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Infection and Immunity, August 1999, p. 4208-4215, Vol. 67, No. 8
Division of Infectious Diseases,
Received 12 February 1999/Accepted 4 May 1999
Neonatal bacterial meningitis remains a disease with unacceptable
rates of morbidity and mortality despite the availability of effective
antimicrobial therapy. Citrobacter spp. cause neonatal meningitis but are unique in their frequent association with brain abscess formation. The pathogenesis of Citrobacter spp.
causing meningitis and brain abscess is not well characterized;
however, as with other meningitis-causing bacteria (e.g.,
Escherichia coli K1 and group B streptococci), penetration
of the blood-brain barrier must occur. In an effort to understand the
pathogenesis of Citrobacter spp. causing meningitis, we
have used the in vitro blood-brain barrier model of human brain
microvascular endothelial cells (HBMEC) to study the interaction
between C. freundii and HBMEC. In this study, we show that
C. freundii is capable of invading and trancytosing HBMEC
in vitro. Invasion of HBMEC by C. freundii was determined to be dependent on microfilaments, microtubules, endosome
acidification, and de novo protein synthesis. Immunofluorescence
microscopy studies revealed that microtubules aggregated after HBMEC
came in contact with C. freundii; furthermore, the
microtubule aggregation was time dependent and seen with C. freundii but not with noninvasive E. coli HB101 and
meningitic E. coli K1. Also in contrast to other meningitis-causing bacteria, C. freundii is able to
replicate within HBMEC. This is the first demonstration of a
meningitis-causing bacterium capable of intracellular replication
within BMEC. The important determinants of the pathogenesis of C. freundii causing meningitis and brain abscess may relate to
invasion of and intracellular replication in HBMEC.
Citrobacter freundii is a
member of the family Enterobacteriaceae and is often the
cause of significant opportunistic infections. C. freundii
has also been associated with neonatal meningitis and brain abscess
(14). The mortality and morbidity rate of Citrobacter meningitis is unacceptably high. The fatality
rate associated with neonatal meningitis is 25 to 50%; moreover,
serious neurological sequelae result in 75% of survivors. Although the implication Citrobacter spp. in neonatal meningitis and
brain abscess is clear, the mechanisms by which these organisms cause disease have been poorly investigated.
One of the least understood aspects of bacterial meningitis is the
mechanisms by which bacteria traverse the blood-brain barrier. Escherichia coli K1 and group B streptococci (GBS), the two
leading causes of bacterial meningitis in neonates, have offered
excellent models for studying bacterial penetration of the blood-brain
barrier. We have previously shown that E. coli K1 and GBS
invade brain microvascular endothelial cells (BMEC) in vitro and are
capable of penetrating the blood-brain barrier in the experimental
newborn rat model of hematogenous meningitis (1, 15, 20).
However, in contrast to Citrobacter spp., there is a much
lower association of brain abscess formation with these organisms
(8, 14). This observation suggests that
Citrobacter spp. may utilize different pathogenic mechanisms
for penetrating and/or replicating in the central nervous system. In an
effort to understand the pathogenesis of Citrobacter spp.
causing meningitis, we have used the in vitro blood-brain barrier model
of human BMEC (HBMEC) to study the interaction between C. freundii and HBMEC. Here we report on the capacity of C. freundii to invade, replicate, and traverse HBMEC in vitro and
present data on the eukaryotic mechanisms for the invasion process.
Bacterial strains.
The C. freundii strain
used in this study, 3009rif, is a spontaneous
rifampicin-resistant mutant derived from urinary tract isolate 3009 (22) that retains wild-type morphology, growth
characteristics, and invasive phenotype (data not shown). Bacteria were
grown aerobically for 14 h at 37°C in brain heart infusion broth
(Difco Laboratories, Detroit, Mich.) with rifampicin (100 µg/ml)
selection. For confocal microscopy experiments, we generated a
construct constitutively expressing gfp; this clone contains
the promoter region of rpsM, which encodes the ribosomal
protein S13. Oligonucleotides that hybridize 5' and 3' of the promoter
region were generated based on the sequence of E. coli K12
rpsM. PCR was performed to amplify the rpsM
promoter, using C. freundii chromosomal DNA as the template. The PCR product was then cloned immediately 5' of the promoterless gfpmut3A construct in the promoter trap vector, pFPV25
(34). This clone was then electroporated into wild-type
C. freundii and assessed for fluorescence. It was determined
that the rpsM::gfpmut3A plasmid gave
rise to highly fluorescent colonies (as visualized by fluorescence
microscopy). This clone did not affect the growth rate, cell density,
or ability of wild-type C. freundii to invade HBMEC.
