-phase acid tolerance depends on at least two mechanisms,
a
B-dependent mechanism and a pH-dependent
mechanism that is at least
partially
B
independent, as cell viability at pH 2.5 following preadaptation
was
not fully recovered in the
sigB strain. These results are
similar to the partially
B-dependent acid
adaptive response observed in
S. aureus cells
that had been
preexposed to pH 4 prior to pH 2 treatment (
9).
By
comparison, three mechanisms contributing to acid tolerance
have been
reported in
S. enterica serovar Typhimurium
(
16).
This pathogenic gram-negative bacterium displays two
distinct
pH-dependent ATRs, a log-phase ATR and a stationary-phase ATR,
as well as pH-independent stationary-phase acid tolerance, which
is
RpoS
dependent.
Role of B in survival during carbon starvation.
The relative viabilities of the L. monocytogenes
sigB and 10403S wild-type strains grown in a defined
medium with limiting glucose (0.04%, wt/vol) were compared to assess
the role of B in survival during carbon
starvation. Plate counts were used to determine culture viabilities for
up to 12 h following growth arrest at an
OD600 of ~0.2 due to glucose depletion. The
sigB strain lost viability more rapidly than the parent
strain under carbon starvation conditions (Fig.
2). After 12 h in a glucose-depleted medium, sigB strain viability was reduced by 85%,
compared with a 25% reduction for the wild-type culture. The viability
loss may have been due to enhanced cell lysis, as suggested by the ~10-fold reduction in OD600 for the
sigB strain. These data suggest an important role for
B in L. monocytogenes survival
during carbon starvation. Expression of more than eight proteins has
been shown to be induced by B in
glucose-starved B. subtilis cells (7).
Furthermore, glucose-starved B. subtilis (2)
and S. aureus (9) sigB strains
have been shown to be less resistant to oxidative stress than their
wild-type parents.
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FIG. 2.
Viabilities of L. monocytogenes
sigB (solid symbols) and wild-type (WT) (open
symbols) cultures that had been grown in a defined medium with limiting
glucose (0.04%, wt/vol). The x axis indicates the time
following growth cessation in the defined medium. OD600
(circles) and viable numbers (squares) were recorded for up to 12 h after the cultures had stopped growing due to carbon limitation. The
error bars indicate standard deviations.
|
|
Role of B in resistance to oxidative stress.
The role of B in protecting L. monocytogenes against oxidative stress was assessed by comparing
the viability of the sigB strain with that of the 10403S
parent following exposure to 13.8 mM CHP for 15 min. The viability of
the sigB strain was 100-fold lower than that of its
wild-type parent (Fig. 3), suggesting
that oxidative stress resistance is at least partially
B dependent in stationary-phase L. monocytogenes cells. In combination with the observed increase in
L. monocytogenes sigB transcription following exposure to
0.15% H2O2
(5), these results provide further evidence that
B contributes to cellular survival under
oxidizing conditions.
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FIG. 3.
Viabilities of L. monocytogenes
sigB and wild-type stationary-phase cultures that
were not exposed to CHP (open bars) or were exposed to 13.8 mM CHP for
15 min (shaded bars). The error bars indicate standard deviations.
|
|
Antelmann et al. (
2) also observed that a
B. subtilis sigB strain was more sensitive to CHP than
wild-type cells were;
however, the cells had been grown under glucose
depletion conditions.
Conversely,
B-dependent
oxidative stress resistance induced by starvation has
been observed in
B. subtilis (
13) and in
S. aureus
(
9) strains
exposed to hydrogen peroxide.
B has been shown to control expression of
several genes involved
in oxidative stress resistance in
B. subtilis, including
katE,
which encodes a catalase
protein (
2,
14), and
dps, which
encodes a
DNA-protecting protein (
3). In the gram-negative
organism
S. enterica serovar Typhimurium (
21) and in
E. coli (
19), oxidative stress resistance has
been shown to depend at
least partially on
RpoS.
In conclusion, this study showed that
B
contributes to survival of stationary-phase
L. monocytogenes
cells under acid and
oxidative stress conditions.
