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Previous Article | Next Article 
Infection and Immunity, April 2001, p. 2442-2447, Vol. 69, No. 4
Children's Hospital Oakland Research
Institute, Oakland, California 94609,1 and
Department of Medicine, Division of Infectious Diseases,
University of California at San Francisco School of Medicine, San
Francisco, California 941102
Received 6 November 2000/Returned for modification 14 December
2000/Accepted 18 January 2001
Microbial modulation of apoptosis has added a new dimension of
understanding to the dynamic interaction between the human host and its
microbial invaders. Persistent infection can be a by-product of
inhibition of apoptosis and may significantly impact the pathogenesis
of diseases caused by organisms such as Chlamydia trachomatis. We compared apoptotic responses among HeLa 229 cells acutely and persistently infected and mock infected with serovar A/HAR-13. Persistence was induced by gamma interferon at 0.2 and 2.0 ng/ml. Cells were treated with etoposide or staurosporine at 24-h
intervals and assayed for apoptosis by cell count, DNA ladder
formation, and cytochrome c translocation. From the 24- to
120-h time points, infected cultures were 87 and 90% viable for
etoposide and staurosporine treatment, respectively, and produced no
DNA ladder, and cytochrome c remained in the mitochondria. In contrast, mock-infected cells were 22 and 37% viable for etoposide (P = 0.0001) and staurosporine
(P = 0.01), respectively, and displayed characteristic DNA ladders, and cytochrome c was
translocated. We found that resistance to apoptotic stimuli was
identical in acute and persistent infections. Since cytochrome
c was not translocated from the mitochondrion, caspase-9
activity was likely not involved. The expression of chlamydial hsp60, a
known stimulator of inflammation in vivo, was measured in both active
and persistent infections by Western blot, with increased production in
the latter with or without staurosporine treatment. Chlamydial
disregulation of apoptosis and the ensuing persistence of organisms
offer an alternative pathogenic mechanism for chlamydial scarring
observed in trachoma and infertility populations via sustained
inflammation induced by immunoreactive molecules such as hsp60.
The recent findings that some
microbial pathogens modulate apoptosis to accommodate the organism's
life cycle and facilitate infection (34) shed an important
and exciting new light on the study of pathogenesis. Apoptosis, or
programmed cell death, is the mechanism for cellular self-destruction
that functions to eliminate cells during immune selection, tissue
development, and tissue regeneration (37). It is a
genetically programmed process in which macromolecules are broken down
and released from the cell in an orderly fashion designed to avoid
eliciting an inflammatory response. Apoptosis occurs in response to
specific internal and environmental stimuli (17).
Necrosis, in contrast, is generally the result of injury and is a rapid
process wherein the cell membrane ruptures, disgorging cell contents
into the system, inducing inflammation. Although apoptosis is designed
to dispose of cell contents with minimal disruption to neighboring
cells, it is possible that necrosis of bystander cells can occur
(23).
Chlamydia has joined the expanding list of pathogens that
modulate apoptosis by a diverse repertoire of methods (9, 10, 28,
30, 31), ranging from interactions with modulating proteins (22, 32) to coding for an inhibitor of inflammatory
molecules (35). Chlamydia spp. cause a myriad
of respiratory, ocular, and sexually transmitted diseases in humans
(6). The sequelae of these infections include trachoma,
the leading cause of preventable blindness in the world today
(7), and pelvic inflammatory disease (PID), a major cause
of infertility and ectopic pregnancy (4, 6). These
sequelae involve scarring that occurs at mucosal sites of inflammation.
Thus, although the pathogenesis of chlamydial diseases is not well
understood, host immune factors such as recurrent inflammation from
repeat infection (14) and hypersensitivity reactions to
chlamydial heat shock protein 60 (hsp60) (25) are thought
to be important. Pathogen-related factors most likely relate to the
fact that Chlamydia has the ability to persist (1, 2).