HBMEC cultures.
HBMEC were isolated from a brain biopsy of
an adult female with epilepsy by previously described methods
(30). These cells were positive for factor VIII-Rag,
carbonic anhydrase IV, and Ulex europaeus agglutinin I. They
took up fluorescently labeled low-density lipoprotein and expressed
gamma glutamyl transpeptidase, thus demonstrating their brain
endothelial cell properties (30). HBMEC were subsequently
immortalized by transfection with simian virus 40 large T antigen and
maintained their morphological and functional characteristics for at
least 30 passages (31, 32). The cells are polarized and
exhibit a transendothelial electric resistance of at least 100 ohms/cm2 (20, 27). HBMEC were plated in 75-ml
tissue cultures flasks previously treated with rat tail
collagen-fibronectin and then cultured in RPMI 1640 supplemented with
heat-inactivated 10% fetal calf serum (Gibco), 10% NuSerum IV (Becton
Dickinson, Bedford, Mass.), 1% modified Eagle's medium nonessential
amino acids, heparin (5 U/ml), sodium pyruvate (1 mM),
L-glutamine (2 mM), vitamins, and penicillin-streptomycin.
Cultures were incubated at 37°C in a humid atmosphere of 5%
CO2.
Invasion assays and inhibition studies.
Invasion assays were
performed as previously described (1), using approximately
107 bacteria added to a well containing a confluent
monolayer of HBMEC at a multiplicity of infection of 100. The number of
intracellular bacteria was determined after the extracellular bacteria
were eliminated by incubation of the monolayer with experimental medium containing gentamicin (100 µg/ml). The MIC of gentamicin for C. freundii was determined to be Transcytosis experiments.
To examine the ability of C. freundii to transcytose polarized HBMEC monolayers, the
double-chamber culture system of Transwell polycarbonate membrane
filters was used as previously described (20, 27). Briefly,
HBMEC were seeded onto the apical side of a 12-mm collagen-coated
polycarbonate membrane with a pore size of 3 µm (Corning Costar
Corp., Cambridge, Mass). The apical chamber of the Transwell contained
0.5 ml of HBMEC medium, while the basolateral chamber contained 1.5 ml
of HBMEC medium.
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Citrobacter freundii Invades and
Replicates in Human Brain Microvascular Endothelial Cells
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
1.0 µg/ml. Results are presented as percent invasion, determined as 100 × [(number of bacteria recovered)/(number of bacteria inoculated)]. Noninvasive E. coli HB101 was used as a negative control.
TEM. Transmission electron microscopy (TEM) was performed on HBMEC incubated with C. freundii for various times. At the designated time point, the HBMEC monolayer was washed four times with RPMI 1640 and gently scraped from the plastic surface. The cell slurry was then centrifuged for 10 min at 7,000 × g. The cell pellet was resuspended and fixed with 2.5% glutaraldehyde in 0.1 M phosphate-buffered saline (PBS). Cells were washed and postfixed with 2% OsO4 for 1 h, rinsed, dehydrated through graded ethanol solutions, and embedded in polypropylene oxide. Ultrathin sections were cut, mounted on colloidion one-hole grids, stained with uranyl acetate and lead citrate, and examined by TEM with a Philips CM transmission electron microscope.
Immunofluorescence.