B also contributes to survival of
growth-arrested
L. monocytogenes cells during carbon
starvation. Furthermore, our data reveal the
existence of at least two
mechanisms of acid resistance in
L. monocytogenes
stationary-phase cells: a pH-independent
B-dependent mechanism and a pH-dependent
mechanism that is at least
partially
B
independent. We hypothesize that in
L. monocytogenes acid
and
oxidative stress protection conferred by
B
may contribute to the virulence of this invasive pathogen, as
this
organism must survive acid and oxidative stresses imposed
by the host
to cause
illness.
| |
ACKNOWLEDGMENT |
A. Ferreira was supported by a fellowship from CAPES
(Fundação Coordenação de Aperfeiçoamento
de Pessoal de Nível Superior-Brasil).
| |
FOOTNOTES |
*
Corresponding author. Mailing address: 413 Stocking
Hall, Department of Food Science, Cornell University, Ithaca, NY 14853. Phone: (607) 255-3111. Fax: (607) 254-4868. E-mail:
kjb4{at}cornell.edu.
| |
REFERENCES |
| 1.
|
Amezaga, M. R.,
I. Davidson,
D. McLaggan,
A. Verheul,
T. Abee, and I. R. Booth.
1995.
The role of peptide metabolism in the growth of Listeria monocytogenes ATCC 23074 at high osmolarity.
Microbiology
141:41-49[Abstract/Free Full Text].
|
| 2.
|
Antelmann, H.,
S. Engelmann,
R. Schmid, and M. Hecker.
1996.
General and oxidative stress responses in Bacillus subtilis: cloning, expression, and mutation of the alkyl hydroperoxide reductase operon.
J. Bacteriol.
178:6571-6578[Abstract/Free Full Text].
|
| 3.
|
Antelmann, H.,
S. Engelmann,
R. Schmid,
A. Sorokin,
A. Lapidus, and M. Hecker.
1997.
Expression of a stress- and starvation-induced dps/pexB-homologous gene is controlled by the alternative sigma factor B in Bacillus subtilis.
J. Bacteriol.
179:7251-7256[Abstract/Free Full Text].
|
| 4.
|
Badger, J. L., and V. L. Miller.
1995.
Role of RpoS in survival of Yersinia enterocolitica to a variety of environmental stresses.
J. Bacteriol.
177:5370-5373[Abstract/Free Full Text].
|
| 5.
|
Becker, L. A.,
M. S. Cetin,
R. W. Hutkins, and A. K. Benson.
1998.
Identification of the gene encoding the alternative sigma factor B from Listeria monocytogenes and its role in osmotolerance.
J. Bacteriol.
180:4547-4554[Abstract/Free Full Text].
|
| 6.
|
Becker, L. A.,
S. N. Evans,
R. W. Hutkins, and A. K. Benson.
2000.
Role of B in adaptation of Listeria monocytogenes to growth at low temperatures.
J. Bacteriol.
182:7083-7087[Abstract/Free Full Text].
|
| 7.
|
Bernhardt, J.,
U. Völker,
A. Völker,
H. Antelmann,
R. Schmid,
H. Mach, and M. Hecker.
1997.
Specific and general stress proteins in Bacillus subtilis a two-dimensional protein electrophoresis study.
Microbiology
143:999-1017[Abstract/Free Full Text].
|
| 8.
|
Bishop, D. K., and D. J. Hinrichs.
1987.
Adoptive transfer of immunity to Listeria monocytogenes. The influence of in vitro stimulation on lymphocyte subset requirements.
J. Immunol.
139:2005-2009[Abstract].
|
| 9.
|
Chan, P. F.,
S. J. Foster,
E. Ingham, and M. O. Clements.
1998.
The Staphylococcus aureus alternative sigma factor B controls the environmental stress response but not starvation survival or pathogenicity in a mouse abscess model.
J. Bacteriol.
180:6082-6089[Abstract/Free Full Text].
|
| 10.
|
Cheville, A. M.,
K. W. Arnold,
C. Buchrieser,
C. M. Cheng, and C. W. Kaspar.
1996.
rpoS regulation of acid, heat, and salt tolerance in Escherichia coli O157:H7.
Appl. Environ. Microbiol.
62:1822-1824[Abstract].
|
| 11.
|
Coynault, C.,
V. Robbe-Saule, and F. Norel.
1996.
Virulence and vaccine potential of Salmonella typhimurium mutants deficient in the expression of the RpoS (S) regulon.
Mol. Microbiol.
22:149-160[Medline].
|
| 12.
|
Davis, M. J.,
P. J. Coote, and C. P. O'Byrne.
1996.
Acid tolerance in Listeria monocytogenes: the adaptive acid tolerance response (ATR) and growth-phase-dependent acid resistance.
Microbiology
142:2975-2982[Abstract/Free Full Text].
|
| 13.
|
Engelmann, S., and M. Hecker.