Chlamydia organisms are obligate intracellular parasites
with a distinct life cycle revolving between an inert, extracellular infectious stage, the elementary body, and an intracellular metabolic stage, the reticulate body. These stages are functionally distinct and
marked by specific protein profiles (27). Another distinct protein profile is seen when a persistent state is induced in vitro by
amino acid deprivation (5), antibiotic treatment
(2), or gamma interferon (IFN- Given the potential importance of persistence in the pathogenesis of
chlamydial diseases, we investigated the apoptotic response of human
epithelial cells to persistent infection with C. trachomatis serovar A. We used the in vitro immune factor model to induce persistence and tested the response to the cell death inducers staurosporine, a protein kinase C (PKC) inhibitor, and etoposide, an
inhibitor of topoisomerase II. We found a similar block in apoptosis to
that seen in acute infections described by Fan et al. (9).
During both active and persistent infection, hsp60 was continuously
expressed. In persistent infection, synthesis of most proteins was
decreased, enhancing the effect of hsp60 expression. This suggests that
an apoptotic block may enable colonization of the organism, while local
concentrations of immunoregulatory factors may favor a chlamydial form
that expresses an inflammation-inducing protein, such as hsp60. This
offers a possible mechanism for the immune injury seen in scarring
disease characteristic of trachoma and PID.
(This research was presented in part at the American Society of
Microbiology symposium "A Cell Biology Approach to Microbial Pathogenesis," Portland, Oreg., 25-28 April 1999.)
Establishment of C. trachomatis infections and
detection of chlamydial protein by microscopy.
Human cervical
adenocarcinoma cells (HeLa 229) were seeded at 106 cells
per ml onto coverslips in paired 12-well plates in minimal essential
medium with 10% fetal bovine serum (MEM-10). After 24 h of
incubation at 37°C in 5% CO2 with establishment of
confluent monolayers, the cells were washed three times with Hanks'
balanced salt solution, infected with C. trachomatis serovar
A/HAR-13 at a multiplicity of infection (MOI) of 50 in 0.4 ml of 0.25 M
sucrose-10 mM sodium phosphate-5 mM L-glutamic acid (pH
7.2), and incubated on a rocker for 2 h. The inoculum was removed
and replaced with MEM-10 containing cycloheximide (1 µg/ml) (Sigma,
St. Louis, Mo.). Coverslips were incubated at 24-h intervals, removed
from the well, fixed in methanol for 30 min at Establishment of persistent C. trachomatis infections
and detection of chlamydial proteins by immunoblot.
Confluent HeLa
229 cell cultures were infected with C. trachomatis as above
except without cycloheximide and treated with IFN- Apoptosis induction and Hoechst dye assay.
HeLa 229 cells
were seeded onto coverslips in 12-well plates, grown to 90%
confluence, and actively, persistently, or not infected as above except
for the omission of cycloheximide. Apoptosis was induced with 1 µM
staurosporine (Sigma) for 4 h or 300 µM etoposide (PharMingen,
San Diego, Calif.) for 6 h at 24-, 48-, 72-, 96-, and 120-h time
points postinfection. Adherent cells were assayed for all apoptosis
experiments. Coverslips for each time point were fixed in 4%
paraformaldehyde in PBS at ambient temperature, permeabilized with
0.25% saponin (Sigma) in PBS for 30 min, and stained with 10 µM
Hoechst 33258 dye (Sigma) for an additional 30 min at room temperature.
The coverslips were washed three times with PBS, mounted onto slides,
and viewed under a fluorescent microscope (Nikon Eclipse TE 300, Tokyo,
Japan) at 40× magnification, using an FITC filter. For each type of
infection, cells from five random fields were counted and divided by
the total number of cells to arrive at the percent apoptotic cells.
Cytochrome c detection.