For staining host cell elements, HBMEC
were grown on eight-well chamber slides and bacteria were added as
described above. At the designated time point, cells were washed three
times with PBS and fixed with 3.7% formaldehyde-0.2% Triton X-100 in
microtubule stabilization buffer (5) for 5 min at room
temperature. Cells were then postfixed with 2% paraformaldehyde in PBS
for 15 min at room temperature and subsequently permeabilized with
0.5% Triton X-100 in PBS for 20 min. The monolayers were first
incubated with anti-
-tubulin monoclonal antibody (Sigma) in PBS
containing 5% normal goat serum, washed three times with PBS, and then
incubated with rhodamine labeled goat anti-mouse antibodies
(Kierkegaard & Perry Laboratories) in PBS containing 5% normal goat
serum. Cells were washed with PBS, chambers were removed, and slides were mounted. Stained cells were visualized with a Zeiss Axioscope confocal microscope.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Ability of C. freundii to invade HBMEC. The ability of C. freundii to enter HBMEC was assessed via tissue culture invasion assays (gentamicin protection assay) as previously described (1). Experiments were performed to optimize and standardize the invasion assays for C. freundii. The frequency of C. freundii invasion was found to be optimal for an inoculum of approximately 107 CFU per well of HBMEC (an approximate multiplicity of infection of 100:1). The incubation time of the bacteria with the HBMEC that yielded the best and most reproducible results was found to be 1.5 h, with a subsequent 1-h incubation in medium containing gentamicin (100 µg/ml) to kill extracellular bacteria (data not shown). With standardized assay conditions, a representative experiment showed that approximately 0.38% ± 0.08% of the C. freundii inoculum was total cellular associated (representing number of bacteria attached and intracellular) and 0.12% ± 0.03% was invasive. Although the noninvasive bacteria control, E. coli HB101, showed similar levels of total cellular-associated inoculum (0.36% ± 0.17%), only 0.001% ± 0.00001% of the inocula invaded HBMEC.
Ability of C. freundii to survive and replicate
within HBMEC.
To ascertain whether C. freundii
survives and replicates within HBMEC, invasion assays were performed as
described above except that the time between the 100-µg/ml gentamicin
treatment and lysis of eukaryotic cells was lengthened. The extended
incubation was done with medium containing a lower level of gentamicin
(20 µg/ml, which was above the MIC). Time points examined were time
zero (as in the standard invasion assay), and 2, 4, and 24 h. As
shown in Table 1, C. freundii
survived extended incubations with HBMEC and demonstrated an increase
of intracellular CFU. An increase in recoverable bacteria was seen at
2 h (0.75% at time zero versus 3.3% at 2 h). Subsequent
time points, however, revealed negligible or no increase in recoverable
intracellular bacteria. These results suggest that C. freundii replicates within the HBMEC and can survive prolonged
intracellular exposure. These data do not distinguish between
exocytosis (or exit) of intracellular bacteria which are then
subsequently killed by the gentamicin in the medium and the ability of
C. freundii to replicate intracellularly long term.
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TEM. TEM was used to characterize the interaction between C. freundii and HBMEC. Infected monolayers were fixed at different times after the addition of bacteria and processed for TEM examination. Figure 1A shows entry of C. freundii after 45 min of incubation with HBMEC. Intimate interaction between the bacteria and the cell surface was observed, with some visible condensation of electron-dense particles accumulating within the vicinity of contact. After 45 min of incubation, C. freundii was occasionally found to be intracellular. After extended incubation for a total of 1.5 h, C. freundii was observed intracellularly in single membrane vacuole-like structures (Fig. 1B).
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Effects of eukaryotic inhibitors on C. freundii invasion of HBMEC. To identify the eukaryotic cellular components necessary for C. freundii invasion, we analyzed the effects of various eukaryotic inhibitors on C. freundii invasion of HBMEC.
(i) Role of microfilaments. The role of actin-based cytoskeleton in C. freundii invasion was examined by using cytochalasin D, an agent that causes microfilament depolymerization in eukaryotic cells (33). We used various concentrations of cytochalasin D to pretreat HBMEC and compared the abilities of C. freundii to invade treated and untreated HBMEC. As shown in Fig. 2A, cytochalasin D had a profound effect on the ability of C. freundii to invade HBMEC. At a cytochalasin D concentration of 0.1 µg/ml, the frequency of invasion was reduced by 75%, while increasing the concentration of cytochalasin D to 0.25 µg/ml led to nearly 100% inhibition of C. freundii invasion. HBMEC treated with cytochalasin D at concentrations of 0.1 to 0.5 µg/ml did not show altered cell morphology.
