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Infection and Immunity, April 2001, p. 2569-2579, Vol. 69, No. 4
Department of Microbiology and Immunology,
University of Kentucky Chandler Medical Center, Lexington, Kentucky
40536-0084,1 and Department of
Microbiology and Parasitology, University of Rijeka, Rijeka,
Croatia2
Received 29 August 2000/Returned for modification 15 December
2000/Accepted 10 January 2001
Legionella pneumophila replicates within alveolar
macrophages, and possibly, alveolar epithelial cells and also within
protozoa in the aquatic environment. Here we characterize an L. pneumophila mutant defective in the HtrA/DegP stress-induced
protease/chaperone homologue and show that HtrA is indispensable for
intracellular replication within mammalian macrophages and alveolar
epithelial cells and for intrapulmonary replication in A/J mice.
Importantly, amino acid substitutions of two conserved residues in the
catalytic domain of (H103 Legionella pneumophila is
a gram-negative, facultative intracellular bacterium that is the
causative agent of Legionnaires' disease, a potentially lethal
pneumonia. Ubiquitous in the aquatic environment as a parasite
of protozoa, the bacteria are transmitted to humans upon
inhalation of contaminated aerosols generated by mechanical devices,
such as whirlpools, cooling towers, and showerheads (7).
Within the lungs, L. pneumophila replicates
intracellularly within macrophages and possibly alveolar epithelial
cells (16, 27). Intracellular replication occurs within a
phagosome that is blocked from maturation along the "default"
endosomal-lysosomal degradation pathway and is surrounded by a
ribosome-studded multilayer membrane (1, 34). The ability
of L. pneumophila to modulate the biogenesis of its
phagosome into this idiosyncratic niche is controlled by the Dot/Icm
type IV-like secretion system (40, 48).
Interestingly, the life cycle of L. pneumophila
within protozoa is highly similar to that within mammalian cells at the morphological and molecular levels (3, 7, 13, 26, 32, 41).
In both host cell types, intracellular replication results in lysis of
the host cell. Killing of macrophages and alveolar epithelial cells
occurs in two phases (21); first, through
caspase-3-mediated induction of apoptosis during early stages of the
infection (20, 22-24, 28), followed by pore
formation-mediated egress of the host cell upon termination of
replication (11). In contrast, killing of amoebae does not
involve apoptosis, but pore-forming toxin-mediated cytolysis is
essential for killing and exiting the protozoan cell (23,
32).
During the course of the infection, intracellular pathogens respond to
changes in their microenvironment by a dramatic phenotypic modulation
(2, 8, 9, 31). This response is most likely dictated by
the nature of the phagosomal microenvironment, which seems to be
distinct between intracellular pathogens (8, 31). Although
the mechanisms by which intracellular bacterial pathogens modulate the
biogenesis of their vacuoles into idiosyncratic replicative niches are
now better understood, the biochemical nature of the replicative niches
inhabited by intracellular pathogens is not known.
Because the ability to replicate intracellularly within host cells is
central to its pathogenesis, L. pneumophila must be able to efficiently adapt to its intracellular microenvironment. In
response to its unique intracellular niche within mammalian macrophages, L. pneumophila undergoes a profound
phenotypic modulation, increasing expression of at least 30 proteins.
At least 13 of these proteins, including GroEL/Hsp60, GroES, and GspA,
are also induced by various in vitro stress stimuli (1, 5,
6). This indicates that, although blocked from acidification and
endosomal maturation, L. pneumophila encounters a
hostile microenvironment within the phagosome (8, 31). The
role of the stress response by L. pneumophila in its
adaptation to the intracellular microenvironment within macrophages is
not known. Whether L. pneumophila manifests a stress
response within protozoa and the role of this response in intracellular
replication are also not known.
In this study we show that the htrA/degP homologue of
L. pneumophila is indispensable for intracellular
replication within mammalian cells in vitro and in vivo, yet is
dispensable for the intracellular infection of protozoa. Our data
provide evidence that, despite the similarity in the intracellular
infection of mammalian and protozoan cells by L. pneumophila, significant differences exist in the phagosomal
microenvironment of the two evolutionarily distant hosts.
Bacterial strains, cultures, and vectors.