1996.
Impaired oxidative stress resistance of Bacillus subtilis sigB mutants and the role of katA and katE.
FEMS Microbiol. Lett.
145:63-69[CrossRef][Medline].
|
| 14.
|
Engelmann, S.,
C. Lindner, and M. Hecker.
1995.
Cloning, nucleotide sequence, and regulation of katE encoding a sigma B-dependent catalase in Bacillus subtilis.
J. Bacteriol.
177:5598-5605[Abstract/Free Full Text].
|
| 15.
|
Hecker, M., and U. Völker.
1998.
Non-specific, general and multiple stress resistance of growth-restricted Bacillus subtilis cells by the expression of the B regulon.
Mol. Microbiol.
29:1129-1136[CrossRef][Medline].
|
| 16.
|
Lee, I. S.,
J. L. Slonczewski, and J. W. Foster.
1994.
A low-pH-inducible, stationary-phase acid tolerance response in Salmonella typhimurium.
J. Bacteriol.
176:1422-1426[Abstract/Free Full Text].
|
| 17.
|
Lou, Y., and A. E. Yousef.
1997.
Adaptation to sublethal environmental stresses protects Listeria monocytogenes against lethal preservation factors.
Appl. Environ. Microbiol.
63:1252-1255[Abstract].
|
| 18.
|
Mead, P. S.,
L. Slutsker,
V. Dietz,
L. F. McCaig,
J. S. Bresee,
C. Shapiro,
P. M. Griffin, and R. V. Tauxe.
1999.
Food-related illness and death in the United States.
Emerg. Infect. Dis.
5:607-625[Medline].
|
| 19.
|
Michan, C.,
M. Manchado,
G. Dorado, and C. Pueyo.
1999.
In vivo transcription of the Escherichia coli oxyR regulon as a function of growth phase and in response to oxidative stress.
J. Bacteriol.
181:2759-2764[Abstract/Free Full Text].
|
| 20.
|
Robbe-Saule, V.,
C. Coynault, and F. Norel.
1995.
The live oral typhoid vaccine Ty21a is a rpoS mutant and is susceptible to various environmental stresses.
FEMS Microbiol. Lett.
126:171-176[CrossRef][Medline].
|
| 21.
|
Seymour, R. L.,
P. V. Mishra,
M. A. Khan, and M. P. Spector.
1996.
Essential roles of core starvation-stress response loci in carbon-starvation-inducible cross-resistance and hydrogen peroxide-inducible adaptive resistance to oxidative challenge in Salmonella typhimurium.
Mol. Microbiol.
20:497-505[CrossRef][Medline].
|
| 22.
|
Völker, U.,
B. Maul, and M. Hecker.
1999.
Expression of the B-dependent general stress regulon confers multiple stress resistance in Bacillus subtilis.
J. Bacteriol.
181:3942-3948[Abstract/Free Full Text].
|
| 23.
|
Wiedmann, M.,
T. J. Arvik,
R. J. Hurley, and K. J. Boor.
1998.
General stress transcription factor B and its role in acid tolerance and virulence of Listeria monocytogenes.
J. Bacteriol.
180:3650-3656[Abstract/Free Full Text].
|
Applied and Environmental Microbiology, October 2001, p. 4454-4457, Vol. 67, No. 10
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.10.4454-4457.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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[Abstract]
[Full Text]
-
Abram, F., Starr, E., Karatzas, K. A. G., Matlawska-Wasowska, K., Boyd, A., Wiedmann, M., Boor, K. J., Connally, D., O'Byrne, C. P.
(2008). Identification of Components of the Sigma B Regulon in Listeria monocytogenes That Contribute to Acid and Salt Tolerance. Appl. Environ. Microbiol.
74: 6848-6858
[Abstract]
[Full Text]
-
Nielsen, J. S., Olsen, A. S., Bonde, M., Valentin-Hansen, P., Kallipolitis, B. H.
(2008). Identification of a {sigma}B-Dependent Small Noncoding RNA in Listeria monocytogenes. J. Bacteriol.
190: 6264-6270
[Abstract]
[Full Text]
-
Dunning, D. W., McCall, L. W., Powell, W. F., Arscott, W. T., McConocha, E. M., McClurg, C. J., Goodman, S. D., Spatafora, G. A.
(2008). SloR modulation of the Streptococcus mutans acid tolerance response involves the GcrR response regulator as an essential intermediary. Microbiology
154: 1132-1143
[Abstract]
[Full Text]
-
Abram, F., Su, W.-L., Wiedmann, M., Boor, K. J., Coote, P., Botting, C., Karatzas, K. A. G., O'Byrne, C. P.