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(ii) Role of microtubules. To establish an involvement of microtubules in C. freundii invasion of HBMEC, invasion assays were performed with different microtubule inhibitors. Pretreatment of HBMEC with nocodazole, a microtubule-depolymerizing agent (10), led to a dramatic effect on C. freundii invasion of HBMEC. As shown in Fig. 2B, cells pretreated with nocodazole at 1.0 µg/ml demonstrated a 99% decrease in C. freundii invasion. Similar effects were seen when cells were treated with another microtubule-destabilizing agent, colchicine (data not shown). In addition, when the microtubule-stabilizing agent vincristine was used, C. freundii invasion was decreased by nearly 90% (Fig. 2C).
(iii) Role of HBMEC protein synthesis. To examine whether de novo eukaryotic protein synthesis plays a role in C. freundii invasion, invasion assays were performed with cycloheximide-treated HBMEC. Cycloheximide concentrations as low as 1.0 µg/ml profoundly inhibited the invasion of C. freundii (i.e., 98% decrease in invasion as compared to untreated HBMEC) (Fig. 2D). [35S]methionine incorporation experiments determined that 0.1 µg of cycloheximide per ml inhibited protein synthesis in HBMEC (data not shown).
(iv) Endosome acidification but not coated pit formation is required for C. freundii invasion. To examine the role of endosome acidification in the C. freundii invasion process, the inhibitor monensin was used in invasion assays. Monensin is a cationic ionophore that has been shown to increase the pH of intracellular vacuoles (18). Pretreatment of HBMEC with monensin at concentrations of 5 to 50 µg/ml was found to inhibit the susceptibility of HBMEC to C. freundii invasion or survival in a dose-dependent manner (Fig. 2E).
Clathrin-coated pit formation has been shown to be inhibited in eukaryotic cells by monodansylcadaverine (MDC) or oabain (3, 17). Preincubation of HBMEC with MDC at concentrations of 5 to 50 µg/ml showed no effect on the ability of C. freundii to invade HBMEC (Fig. 2F). Similar results were seen when oabain was used to inhibit coated pit formation in HBMEC (data not shown). In contrast, 20 µg of MDC per ml inhibited the ability of E. coli K1 to invade HBMEC by 50%, similar to results previously reported by Prasadarao et al. (24). MDC at concentrations higher than 50 µg/ml appeared to be toxic to the HBMEC and thus could not be assayed. However, control experiments revealed that HBMEC pretreated with 50 µg of MDC per ml significantly protected the eukaryotic cell from diphtheria toxin toxicity (data not shown). Taken together, the above results suggest that C. freundii invasion of HBMEC is dependent on microfilaments, microtubules, de novo protein synthesis, and endosome acidification but not coated pit formation.Microtubule aggregation is associated with C. freundii
invasion of HBMEC.
To further substantiate the apparent role of
microtubules in C. freundii invasion of HBMEC, we examined
by fluorescence microscopy whether there were changes in the
microtubule network. Anti--tubulin staining of noninfected HBMEC
showed uniform staining of microtubules (Fig.
3A). However, when
C. freundii was incubated with HBMEC for 30 min, the
microtubules appeared to be in aggregates (Fig. 3C). This
observed aggregation was a time-dependent process; no effect on the
microtubules was seen when bacteria and HBMEC were incubated
for 5 min (data not shown), and only slight effects were seen when the
incubation time was increased to 15 min (Fig. 3B). The microtubule
aggregation-staining pattern did not appear to coexist with bacterial
binding; other areas of HBMEC that did not have C. freundii
bound also demonstrated pronounced microtubule clumping. Furthermore,
this microtubule aggregation was not observed when C. freundii was incubated for 30 min with nocodazole (5 µg/ml)-pretreated HBMEC (Fig. 3D). Of interest, microtubule
aggregation was not seen when bacteria were incubated for 30 min with
cytochalasin D-pretreated HBMEC (Fig. 3E). Control experiments
performed with noninvasive E. coli HB101 or invasive
E. coli K1 did not show alterations in the HBMEC microtubule
staining pattern (data not shown). These results indicate that a
microtubule-depolymerizing agent can inhibit the formation of C. freundii-dependent microtubule aggregates and that a
microfilament-depolymerizing agent (cytochalasin D) may have direct or
indirect effects on the microtubule-dependent process of C. freundii invasion of HBMEC.