The virulent
strain of L. pneumophila (AA100/130b) is a clinical
isolate and has been described previously (4). The GL10 and GT20 mutants have been described previously (25, 26). L. pneumophila strains were grown on buffered charcoal
yeast extract (BCYE) agar plates or in buffered yeast extract (BYE)
broth, supplemented with kanamycin for the mutants. The plasmid
PBC-SK+ was used to subclone L. pneumophila
DNA (Stratagene, La Jolla, Calif.). Escherichia coli strain
DH5 DNA and RNA manipulations.
All DNA manipulations were
performed as previously described (44). RNA extraction for
Northern analysis was performed using TriReagent (Gibco-BRL) exactly as
prescribed by the manufacturer. Transfer of RNA to nitrocellulose was
performed according to standard protocols (39).
PCR-generated DNA probes for Northern hybridizations were radiolabeled
with [32P]-dCTP, and hybridization and detection were
performed as described elsewhere (39).
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.4.2569-2579.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
HtrA Homologue of Legionella
pneumophila: an Indispensable Element for Intracellular Infection
of Mammalian but Not Protozoan Cells
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
R and S212A) and
in-frame deletions of either or both of the two conserved PDZ domains
of HtrA abolish its function. Interestingly, the htrA mutant exhibits a parental-type phenotype in intracellular replication within the protozoan host Acanthamoeba polyphaga. We used a
promoterless lacZ fusion to the htrA
promoter to probe the phagosomal microenvironment harboring
L. pneumophila within macrophages and within A. polyphaga for the exposure to stress stimuli. The data show that
expression through the htrA promoter is induced by 12,000- to 20,000-fold throughout the intracellular infection of macrophages
but its induction is by 120- to 500-fold within protozoa compared to in vitro expression. Data derived from confocal laser scanning microscopy reveal that in contrast to the parental strain, phagosomes harboring the htrA mutant within U937 macrophages colocalize with the
late endosomal-lysosomal marker LAMP-2, similar to killed L. pneumophila. Coinfection experiments examined by confocal laser
scanning microscopy show that in communal phagosomes harboring both the
parental strain and the htrA mutant, replication of the
mutant is not rescued, while replication of a dotA
mutant control, which is normally trafficked into a phagolysosome, is
rescued by the parental strain. Our data show, for the first time, that
the stress response by L. pneumophila (mediated, at least
in part, by HtrA) is indispensable for intracellular replication within
mammalian but not protozoan cells.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
(BRL, Gaithersburg, Md.) was used for the majority of cloning
experiments. The L. pneumophila chromosomal cosmid
library has been previously described (44, 45). The
plasmid pUC-4K was purchased from Pharmacia (Piscataway, N.J.) and was
the source of the kanamycin resistance gene used as a probe for
Southern hybridization. Plasmid pLP101 was a pBC-SK+-based
plasmid with a 3.9-kb PstI-XbaI insert containing
the htrA gene. To generate pLP102, the pLP101 plasmid was
digested with NdeI and XbaI to liberate 1.6 kb of
DNA downstream of the htrA gene. The noncompatible ends were
blunt ended, and the plasmid was religated. Plasmid pLPHtrA was a
pBC-SK+-based plasmid containing a 2.1-kb PCR-generated
insert with the htrA gene. Plasmid pAM239 containing the
isopropyl-
-D-thiogalactopyranoside (IPTG)-inducible
gfp gene has been described previously (17). Plasmids pH103R, pS212A, p
PDZ1, pPDZ2, and pPDZ1+2 were
constructed by splice overlap extension PCR and cloned into pBC-SK+
(see below). phtrA-lacZ was constructed by cloning a 4-kb
BamHI-EcoRI fragment containing the
lacZ gene from pEU730 (19) into the low-copy vector pTLP6 (Cmr) (44), and the resulting
plasmid was designated placZ. To generate the promoter
fusion construct, the htrA promoter was amplified by PCR
using pfu polymerase. Primers used to amplify the
htrA promoter were pP1Xb (5'-GGCTGCAGAACCAATCTGG-3')
and pP2BH (5'-GCGGATCCTTATTAATCCTGATTTTACTCATTAATCC-3'). The resulting fragment was ligated into placZ
(designated phtrA-lacZ) so that the promoter was inserted
immediately upstream of the lacZ gene.
Construction of point mutations and in-frame deletions.