Acutely infected,
persistently infected, and noninfected cells as described above were
harvested with trypsin at 48, 96, and 48 h, respectively, and
centrifuged at 800 rpm for 8 min at 4°C. The cytochrome c
assay was performed as per Fan et al. (9). Briefly, the
pellets were washed with ice-cold PBS, resuspended in up to 5 volumes
of buffer A (20 mM HEPES-KOH [pH 7.5], 10 mM MgCl2, 1 mM
sodium EDTA, 1 mM sodium EGTA, 1 mM dithiothreitol, 0.1 mM
phenymethylsulfonyl fluoride, 250 mM sucrose), and incubated for 15 min
at 4°C. Homogenization was performed using a 22 Kontes Douncer with
an average of 20 strokes prior to centrifugation at 750 × g for 10 min, which was repeated twice at 4°C. The supernatants were centrifuged at 10,000 × g for 15 min at 4°C to
generate the pellets containing the mitochondrial fraction. This
fraction was solubilized in buffer A and stored at DNA ladder assay.
Confluent HeLa cells were actively,
persistently, and noninfected as above but without cycloheximide and
treated with 1 µM staurosporine at 48 and 96 h postinfection for
4 h. A total of 2 × 106 cells were washed with
PBS after harvesting with trypsin and collected by centrifugation at
800 rpm for 10 min. The pellets were resuspended in 42°C lysis buffer
containing 5 mM EDTA, 5 mM Tris (pH 8.0), and 0.5% Triton. The lysates
were phenol-chloroform extracted and ethanol precipitated. The DNA was
resuspended in TE (5 mM Tris, 1 mM EDTA) with RNase for 30 min at
37°C, loaded onto a 2% agarose gel, and stained with ethidium bromide.
Statistical analyses.
Cell survival was calculated as the
percentage of cells surviving for each experiment. Because the
percentages were not normally distributed, percentages were transformed
using the arcsin of the square root of the percentage, which permitted
an analysis of variance on the data. In addition, a Tukey-Kramer
multiple-comparison analysis was performed to determine statistical
significance at a P value of < 0.05 between two pairs.
Effect of persistent chlamydial infection on apoptosis induction in
epithelial cells.
We used C. trachomatis strain A/HAR
at an MOI of 50 to establish active and persistent infections in HeLa
229 cells and found that apoptotic stimulation was blocked for adherent
cells treated with etoposide or straurisporine. Cell death was induced
by etoposide, which inhibits topoisomerase II and is active during S
phase. Cell death was also induced by staurosporine, a PKC inhibitor. Uninfected cells that were treated with low and high doses of IFN-
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.4.2442-2447.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Persistent Chlamydia trachomatis
Infections Resist Apoptotic Stimuli
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
) (1). In
the latter case, infected cells produce aberrant organisms that present
antigen but remain noninfectious until IFN- is removed.
Interestingly, the antigenic profile in persistent infections differs
from that of both the elementary and reticulate bodies. The overall
expression of all proteins decreases except for hsp60. A comparatively
high concentration of this molecule is maintained for the duration of
the persistent state (2). In a recent in vivo study, we
found that 24% of women with recurrent Chlamydia
trachomatis infections had the same ompA genotype
despite appropriate treatment (8). Intervening culture-negative episodes for these women were significantly more likely to be positive for chlamydiae by ligase chain reaction than for
women with recurrences due to different serovars or for women
undergoing test of cure.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
20°C, air dried, and
stained with fluorescein isothiocyanate (FITC)-conjugated anti-major
outer membrane protein (anti-MOMP) chlamydial antibody (Cortex Biochem, San Leandro, Calif.) for an additional 30 min at room temperature. The
coverslips were washed three times with phosphate-buffered saline (PBS)
and then mounted onto slides and viewed under a fluorescent microscope
(Nikon Eclipse TE300, Tokyo, Japan) at 40× magnification, using a FITC filter.