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C. freundii transcytoses polarized HBMEC monolayers. We and others have previously used Transwell experiments as a model system for studying bacterial transcytosis through an intact polarized HBMEC monolayer constituting the blood-brain barrier (20, 27). Briefly, bacteria are added to the apical chamber of polarized HBMEC in the Transwell. After a designated time, the bottom chamber (basolateral side of HBMEC) is sampled to ascertain bacterial penetration through the HBMEC. E. coli HB101 is used as a noninvasive bacteria control. 3H-inulin (4,000 Da) is simultaneously added in the apical chamber and collected with the bacteria from the basolateral chamber to assay for passive diffusion. As shown in Fig. 4, C. freundii could cross the polarized monolayer in a time-dependent process, whereas noninvasive HB101 demonstrated no HBMEC penetration. The levels of 3H-inulin migration were similar for all conditions (i.e., no bacteria versus invasive or noninvasive bacteria added), which indicates that the migration of C. freundii occurs principally through the HBMEC and is not passive and that the integrity of the cells has not been altered.
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, no bacteria; 
, C. freundii; 
, HB101. Results are
presented as a representative assay of four independent experiments,
each performed in triplicate and all yielding similar results.
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DISCUSSION |
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Citrobacter is a significant cause of opportunistic infections; C. diversus is associated with approximately 40% of presenting cases, while C. freundii represents approximately 29% (11). Citrobacter spp. cause neonatal meningitis and have an unusual propensity for causing brain abscess (8, 14). The pathogenesis of Citrobacter spp. causing meningitis and brain abscess is not well characterized; however, as with other meningitis-causing bacteria, penetration of the blood-brain barrier must occur. The present study was undertaken to better understand the potential interactions of Citrobacter with the blood-brain barrier. C. freundii was chosen as a model bacterium for these studies because the bacterial genetics are better defined and a genomic library is available for eventual studies regarding the molecular basis of Citrobacter invasion and replication in HBMEC. Experiments performed with a cerebrospinal fluid isolate of C. diversus yielded similar results (data not shown), suggesting that the frequency and mechanism of HBMEC invasion for these two species may be alike.
The blood-brain barrier is a complex structure that consists of the choroid plexus epithelium and the brain capillary endothelium. The presence of tight junctions and low pinocytotic activity for the endothelial cells results in the restriction of macroelements passing through the blood-brain barrier. At this time, it is not known where in the blood-brain barrier C. freundii penetrates, but the choroid plexus was found to be rarely involved in the infant rat model of experimental hematogenous Citrobacter meningitis (16). In addition, endothelial microvascular cells cover the largest surface area of the blood-brain barrier, and other meningitis-causing bacteria have been shown to invade microvascular endothelial cells in vitro (13, 20, 25). We therefore selected HBMEC for our study. Tissue culture invasion assays and TEM studies provided evidence that C. freundii invades HBMEC. Results from invasion assays performed in the presence of various eukaryotic cellular inhibitors suggest that the invasion of C. freundii into HBMEC is a microfilament-, microtubule-, de novo protein synthesis-, and endosome acidification-dependent process. Extended invasion assays determined that C. freundii can survive and replicate intracellularly for prolonged periods in vitro. TEM analyses revealed the intracellular location of individual and multiple C. freundii cells to be within single membrane vacuole-like structures. Transwell experiments demonstrated that C. freundii could traverse a polarized monolayer of HBMEC, whereas noninvasive E. coli could not. Furthermore, our preliminary data shows that C. freundii penetrates the blood-brain barrier in the neonatal rat model of experimental hematogenous meningitis (21). Taken together, these findings suggest that C. freundii invades vacuoles, possibly replicates, transcytoses through the HBMEC, is released into the basolateral side, and thus penetrates the blood-brain barrier.