Splice overlap extension PCR was performed using pfu
polymerase (Stratagene, La Jolla, Calif.) as we previously described to
generate various mutants (6). PCR primers used for the
synthesis of pS212A were pCATA-Ps (5'-GGCTGCAGAACCAATCTGG-3'),
pS212A-B (5'-CCAAAGCACCTCCTGCATTACCGG-3'),
pS212A-C (5'-CCCGGTAATGCAGGAGGTGCTTTGG-3'), and pCATD-Xb (5'-GCTCTAGATGTGAAATGGTGGTATGGG-3'). The
underlined bold residues are the point mutations. The PCR product of
the pCATA-Ps and pS212A-B primer pair and the pS212A-C and pCATD-Xb primer pair were mixed and amplified to generate S212A-AD. PCR primers
used for the synthesis of pH103R were pCATA-Ps (described above),
pH103R-B (5'-CGAATAACACGGTCATTCGTTATAATAATGC-3'), pH103R-C (5'-GCATTATTATAACGAATGACCGTGTTATTCG-3'),
and pCATD-Xb (described above). The underlined bold residues are
the point mutations. The PCR products of the pCATA-Ps and pH103R-B
primer pair and the pH103R-C and pCATD-Xb primer pair were mixed and amplified to generate H103R-AD. PCR primers used to generate the deletion construct pPDZ1 were pCATA-Ps (described above), pPDZ1-B (5'- GATATCTGTGACTTGCTGCGCTACATCTTTTGCCATATTAATTGG-3'), pPDZ1-C (5'-GTAGCGCAGCAAGTCACAGATATCAAAAAACATGAA CAAAAATTACAATCC-3'), and pCATD-Xb (described above). The two PCR products were mixed and amplified to generate pPDZ1-AD. PCR primers used to generate the
deletion construct pPDZ2 were pCATA-Ps (described above), pPDZ2-B
(5'-GGATAAGAAATTTATGTAAGCGGCTTATTATCCCGC-3'), pPDZ2-C
(5'-GCCGCTTACATAAATTTCTTATCCTAATAACGAAATAACGC-3'), and pCATD-Xb (described above). The two PCR products generated by the
pCATA-Ps and pPDZ2-B primer pair and the pPDZ2-C and pCATD-Xb primer pair were mixed and amplified to generate pPDZ2-AD. PCR primers used to generate the deletion construct pPDZ1+2 were pCATA-Ps (described above), pPDZ-B
(5'-GGATAAGAAATTTATTGCTGCGCTACATCTTTTGCCATATTAATTGG-3'), and
pPDZ-C (5'-GTAGCGCAGCAATAAATTTCTTATCCTAATAACGAAATAACGC-3'). The two PCR products generated by the pCATA-Ps and pPDZ-B
primer pair and the pPDZ-C and pCATD-Xb primer pair were mixed and
amplified to generate pPDZ-AD. Each mutant construct generated by
PCR was confirmed by sequencing.
Infection protocol. Macrophage-like U937 cells and human type I alveolar epithelial cells (WI-26 VA4; ATCC CCL-95.1) and axenic A. polyphaga were maintained and used for infections as described previously (26, 27). Infections to determine growth kinetics and cytotoxicity were performed as described previously (25). A multiplicity of infection (MOI) of 0.5 was used to determine bacterial growth kinetics and cytopathogenicity in U937 macrophage-like cells, WI-26 alveolar epithelial cells, and A. polyphaga. The number of intracellular bacteria was determined as we previously described (26). At least three independent experiments, in triplicate, were performed for all infections.
An MOI of 1 to 20 was used in laser scanning confocal microscopy experiments for the determination of LAMP-2 colocalization (see below). Coinfection experiments were performed as described previously (17) using AA100 at an MOI of 5, 10, 20, or 40 and GT20(pAM239) or GL10(pAM239) was added simultaneously with AA100 at an MOI of 20, 40, 80, or 160. An MOI of 50 was used for DNA fragmentation assays (see below). An MOI of 10 in six-well plates was used for lacZ promoter fusion studies. At least three independent experiments, in triplicate, were performed.Antibodies, stains, and laser scanning confocal microscopy. Confocal laser scanning microscopy and sample analysis using monoclonal anti-LAMP-2 (H4B4) antibody and differential detection of intracellular and extracellular bacteria were performed exactly as we described previously (29). For colocalization experiments of the two strains, all bacteria were labeled with polyclonal anti-L. pneumophila antibody and stained with secondary antibody labeled with Alexa Red or indocarbocyanine (red pseudocolor). Mutant strains harbored the plasmid pAM239 encoding gfp to differentiate them from AA100. Triplicate samples from at least three independent experiments were analyzed.
Promoter expression assays.