at 0, 0.2, or 2.0 ng/ml (Sigma) at 2 h postinfection to induce persistence as
described elsewhere (1). Uninfected HeLa cells were also
propagated. These experiments were performed with and without 1 µM
staurosporine at 24, 48, 72, 96, and 120 h postinfection as
described below except that control HeLa cells were not treated, as
this would induce apoptosis and negate the control effect of viable
cells. At 24, 48, 72, 96, and 120 h postinfection, cells were
harvested in 200 µl of Laemmli buffer (Bio-Rad, Richmond, Calif.),
boiled for 10 min, and sonicated briefly, and 40 µl of lysate was
loaded on a sodium dodecyl sulfate (SDS)-12.5% polyacrylamide gel
electrophoresis (PAGE) gel. After transfer, nitrocellulose (Bio-Rad)
was probed with a mouse anti-chlamydial hsp60 monoclonal antibody
(Affinity Bioreagents, Golden, Colo.) and a mouse anti-chlamydial MOMP
monoclonal antibody (Cortex, San Leandro, Calif.) and detected by an
anti-mouse immunoglobulin G (IgG)-alkaline phosphatase conjugate (Sigma, St. Louis, Mo.). A second set of experiments were performed as
described above except that at 96 h post-initial infection for the
persistent infections, the medium was removed from the cells and
replaced with MEM-10 without IFN-. The cells were allowed to grow
for an additional 24 and 48 h before harvesting in Laemmli buffer.
Western blot was performed as above.
70°C. The
supernatants were purified of mitochondria by centrifugation in an
ultracentrifuge at 100,000 × g for 1 h at 4°C.
The supernatants, now representing the cytosolic fraction, were stored
at 70°C. Aliquots were thawed on ice, and the proteins were
quantitated by the BCA assay (Pierce, Rockford, Ill.). Twenty-five
micrograms of protein from each fraction was loaded on a 15%
polyacrylamide gel. After PAGE, proteins were transferred by standard
procedure to nitrocellulose and probed with mouse monoclonal antibody
7H8.2C12 (IgG2b; PharMingen) specific for the denatured form of
cytochrome c. An anti-mouse IgG monoclonal antibody
conjugated with alkaline phosphatase (Sigma) was used for detection.
RESULTS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
showed the same sensitivity to apoptosis induction as uninfected, untreated HeLa cells. Although Chlamydia is routinely
cultured in the presence of cycloheximide, it was omitted during these assays to avoid the possible confounding effect of cycloheximide on
cell viability and the potential inhibitory effect on IFN-. An
indicator of apoptosis, membrane permeability to vital dyes such as
Hoechst and propidium iodide showed an average of 8% cell death for
persistently infected and treated cells, while apoptosis-induced uninfected cells were almost entirely permeable by 24 h (Fig. 1). Permeability data were expressed as a
percentage derived by observing slides microscopically and counting a
minimum of five 40× fields per slide for three different experiments.
For each 24-h interval from 24 to 120 h postinfection, infected
cultures were 87 and 90% viable for etoposide (not shown) and
staurosporine (shown) treatment, respectively, compared with
mock-infected cells, which were 22% (P = 0.0001) and
37% (P = 0.01) viable, respectively.
View larger version (12K):
[in a new window]
FIG. 1.
Persistent C. trachomatis infections allow
cells to resist apoptotic induction by staurosporine for up to 120 h. HeLa cells were actively, persistently, or not infected with
C. trachomatis serovar A/HAR-13 as described in the text. At
24-h intervals up to and including 120 h, the cells were treated
with 1 µM staurosporine for 4 h. DNA was detected using Hoechst
dye, and five random fields under 40× power were counted for apoptotic
cells to generate a percentage as described in the text. The graph
shows the averages of three independent experiments which varied by
~10% from each other. Series 1, uninfected, IFN- treated (2.0 µg) and not treated with staurosporine. Series 2, uninfected, IFN-
(2.0 µg), and staurosporine treated. Series 3, persistently infected
with serovar A/HAR-13 induced with 2.0 µg of IFN- (IFN- removed
at 72 h) and not treated. Series 4, persistently infected and
staurosporine treated, with IFN- removed at 72 h. Series 5, persistently infected and not treated. Series 6, persistently infected
and staurosporine treated. Of note is that the results for persistent
infections induced with 0.2 µg of IFN- were similar to series 3 and 4 and therefore are not shown.