Invasion of eukaryotic cells by C. freundii has been reported (22, 35). However, this is the first report on the invasion of HBMEC by C. freundii. Curiously, the eukaryotic requirements for C. freundii invasion are as diverse as the cell types that C. freundii has been shown to invade. For example, the clathrin-coated pit inhibitor MDC has been shown to inhibit C. freundii invasion in all other cell types assayed (e.g., human vascular, intestinal, and bladder epithelial cells) except, as shown in this study, HBMEC. In addition, other meningitis-causing bacteria characterized thus far enter HBMEC in a route(s) that is dependent on microtubules and is MDC sensitive (20, 24, 27). Clathrin-coated pit inhibitors MDC and ouabain have not been shown to inhibit all receptors; thus, it may be that the receptor necessary for C. freundii invasion of HBMEC is not affected by the inhibitor MDC or ouabain. Although evidence collected so far suggests that C. freundii entry into HBMEC may not occur through an MDC- or oabain-sensitive receptor-mediated route, it does appear that endosome acidification and de novo protein synthesis are both required. The available data suggest two possible scenarios. Endosome acidification may be needed as an environmental trigger for intracellular bacterial survival. Similar requirements have been characterized for Salmonella epithelial invasion (26). Alternatively, endosome acidification and protein synthesis may be required for the separation of ligand-receptor complex, synthesis of receptor, and/or presentation of receptor to HBMEC surface in order for C. freundii invasion to occur. The latter scenario is reminiscent of other invasive pathogens, where contact of the viable organism is needed for modulation of eukaryotic cell adhesion molecules that are necessary for invasion (e.g., Streptococcus pneumoniae and platelet-activating factor receptor) (2). Experiments are in progress in our laboratory to distinguish between these proposed scenarios.
Invasion assays performed in the presence of microtubule inhibitors
(both depolymerizing and stabilizing agents) significantly decreased
the ability of HBMEC to take up C. freundii. Confocal microscopy experiments with anti--tubulin antibodies showed that microtubules aggregate after HBMEC come in contact with C. freundii. The microtubule aggregation was a time-dependent
process; no aggregation was seen at 5 min, little seen in 15 min, and
clear-cut aggregation was observed after 30 min of incubation of
C. freundii with HBMEC. This microtubule aggregation was
inhibited when cells were treated with either microtubule inhibitors or
microfilament-inhibiting agents. Of interest, the microtubule
aggregation staining pattern did not colocalize with bacterial binding
and areas of HBMEC which did not show C. freundii binding
also demonstrated pronounced microtubule clumping. This suggests that
the contact of the bacteria with HBMEC may globally stimulate
microtubule aggregation. Whether the microtubule aggregation is a
result of a secreted bacterial factor or paracrine response to bacteria
binding to HBMEC remains to be seen. Furthermore, the aggregation of
microtubules in response to C. freundii binding may be
related to the postulated receptor presentation via de novo protein
synthesis and endosome acidification. It has been previously shown that
the transport of many receptors to and from the cell surface is
dependent on microtubules (10). Therefore, one explanation
for the inhibitory effect of microtubule inhibitors on entry of
C. freundii into HBMEC is that the agents may decrease the
numbers of HBMEC receptors that mediate C. freundii invasion. Experiments are under way to discern between these possibilities.