AA100 harboring
phtrA-lacZ or placZ was used to infect U937 cells
or A. polyphaga cells at an MOI of 10 for 1 h, followed by 1 h in gentamicin (50 µg/ml) to kill extracellular bacteria (26). At the end of each time interval, U937 monolayers
were lysed hypotonically, and A. polyphaga monolayers were
lysed with 0.05% Triton X-100 and treated with 10 µl of 10-mg/ml
DNase I for approximately 20 min. The bacteria and cellular debris were pelleted and washed twice with Z-buffer (40 mM
NaH2PO4 · H2O, 60 mM
Na2HPO4 · 7H2O, 10 mM KCl, 1 mM MgSO4 · H2O, 40 mM
-mercaptoethanol [pH 7]), followed by assay for -galactosidase
activity using 7 mM fluorodiisogalactopyranoside (FDG);(Molecular
Probes, Eugene, Oreg.), as described previously (36). The
fluorescence was measured using a Perkin Elmer luminescence
spectrometer LS50B at an excitation wavelength of 488 nm and an
emission wavelength of 520 nm. The -galactosidase activity of each
sample was measured as the increase in fluorescence over time per CFU
and calculated as (fluorescence per minute per CFU × 5 × dilution factor), as described previously (42). Background
fluorescence, determined as the increase in fluorescence generated by
the AA100(plac) control under identical conditions, was
subtracted from the final calculated value at each time point. The data
are presented as the ratio of arbitrary fluorescence units per CFU of
intracellular bacteria to arbitrary fluorescence units per CFU of in
vitro-grown bacteria.
Infection of A/J mice. A/J mice were inoculated intratracheally with 106 CFU of L. pneumophila strains, as we previously described (27). The CFU from homogenized lungs were enumerated on BCYE agar containing polymyxin B, cefamandole, and anisomycin (BCYE+PAC; Becton Dickinson, Cockeysville, Md.) after 3 to 4 days of incubation.
DNA fragmentation analysis and hemolysis assays. DNA fragmentation analysis was performed at 3 h postinfection as we previously described (21). Contact-dependent hemolysis of sheep red blood cells was performed as previously described (11).
Sensitivity to in vitro stress. To examine sensitivity to NaCl, bacteria were grown in BYE broth in a 37°C shaker incubator to post-exponential phase (optical density at 550 nm [OD550] = 2.1). Cultures were diluted to an OD550 of 1 and plated on BCYE plates in the presence or absence of 0.6% NaCl for enumeration of bacteria as we described before (26).
To examine sensitivity to heat stress, bacteria grown in BYE broth to post-exponential phase were diluted to an OD550 of 1.0, and aliquots were incubated in triplicate at 37 or 53°C for 1 h, as described previously (6). Following incubation, aliquots were plated on BCYE plates for enumeration of viable bacteria. To examine sensitivity to oxidative stress, post-exponential-phase broth-grown bacteria were resuspended at an OD550 of 1.0 in BYE broth, pelleted, and resuspended in various concentrations of H2O2 for 30 min at 37°C (6). Following incubation, aliquots were plated on BCYE for enumeration of viable bacteria. Alternatively, bacteria were spread on BCYE plates to generate a lawn of bacteria, and a filter disk saturated with 1 µl of 30% H2O2 was placed in the center of the plate. After 72 h of incubation, the zone of inhibition around the filter disk was measured. At least three independent experiments, in triplicate, were performed.| |
RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Intracellular growth of GT20 within mammalian and protozoan
cells.
Initially, characterization of the 121 transposon insertion
mutants of L. pneumophila (25, 26) was
performed using L. pneumophila grown in broth to an
OD550 of ~1 (mid-exponential phase) and showed that GT20
was largely killed by the macrophages by 48 h postinfection
(25). Recently, it has been shown that post-exponential-phase L. pneumophila exhibit enhanced
virulence compared to mid-log-phase bacteria (14).
Therefore, we reexamined the phenotype of GT20 using 3-day plate-grown
bacteria or post-exponential-phase broth-grown bacteria
(OD550 of 2.1 to 2.2). Under these growth conditions, the
mutant GT20 remained severely defective for intracellular replication
within U937 macrophages (Fig. 1a) and
WI-26 epithelial cells (Fig. 1b). In contrast,
post-exponential-phase-grown GT20 was able to replicate within the
protozoan host A. polyphaga. There were approximately
10-fold-fewer GT20 compared to AA100 by 72 h postinfection (Fig.