(2008). Proteomic Analyses of a Listeria monocytogenes Mutant Lacking {sigma}B Identify New Components of the {sigma}B Regulon and Highlight a Role for {sigma}B in the Utilization of Glycerol. Appl. Environ. Microbiol.
74: 594-604
[Abstract]
[Full Text]
-
Raengpradub, S., Wiedmann, M., Boor, K. J.
(2008). Comparative Analysis of the {sigma}B-Dependent Stress Responses in Listeria monocytogenes and Listeria innocua Strains Exposed to Selected Stress Conditions. Appl. Environ. Microbiol.
74: 158-171
[Abstract]
[Full Text]
-
Hu, Y., Raengpradub, S., Schwab, U., Loss, C., Orsi, R. H., Wiedmann, M., Boor, K. J.
(2007). Phenotypic and Transcriptomic Analyses Demonstrate Interactions between the Transcriptional Regulators CtsR and Sigma B in Listeria monocytogenes. Appl. Environ. Microbiol.
73: 7967-7980
[Abstract]
[Full Text]
-
Hu, Y., Oliver, H. F., Raengpradub, S., Palmer, M. E., Orsi, R. H., Wiedmann, M., Boor, K. J.
(2007). Transcriptomic and Phenotypic Analyses Suggest a Network between the Transcriptional Regulators HrcA and {sigma}B in Listeria monocytogenes. Appl. Environ. Microbiol.
73: 7981-7991
[Abstract]
[Full Text]
-
Chan, Y. C., Boor, K. J., Wiedmann, M.
(2007). {sigma}B-Dependent and {sigma}B-Independent Mechanisms Contribute to Transcription of Listeria monocytogenes Cold Stress Genes during Cold Shock and Cold Growth. Appl. Environ. Microbiol.
73: 6019-6029
[Abstract]
[Full Text]
-
McGann, P., Wiedmann, M., Boor, K. J.
(2007). The Alternative Sigma Factor {sigma}B and the Virulence Gene Regulator PrfA Both Regulate Transcription of Listeria monocytogenes Internalins. Appl. Environ. Microbiol.
73: 2919-2930
[Abstract]
[Full Text]
-
Chaturongakul, S., Boor, K. J.
(2006). {sigma}B Activation under Environmental and Energy Stress Conditions in Listeria monocytogenes. Appl. Environ. Microbiol.
72: 5197-5203
[Abstract]
[Full Text]
-
Garner, M. R., James, K. E., Callahan, M. C., Wiedmann, M., Boor, K. J.
(2006). Exposure to Salt and Organic Acids Increases the Ability of Listeria monocytogenes To Invade Caco-2 Cells but Decreases Its Ability To Survive Gastric Stress. Appl. Environ. Microbiol.
72: 5384-5395
[Abstract]
[Full Text]
-
Shen, Y., Liu, Y., Zhang, Y., Cripe, J., Conway, W., Meng, J., Hall, G., Bhagwat, A. A.
(2006). Isolation and Characterization of Listeria monocytogenes Isolates from Ready-To-Eat Foods in Florida.. Appl. Environ. Microbiol.
72: 5073-5076
[Abstract]
[Full Text]
-
Kazmierczak, M. J., Wiedmann, M., Boor, K. J.
(2006). Contributions of Listeria monocytogenes {sigma}B and PrfA to expression of virulence and stress response genes during extra- and intracellular growth. Microbiology
152: 1827-1838
[Abstract]
[Full Text]
-
Gray, M. J., Freitag, N. E., Boor, K. J.
(2006). How the Bacterial Pathogen Listeria monocytogenes Mediates the Switch from Environmental Dr. Jekyll to Pathogenic Mr. Hyde.. Infect. Immun.
74: 2505-2512
[Full Text]
-
Begley, M., Hill, C., Ross, R. P.
(2006). Tolerance of Listeria monocytogenes to Cell Envelope-Acting Antimicrobial Agents Is Dependent on SigB.. Appl. Environ. Microbiol.
72: 2231-2234
[Abstract]
[Full Text]
-
Garner, M. R., Njaa, B. L., Wiedmann, M., Boor, K. J.
(2006). Sigma B Contributes to Listeria monocytogenes Gastrointestinal Infection but Not to Systemic Spread in the Guinea Pig Infection Model. Infect. Immun.