-and
staurosporine-treated (lane 7) HeLa cells, as demonstrated by SDS-PAGE
(Fig. 2). Similar results were obtained for the experiments where
etoposide was used to induce apoptosis (data not shown).
|
Lack of cytochrome c relocation to the cytoplasm in
response to apoptosis induction of actively and persistently infected
cells.
In order to compare the possible mechanisms of the
apoptotic block between active and persistent infections, we determined that cytochrome c was not translocated from the
mitochondrion in either type of infection (Fig.
3). In uninfected cells, cytochrome c appeared in the cytoplasm after treatment with
staurosporine. Western blot analysis demonstrated that in active (up to
48 h) and persistent (up to 120 h) chlamydial infection of
HeLa cells, cytochrome c remained sequestered in the
mitochondrial fraction after apoptotic induction (Fig. 3). Uninfected
HeLa controls that were treated with staurosporine showed translocation
of cytochrome c from the mitochondria. Presumably, caspases
were involved, although we did not assay for procyclic acidic
repetitive protein (PARP) cleavage.
|
Cultures actively infected with C. trachomatis become
sensitive to apoptotic stimuli, whereas persistently infected cells
continue to resist apoptotic induction.
During the time course of
an active or persistent infection, permeability remained intact and DNA
was not fragmented in response to apoptotic induction. The
characteristic DNA ladder produced by nuclease activity was not seen
during the course of the infection. However, starting at 48 h and
at longer time points, actively infected cells underwent apoptosis with
loss of protection followed by permeability (Fig. 1) and DNA
fragmentation (data not shown). Persistent infections that were
maintained up to 120 h continued to resist DNA fragmentation upon
staurosporine treatment. However, within 24 to 48 h of washing
cells and removing IFN-, an active infection resumed, as evidenced
by resumption of expression of both hsp60 and MOMP (Fig.
4). These infections ultimately lysed the
host cells, which died by apoptotic mechanisms, as evidenced by cell
count (Fig. 1) and DNA ladder formation (data not shown).
|
Expression of C. trachomatis proteins during active and
persistent infection.
Both MOMP and hsp60 were expressed during
active infection, but almost undetectable amounts of MOMP were
expressed during persistent infections at the same time point of 48 h
(Fig. 4). At 96 h postinfection, hsp60 continued to be expressed
for persistent infections induced by either 0.2 or 2.0 ng of IFN-.
Treatment with staurosporine had no effect on protein expression.
Uninfected control HeLa cells were not treated with staurosporine, as
this would have instituted cell death, with no cells for remaining time
points. Similar results were obtained in the same experiments when
staurosporine was omitted (data not shown). Forty-eight hours after
removal of IFN-, there was resumption of near-normal MOMP expression
for the persistent infections that had been treated with 0.2 ng but not
2.0 ng of IFN-.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
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Chlamydia successfully evades host defense mechanisms,
including apoptosis, by growing within an inaccessible cellular
compartment, the inclusion body, derived from components in the
exocytic pathway (15). The organism appears to confer
resistance to apoptosis upon actively infected cells, which prolongs
the life of the infected cell, allowing the organism to complete its
complex intracellular life cycle within 48 to 72 h. In vitro data
suggest that host cytokines cooperatively induce and prolong apoptotic
resistance by allowing Chlamydia to persist in tissue. In
this study, a persistent infection was established with concentrations
as low as 0.2 ng of IFN-, which is in the physiologic range seen in
tissue. Thus, although the initial host response of inflammatory
molecules, including interferons, occurs to eradicate infection, it may
also contribute to initiation of a persistent chlamydial infection. The
duration of persistence in vivo is not known, but recent evidence suggests that organisms may persist for as long as 5 years in the
genital tract (8); in vitro persistence has been
documented for up to 1 year (2).