1c), but this difference was not due to an increased sensitivity of
GT20 to the A. polyphaga assay buffer used throughout the
infection process (data not shown). In vitro growth of GT20 in BYE
broth and on solid medium was similar to that of the parental strain
(data not shown).
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Cytopathogenicity to U937 macrophage-like cells.
Intracellular
replication of L. pneumophila within the host cell is
associated with killing of the host cell. The data showed that while
AA100 was ~100% cytopathogenic by 72 h, GT20 was completely noncytopathogenic (Fig. 2a). Since both
the induction of apoptosis and the pore-forming activity of
L. pneumophila contribute to killing of mammalian cells
(11, 21), we examined both modes of killing by GT20. Our
results showed that GT20 was as effective at inducing DNA
fragmentation, consistent with apoptosis, as the wild-type strain AA100
(Fig. 2b). In addition, GT20 and AA100 exhibited similar levels of
contact-dependent pore formation when examined by hemolysis of sheep
red blood cells (Fig. 2c). Taken together, the data indicated that the
noncytopathogenicity of GT20 was due to the severe defect in
intracellular replication.
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size standard is shown on the left. (c)
Contact-dependent hemolysis of sheep red blood cells following 1 h
of incubation at a bacterium-blood cell ratio of 25:1. Hemolysis was
measured spectrophotometrically at A415. RBC
represents red blood cells incubated in the absence of bacteria. These
data are representative of at least three independent experiments
performed in triplicate. The absence of error bars indicates very small
standard deviations that could not be displayed.
Intrapulmonary replication in A/J mice.
To examine the
virulence of GT20 in vivo, A/J mice were intratracheally inoculated
with 106 bacteria of either the wild-type AA100 or the
mutant GT20 strain. As shown in Table 1,
by 48 h postinfection, while there was at least a 100-fold increase in
the number of bacteria recovered from the lungs of the mice infected by
AA100, there was a 10-fold decrease in the number of GT20 recovered. In
addition, while AA100 persisted through 7 days postinfection, GT20 was
effectively cleared by 72 h postinfection. The data showed that
the severely defective phenotype of GT20 within macrophages and
alveolar epithelial cells in vitro correlated with its defect in
intrapulmonary replication.
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Genetic characterization and complementation of the defective locus
in GT20.
A chromosomal EcoRI fragment containing the
mini-Tn10::kan cassette and flanking
Legionella DNA was subcloned from GT20 genomic DNA,
and the regions flanking the kan cassette were sequenced. The kan cassette was inserted within the C terminus of a
726-nucleotide open reading frame (ORF), ORF 2, 22 nucleotides upstream
of the termination codon (Fig. 3a). ORF 2 was preceded immediately upstream by a 474-nucleotide ORF (ORF 1) and
followed, 17 nucleotides downstream, by a 1,377-nucleotide ORF (ORF 3).
A perfect inverted repeat was located 42 nucleotides downstream of the
termination codon of ORF 3, indicating rho-independent termination
(Fig. 3b). The next downstream ORF (ORF 4) was located 1,043 nucleotides from the termination codon of ORF 3 (Fig. 3a).
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E
(37). Within the sequence upstream of the putative
L. pneumophila htrA start codon, a putative
E promoter region was identified (Fig. 3b)
(37). Interestingly, the plasmid pLPHtrA, which lacked the
putative 
35 region of the predicted E promoter, did
not complement the defective phenotype of GT20 (data not shown),
suggesting a role for this putative promoter in the expression of
htrA (Fig. 3a). Further promoter studies, however, must be
performed to confirm the role of this putative promoter in the
expression of htrA.
Mutational analyses of the conserved regions of HtrA and their
effects on function.
Analysis of the amino acid sequence of the
htrA gene revealed the presence of certain features
conserved in HtrA that were also conserved in the L. pneumophila HtrA homologue (Fig. 3b and c). These include a
hydrophobic leader peptide predicted to be cleaved between residues 23 and 24, an RGD domain, two tandem PDZ domains, and a trypsin-like
catalytic domain (Fig. 3c) containing three conserved residues, His,
Asp, and Ser, which constitute the catalytic triad (38).