74: 876-886
[Abstract]
[Full Text]
-
Kazmierczak, M. J., Wiedmann, M., Boor, K. J.
(2005). Alternative Sigma Factors and Their Roles in Bacterial Virulence. Microbiol. Mol. Biol. Rev.
69: 527-543
[Abstract]
[Full Text]
-
van Schaik, W., Zwietering, M. H., de Vos, W. M., Abee, T.
(2005). Deletion of the sigB Gene in Bacillus cereus ATCC 14579 Leads to Hydrogen Peroxide Hyperresistance. Appl. Environ. Microbiol.
71: 6427-6430
[Abstract]
[Full Text]
-
Kim, H., Boor, K. J., Marquis, H.
(2004). Listeria monocytogenes {sigma}B Contributes to Invasion of Human Intestinal Epithelial Cells. Infect. Immun.
72: 7374-7378
[Abstract]
[Full Text]
-
Sue, D., Fink, D., Wiedmann, M., Boor, K. J.
(2004). {sigma}B-dependent gene induction and expression in Listeria monocytogenes during osmotic and acid stress conditions simulating the intestinal environment. Microbiology
150: 3843-3855
[Abstract]
[Full Text]
-
Chaturongakul, S., Boor, K. J.
(2004). RsbT and RsbV Contribute to {sigma}B-Dependent Survival under Environmental, Energy, and Intracellular Stress Conditions in Listeria monocytogenes. Appl. Environ. Microbiol.
70: 5349-5356
[Abstract]
[Full Text]
-
van Schaik, W., Zwietering, M. H., de Vos, W. M., Abee, T.
(2004). Identification of {sigma}B-Dependent Genes in Bacillus cereus by Proteome and In Vitro Transcription Analysis. J. Bacteriol.
186: 4100-4109
[Abstract]
[Full Text]
-
Wemekamp-Kamphuis, H. H., Wouters, J. A., de Leeuw, P. P. L. A., Hain, T., Chakraborty, T., Abee, T.
(2004). Identification of Sigma Factor {sigma}B-Controlled Genes and Their Impact on Acid Stress, High Hydrostatic Pressure, and Freeze Survival in Listeria monocytogenes EGD-e. Appl. Environ. Microbiol.
70: 3457-3466
[Abstract]
[Full Text]
-
van Schaik, W., Tempelaars, M. H., Wouters, J. A., de Vos, W. M., Abee, T.
(2004). The Alternative Sigma Factor {sigma}B of Bacillus cereus: Response to Stress and Role in Heat Adaptation. J. Bacteriol.
186: 316-325
[Abstract]
[Full Text]
-
Sue, D., Boor, K. J., Wiedmann, M.
(2003). {sigma}B-dependent expression patterns of compatible solute transporter genes opuCA and lmo1421 and the conjugated bile salt hydrolase gene bsh in Listeria monocytogenes. Microbiology
149: 3247-3256
[Abstract]
[Full Text]
-
Kazmierczak, M. J., Mithoe, S. C., Boor, K. J., Wiedmann, M.
(2003). Listeria monocytogenes {sigma}B Regulates Stress Response and Virulence Functions. J. Bacteriol.
185: 5722-5734
[Abstract]
[Full Text]
-
Cotter, P. D., Hill, C.
(2003). Surviving the Acid Test: Responses of Gram-Positive Bacteria to Low pH. Microbiol. Mol. Biol. Rev.
67: 429-453
[Abstract]
[Full Text]
-
Ferreira, A., Sue, D., O'Byrne, C. P., Boor, K. J.
(2003). Role of Listeria monocytogenes{sigma}B in Survival of Lethal Acidic Conditions and in the Acquired Acid Tolerance Response. Appl. Environ. Microbiol.
69: 2692-2698
[Abstract]
[Full Text]
-
Fraser, K. R., Sue, D., Wiedmann, M., Boor, K., O'Byrne, C. P.
(2003). Role of {sigma}B in Regulating the Compatible Solute Uptake Systems of Listeria monocytogenes: Osmotic Induction of opuC Is {sigma}B Dependent. Appl. Environ. Microbiol.
69: 2015-2022
[Abstract]
[Full Text]
-
Begley, M., Gahan, C. G. M., Hill, C.
(2002). Bile Stress Response in Listeria monocytogenes LO28: Adaptation, Cross-Protection, and Identification of Genetic Loci Involved in Bile Resistance. Appl. Environ. Microbiol.
68: 6005-6012
[Abstract]
[Full Text]
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Abstract
Introduction