In order to compare the possible mechanisms of the apoptotic block between active and persistent infections, we determined that cytochrome c was not translocated from the mitochondrion in either type of infection. This is a critical upstream event in caspase activation, which occurs early in apoptosis. In uninfected cells, cytochrome c has been shown to appear in the cytoplasm as early as 1 h following treatment with staurosporine (38). Release into the cytoplasm allows cytochrome c to bind Apaf-1 and, in the presense of ATP, cleaves procaspase-9 to the active caspase-9. Caspase-9 in turn activates caspase-3 and continues the cascade toward dismantling the cell (21). We found that in active and persistent chlamydial infections, cytochrome c remained sequestered in the mitochondrial fraction after apoptotic induction. However, noninfected, treated cells showed translocation of cytochrome c from the mitochondria. Persistently infected cells also resisted two different modes of apoptotic induction (etoposide and staurosporine), suggesting that the block occurred at a common point upstream of varied mechanisms for implementing programmed cell death. Presumably caspases are involved, although we did not assay for PARP cleavage.
It has been suggested that cytochrome c depletion from the mitochondrion may also be an indicator of necrotic cell death, since it results in a dismantling of the electron transport chain (ETC) (36). However, this did not appear to be a factor in the control cells, since necrosis derived from ETC degradation occurs in a very delayed manner, as long as 24 h post-apoptotic induction (23). For both the permeability (Hoechst dye) and DNA fragmentation experiments, samples were treated for 4 h with staurosporine at 24-h intervals and then immediately assayed. Thus, these data do not support necrosis as a mechanism for the demise of uninfected control cells.
Our findings are similar to those of others who have investigated antiapoptotic events in vitro in C. trachomatis-infected human cell lines (9, 30). Inhibition of apoptosis has also been described for Chlamydia pneumoniae, whereby one of the mechanisms appeared to involve induction of interleukin-10 (10). In contrast (9, 30), infection with the mouse pneumonitis strain (MoPn) of C. trachomatis induced apoptosis. Furthermore, induction of tumor necrosis factor alpha appeared to precipitate additional programmed death of surrounding cells. Chlamydia psittaci has been reported to induce cell death in infected and bystander macrophages and epithelial cells by a mechanism that is independent of known caspases (11, 28). These conflicting data may reflect the fact that human C. trachomatis strains, MoPn, and C. psittaci represent vastly different subtypes and species, with unique host and tissue tropisms. Alternatively, it is possible that C. trachomatis both induces apoptosis and protects infected cells from programmed cell death. These dual properties have been reported for other microorganisms, such as adenovirus (34). Additional research will be required to fully understand the properties that can be attributed to human C. trachomatis strains.
The ability to establish a persistent infection is an important step in
the pathogenesis of scarring disease seen in both trachoma and
chlamydial sexually transmitted diseases. A recent in vitro model
showed that macrophages infected with C. trachomatis serovar
K induced apoptosis of uninfected T cells, which supports the notion
that chlamydia-infected macrophages may persist by avoiding T-cell
surveillance via reduction of their overall numbers (20).
Resistance to cell death induced by these infections may also allow a
continuous antigenic pool that may stimulate ongoing inflammation and
subsequent fibrosis. Persistent chlamydial organisms are noninfectious
and exhibit a protein profile that is completely different from that
seen in active infection, where the predominant antigen expressed is
the MOMP (26), the most abundant and immunogenic protein
of the organism. We found that in persistent infections, hsp60 was
expressed in greater abundance than MOMP, which is consistent with the
findings of others (1). Treatment with staurosporine did
not affect expression of either hsp60 or MOMP. After withdrawal of
IFN- from persistently infected cells, active infection resumed, with expression of MOMP and hsp60. However, we were not able to recover
active infection when cells had been treated with 2.0 ng of IFN-.