We generated amino acid substitutions of the His103 and
Ser212 conserved catalytic residues to Arg and Ala,
respectively, resulting in the pLP102-based constructs pH103R and
pS212A, respectively (Fig. 3c). We also generated in-frame deletions of
PDZ1, PDZ2, or both, which were designated pPDZ1, pPDZ2, and
pPDZ1+2, respectively (Fig. 3c). The fidelity of all of these
constructs was confirmed by DNA sequencing. The single amino acid
substitutions as well as the deletion of both PDZ domains (pPDZ1+2)
or PDZ1 alone (pPDZ1) abolished the ability of the htrA
gene to complement the intracellular replication defect of GT20 (Fig.
4a and b). However, pPDZ2 partially complemented GT20 (Fig. 4b). These data confirmed that these conserved residues are essential for the function of L. pneumophila HtrA during the intracellular infection of
macrophages. Although deletion of the PDZ domains in E. coli
htrA does not result in unstable proteins (43), we
cannot exclude that similar deletions in L. pneumophila
htrA may result in unstable proteins.
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Increased sensitivity of GT20 to certain in vitro stress
stimuli.
In E. coli, HtrA has been shown to be a
periplasmic chaperone/serine protease involved in refolding or
degrading misfolded proteins in the periplasm (38) and is
indispensable for survival at elevated temperatures (>42°C)
(38). Our data showed that GT20 exhibited no difference in
viability compared to the wild-type strain AA100 when incubated at
42°C (data not shown). At 53°C, the viability of GT20 was reduced
by ~10,000-fold compared to the wild-type strain (Fig.
5a). In addition, GT20 exhibited
significantly higher growth inhibition (>10,000-fold) in the presence
of 0.6% NaCl than the wild-type AA100 (Fig. 5b). These temperature and salt sensitivities were complemented by the htrA gene in
trans. In contrast, AA100 and GT20 exhibited similar
sensitivity to oxidative stress (zones of inhibition by
H2O2 were 37.375 ± 1.411, 36.89 ± 0.536, and 37.75 ± 1.494 mm, respectively). In addition, GT20 did
not display any increased sensitivity when incubated for 16 h at
pH 3, 5.2, or 6.2 compared to the wild-type strain (data not shown).
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Intracellular trafficking of GT20. Laser scanning confocal microscopy was used to examine colocalization of the GT20 phagosomes with the late endosomal-lysosomal marker LAMP-2 at 2 h postinfection of U937 macrophages. The visual assessment of colocalization was corroborated by measurement of fluorescence intensity across the phagosome (29). Colocalization was determined by the presence of two completely overlapping fluorescence peaks (one green for LAMP-2 and one blue for intracellular bacteria) (see, for example, Fig. 4 in reference 29). Of 59 phagosomes examined, 86.5% of the GT20 phagosomes colocalized with LAMP-2. In contrast, of 75 phagosomes examined, only 17.3% of the AA100 phagosomes colocalized with LAMP-2. As expected, of 67 phagosomes examined, 90% of the paraformaldehyde-killed bacterial phagosomes colocalized with LAMP-2. Therefore, the inability of GT20 to replicate intracellularly was associated with a defect in intracellular trafficking.
htrA mutant is unable to replicate within a niche
created by parental strain.
To examine whether the defect in
trafficking of the htrA mutant was due to intolerance of the
microenvironment within the phagosome, we coinfected U937 macrophages
with the wild-type strain AA100 and either the htrA mutant
GT20 or the dotA mutant GL10 derivative of AA100
(26) to examine whether colocalization with AA100 could
rescue each mutant for intracellular replication. Coinfections were
performed using AA100 and gfp-expressing GT20 or GL10.
Phagosomes were examined at 2, 10, and 16 h postinfection using
laser scanning confocal microscopy. As expected, at 2 h there was
no evidence of intracellular replication of any of the strains (data
not shown). In single infections, there was no evidence of replication
of GT20 or GL10 at any time point tested (data not shown). When GT20 or
GL10 was present in phagosomes lacking AA100 in the dual infections,
there was no detectable replication of either of the mutants at any
time point examined (data not shown). In coinfection experiments with
AA100 and GL10, of 692 phagosomes examined at 16 h postinfection,
5.5% colocalization of AA100 and GL10 was observed. In 23.6% of the
coinhabited phagosomes, rescue of GL10 was clearly observed (Fig. 6b
and d). Results were similar at 10 h postinfection
(673 phagosomes examined). In coinfection experiments using AA100 and
GT20, of 472 phagosomes examined at 16 h postinfection, 23%
colocalization of AA100 and GT20 was observed. In contrast to the
dotA mutant, no detectable replication of GT20 was ever
observed in communal phagosomes (Fig. 6a and c). Similar results were
observed at 10 h postinfection (262 phagosomes examined). In
qualitative examination of thousands of coinfected cells at 10 h
and 16 h postinfection, we never observed any detectable replication of GT20. Our data showed that rescue of the htrA
mutant for the defect in intracellular trafficking was not sufficient to rescue its intracellular replication and that the replication defect
of the htrA mutant was most likely due to an inability to
withstand the phagosomal microenvironment in mammalian cells.