Microtubules have previously shown to be required for invasion of many pathogens (e.g., Neiserria gonorrheae, Haemophilus influenzae, enteropathogenic and enterohemorrhagic E. coli, and Campylobacter jejuni (4, 9, 22, 23, 29). General thinking has been that although these pathogens may enter through microtubule-dependent pathways, they usually do not replicate intracellularly (6). The data acquired in this study from extended invasion assays and TEM analysis suggest that C. freundii may be an exception to that generalization. In contrast to what has been described for another intravacuole-replicating bacterium, Legionella pneumophila (12), there was no appearance of mitochondria or ribosomes in close proximity to the bacteria. This suggests that C. freundii may not use these organelles to directly obtain energy or that recruitment of specific host cell proteins may not be required for intracellular survival and proliferation (as in the case of L. pneumophila). Of particular relevance to central nervous system infections, other meningitis-causing bacteria such as E. coli K1, GBS, and S. pneumoniae have similarly been shown to invade (1, 13, 25) or invade and transcytose (20, 27) BMEC; however, the organisms have not been found to replicate within HBMEC. As described above, Citrobacter meningitis has been documented for its high frequency of brain abscess formation. Whether replication within HBMEC vacuoles is unique for Citrobacter and if there is a correlation with abscess formation remains to be determined.
Cytochalasin D inhibits C. freundii invasion into HBMEC; however, using immunostaining, we found no detectable reorganization of microfilaments when C. freundii interacted with HBMEC (data not shown). In addition, cytochalsin D pretreatment of HBMEC inhibited the bacterium-dependent microtubule aggregation as visualized by confocal microscopy. There may be several explanations for these results. The cytochalsin D effect on bacterium-dependent microtubule aggregation may be due to indirect effects of the microfilament inhibitor on the microtubule network. For example, microtubules have been observed to act as anchoring structures for F-actin (28). Therefore, disruption of the microfilament network may affect the microtubule network and thus indirectly affect the microtubule-dependent C. freundii invasion of HBMEC. Alternatively, an actin-dependent invasion step may precede a microtubule-dependent step in the C. freundii invasion of HBMEC. This initial step may result in microfilament reorganization when bacteria are initially in contact with the HBMEC; however these events may be transient, and the experimental design utilizing immunofluorescence microscopy may not adequately detect their occurrence. A similar situation is noted for Yersinia invasin-mediated invasion (36). Therefore, if the initial stages of invasion are prevented by cytochalasin D, the subsequent stages of invasion which are microtubule dependent are not triggered. It has previously been shown that actin functions in the translocation of actin-binding protein factors to the plasma membrane as well as in cytosolic signaling (19). In addition, cytochalasin D inhibits Salmonella entry via disruption of the translocation of actin-binding proteins to the bacterial entry site (7). It is possible that in the case of C. freundii invasion of HBMEC, actin microfilaments are necessary for cytosolic signaling and/or bacterial penetration at the plasma membrane, and microtubules may be necessary for the transportation of membrane-bound bacteria from the plasma membrane toward the basolateral side (or just deeper into the cell). Thus, a disruption at either stage of invasion would result in a "traffic jam."
In summary, the results presented here indicate that C. freundii can invade, multiply within, and transcytose HBMEC in vitro. Determining the genetic basis for these phenotypes will provide significant insight into the pathophysiology of Citrobacter meningitis and potentially aid in developing novel therapeutic and preventative strategies. Furthermore, an extensive molecular comparative analysis of Citrobacter with other meningitis-causing bacteria may shed light on Citrobacter's unique property of brain abscess formation.
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ACKNOWLEDGMENTS |
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We thank Carol A. Wass for excellent technical assistance, Hiroyuki Shimada for the TEM studies, Ernesto Barron at the USC School of Medicine Doheny Eye Institute for the confocal microscopy studies (EM Core grant EY03040), and Tobias Oelschlaeger and Joseph St. Geme III for providing Citrobacter strains.
This work was supported by Public Health Service grant NS 26310 to K.S.K. and CHLA Research Institute AIDS/Host Defense Program grant to J.L.B.
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FOOTNOTES |
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* Corresponding author. Mailing address: Division of Infectious Diseases, MS #51, Childrens Hospital Los Angeles, 4650 Sunset Blvd., Los Angeles, CA 90027. Phone: (323) 669-2509. Fax: (323) 660-2661. Email: kskim{at}chla.usc.edu.
Editor: E. I. Tuomanen
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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, August 1999, p. 4208-4215, Vol. 67, No. 8
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