Hypersensitivity reactions are known to be elicited by chlamydial hsp60 (24, 25, 29), which is produced throughout the life cycle of the organism (1). Since it has long been known that host factors are important in disease progression, the protein profile shift offers an explanation for how this response is induced. Persistently infected cells, by blocking apoptosis, ensure indefinite survival of the bacteria while expressing their most inflammatory antigen. Reversion to active infection would result in a fully infectious organism that may spread through tissue and precipitate disease both during active infection and on resumption of a persistent state. Since hsp60 is the most abundant protein expressed during both types of infections and parallels the resistance to apoptotic stimuli, it is possible that hsp60 may play a role in the inability of infected cells to undergo apoptosis. Chlamydiae are known to have a type III secretory apparatus (19, 33), which may facilitate transport of molecules such as hsp60 to the host cytoplasm. This would provide the opportunity for hsp60 to interact with cellular molecules such as procaspase-9 to prevent activation and thereby interrupt apoptosis. This mechanism has been described for mammalian heat shock proteins (3). If this is the case, it could account for one mechanism for how chlamydiae establish a persistent infection.
Another mechanism is suggested from apoptotic regulation, which occurs at the protein level by the formation of hetero- and homodimers among members of the Bcl-2 family of proteins. This family consists of antagonistic members that inhibit or induce apoptosis, depending upon the ratio of proapoptotic to antiapoptotic proteins within the cell following a stimulus. These proteins have regions of homology that are conserved in mammals from humans to nematodes, and homologues have been identified in viral pathogens (17, 18). With the addition of homologous viral proteins, the cellular protein balance can be shifted. An interesting example is provided by adenovirus, in which the E1A and E1B loci code for proteins that are pro- and antiapoptotic, respectively, serving the purpose of prolonging cell survival to allow replication and then inducing apoptosis to facilitate virion release and spread to other cells (34). The E1B 19-kDa protein blocks apoptosis by binding to the cellular apoptosis-inducing protein Bax and titrating out its effect (16). However, overexpression of E1B enhances survival of adenovirus-infected human but not mouse cells (12, 13). These data suggest that it is the overall protein environment of the cell that finally determines whether a protein or organism will provide an apoptotic stimulus or not.
Although C. trachomatis has been shown to modulate apoptosis, no proteins with homology to Bcl-2 have been identified, and this mechanism has not been explored. However, it is intriguing that overexpression of Bcl-2 has been shown to block the translocation of cytochrome c from the mitochondrion after apoptotic induction, whereas other apoptotic inhibitors such as caspase had no effect (38). This suggests that a Bcl-2 homologue or a nonhomologous protein that can interact with the mitochondrial membrane in a similar fashion may be involved. Bcl-2 is thought to stabilize the mitochondrial membrane, where it is located in the outer membrane, preventing the release of cytochrome c from the intermembrane space, where it is localized. It is interesting that exogenous cytochrome c added to the cytosol can mitigate the effect of Bcl-2 apoptotic inhibition and induce caspase activation (21). Bcl-2 may play additional roles in mitochondrial function as well. Further research will be required to determine whether C. trachomatis produces a homologue or nonhomologue protein with similar activity and whether hsp60 can be functionally described as an antiapoptotic protein.
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ACKNOWLEDGMENTS |
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We thank Amy Helmer and Shanya Becha for excellent technical assistance.
This research was supported by Public Health Service grant R01 AI39499 (to D.D.) from the National Institutes of Health.
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FOOTNOTES |
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* Corresponding author. Mailing address: Children's Hospital Oakland Research Institute, 5700 Martin Luther King Jr. Way, Oakland, CA 94609. Phone: (510) 450-7655. Fax: (510) 450-7910. E-mail: ddean{at}chori.org.
Editor: R. N. Moore
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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