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Expression of htrA within macrophages and within
protozoa.
Although it is well documented that L. pneumophila is exposed to stress stimuli within macrophages
(8, 31), it has never been examined whether a similar
stress response is also manifested within protozoa. This prompted us to
use the htrA promoter to probe the phagosomal
microenvironment for exposure of L. pneumophila to
stress stimuli within protozoa and contrast that to mammalian cells. We
constructed a promoter fusion of the L. pneumophila htrA to the promoterless lacZ gene on a low-copy-number
vector (designated phtrA-lacZ) to monitor the kinetics of
expression of htrA during the intracellular infection of
macrophages. The use of FDG fluorescence substrate for
-galactosidase facilitated detection of expression during early
stages of the infection, when the number of intracellular bacteria is
small. The background of -galactosidase activity from the vector
with the promoterless lacZ gene was subtracted from the
-galactosidase activity of phtrA-lacZ under the same
experimental conditions and each time point examined (4, 8, and 14 h). The -galactosidase activity increased by 12,320- to 20,545-fold
throughout the intracellular infection of macrophages compared to
bacteria incubated in tissue culture medium or in BYE broth (Fig.
7). There was no significant difference in
-galactosidase expression between in vitro-grown bacteria incubated
in BYE and in tissue culture medium or during different phases of
growth in BYE (Fig. 7). In addition, the macrophage lysates had no
detectable effect on expression of -galactosidase by in vitro-grown
bacteria (data not shown). When AA100 harboring the
htrA-lacZ promoter construct was used to infect A. polyphaga, the -galactosidase activity was induced by 120- to
500-fold compared to bacteria incubated in assay medium or in BYE (Fig.
7). The lysate of amoebae had no detectable effect on expression of
-galactosidase by in vitro-grown bacteria (data not shown). These
data showed that although htrA was induced within both
macrophages and protozoa, levels were consistently much higher within
macrophages (by approximately 100
fold) than in protozoa.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Despite evasion of the major microbicidal mechanisms of macrophages (35) and the profound modifications of the phagosome (1), L. pneumophila manifests the induction of many stress proteins during intracellular replication (1, 4, 18). However, the role of the stress response in the intracellular survival of L. pneumophila is not known. In addition, whether L. pneumophila is exposed to stress stimuli within protozoa has never been demonstrated. Here we show that a stress-induced gene (htrA) of L. pneumophila is indispensable for the intracellular replication of L. pneumophila within mammalian but not protozoan cells. We show that regardless of the growth phase at which the infection is initiated, the htrA mutant is severely impaired in its ability to replicate intracellularly within macrophages and epithelial cells, yet exhibits a parental strain-like phenotype within protozoa. Importantly, the inability of the htrA mutant to replicate within mammalian cells in vitro correlates with a similar defect in intrapulmonary replication in A/J mice. Similarly, htrA mutants of other bacteria also exhibit a defect in intracellular survival and replication within macrophages and are also attenuated in animal models (12, 15). These observations provide strong evidence that although these intracellular bacteria inhabit distinct niches within their host cells, they are all exposed to stressful conditions within their phagosomal microenvironments (8, 31), but the nature of these stress stimuli is likely to be different for different pathogens.
Although alveolar epithelial cells are not professional phagocytic cells, the htrA mutant is similarly defective for intracellular replication within these cells. Although it is well established that numerous stress proteins are induced by L. pneumophila during the intracellular infection of macrophages, the essential role of HtrA during the intracellular infection of alveolar epithelial cells provides the first evidence that the stress response (mediated at least in part by HtrA) is indispensable for the intracellular survival and replication of L. pneumophila within macrophages and epithelial cells.
We have demonstrated that amino acid substitution of either of two of the conserved catalytic residues, His103 and Ser212, renders the L. pneumophila HtrA nonfunctional during the intracellular infection of macrophages. Similar substitutions in the E. coli HtrA also results in loss of function. Our data also show that deletion of either both PDZ domains or PDZ1 alone completely disrupts the function of HtrA during intracellular infection of macrophages, while deletion of PDZ2 alone resulted in partial function of HtrA in the intracellular infection. Similar deletions in E. coli HtrA result in a similar pattern of loss of function (43). Our data confirm an essential role of the L. pneumophila HtrA during the intracellular infection of macrophages and epithelial cells.
We have shown that the htrA mutant is unable to exclude the late endosomal-lysosomal marker LAMP-2 from its phagosome. In addition, we have previously shown, by electron microscopy, that the GT20 phagosome does not associate with the rough endoplasmic reticulum within macrophages, yet does recruit this organelle during replication within protozoa (25). Therefore, the defect in intracellular replication within macrophages is associated with the inability of the htrA mutant to perform essential modifications of its phagosome at early stages of the infection.
The observation that the L. pneumophila htrA mutant is found in a phagosome that colocalizes with LAMP-2 suggests that the mutant may be unable to properly fold the proteins (including the Dot/Icm proteins) necessary for the rapid establishment of its protective replicative niche, resulting in trafficking of the phagosome along the "default" endosomal-lysosomal degradation pathway (38, 43). It has recently been demonstrated that several dot/icm mutants, including a dotA mutant, which are defective in early phagosomal modulation and are trafficked into a phagolysosome, can be rescued by the parental strain when they occupy a communal phagosome (17). Similarly, we have demonstrated that a dotA mutant can also be rescued when it resides within a communal phagosome with the parental strain. In contrast, the htrA mutant cannot be rescued by the parental strain when they inhabit the same phagosome. Thus, the defect in intracellular trafficking of the htrA mutant is most likely due to an intolerance of the phagosomal microenvironment inhabited by the wild-type strain within the macrophage.
Our data suggest that the intracellular niche inhibited by L. pneumophila within protozoa is less stressful than that of mammalian cells. This is supported by several lines of evidence. First, the number of GT20 recovered at 72 h postinfection of A. polyphaga is consistently 10-fold less than that of AA100, suggesting that L. pneumophila may be exposed to a low level of stress stimuli within protozoa, or that HtrA plays a minor role in this host. In contrast, there is no detectable replication of the htrA mutant within mammalian cells. Second, promoter fusion studies revealed that the induction levels of the htrA promoter are approximately 100-fold higher during the intracellular infection of macrophages compared to protozoa. It is possible that different stress stimuli are encountered by L. pneumophila within protozoa, such that additional proteins induced within protozoa, but not within macrophages, may compensate for the absence of HtrA within protozoa. Our data favor the prediction that it is more likely that L. pneumophila is exposed to a significantly lesser degree of stress stimuli within protozoa than within macrophages. We have recently shown that the Rep helicase of L. pneumophila, which is required for DNA repair following damage by stress stimuli, is also indispensable with mammalian cells but not within protozoa (30). These observations provide compelling evidence that although the intracellular infection is similar at the molecular and ultrastructural levels (3, 13, 26, 41), significant differences exist between the phagosomal microenvironments within protozoan and mammalian host cells. It is possible that the different receptors (10, 33, 46, 47) utilized in both host cells to internalize legionellae result in different signaling events that result in exposure to stress stimuli within mammalian but not protozoan cells.
In summary, we have provided evidence that differences exist in the phagosomal microenvironments within protozoan and mammalian cells. Despite its dispensability within protozoa, HtrA is essential for L. pneumophila replication within macrophages and epithelial cells and for intrapulmonary replication, the hallmarks of Legionnaires' disease. The data show a critical role for the stress response mediated, at least in part, by HtrA, in the intracellular replication of L. pneumophila within mammalian cells.
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ACKNOWLEDGMENTS |
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Y.A.K. is supported by Public Health Service grants R29AI38410 and RO1AI43965.
We thank Craig R. Roy for kindly providing the pAM239 plasmid. We thank Lian-Yong Gao for technical help. We also thank Bruce Maley, Omar S. Harb, Richard Watson, and Mary Gail Engle for technical assistance with laser scanning confocal microscopy.
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Microbiology and Immunology, University of Kentucky Chandler Medical Center, Lexington, KY 40536-0084. Phone: (859) 323-3873. Fax: (859) 257-8994. E-mail: yabukw{at}pop.uky.edu.
Editor: J. T. Barbieri
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Infection and Immunity, April 2001, p. 2569-2579, Vol. 69, No. 4
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.4.2569-2579.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
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