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Infect Immun, January 1998, p. 336-342, Vol. 66, No. 1
Department of Microbiology, Molecular Biology
and Biochemistry, University of Idaho, Moscow, Idaho
83844,1 and
Department of Veterinary
Clinical Medicine and Surgery, Washington State University, Pullman,
Washington 991642
Received 20 August 1997/Returned for modification 3 October
1997/Accepted 21 October 1997
We examined the invasion of an established bovine mammary
epithelial cell line (MAC-T) by a Staphylococcus aureus
mastitis isolate to study the potential role of intracellular survival in the persistence of staphylococcal infections. S. aureus
cells displayed dose-dependent invasion of MAC-T cells and
intracellular survival. An electron microscopic examination of infected
cells indicated that the bacteria induced internalization via a
mechanism involving membrane pseudopod formation and then escaped into
the cytoplasm following lysis of the endosomal membrane. Two hours after the internalization of S. aureus, MAC-T cells
exhibited detachment from the matrix, rounding, a mottled cell
membrane, and vacuolization of the cytoplasm, all of which are
indicative of cells undergoing programmed cell death (apoptosis). By
18 h, the majority of the MAC-T cell population exhibited an
apoptotic morphology. Other evidence for apoptosis was the generation
of MAC-T cell DNA fragments differing in size by increments of
approximately 180 bp and terminal deoxynucleotidyl transferase-mediated
dUTP nick end labeling of the fragmented nuclear DNA of the infected host cells. These results demonstrate that after internalization S. aureus escapes the endosome and induces apoptosis in
nonprofessional phagocytes.
Staphylococcus aureus is
a pathogen with a broad host range and is a leading cause of infections
in humans and domesticated animals worldwide. The rapidly increasing
frequency of methicillin-resistant isolates and the looming threat of
resistance to vancomycin by this organism have recently caused
considerable alarm within the medical community. Infections associated
with this organism are extremely common and often life threatening;
therefore, there is serious potential for S. aureus to cause
increased morbidity and mortality. S. aureus is also the
leading cause of intramammary infection in ruminants, which is the most
economically important disease to the dairy industry in the United
States, with approximately one-half of dairy cows afflicted with some
form of mastitis. This disease accounts for approximately 70% of the
total expenses for dairy farmers (14) and results in the
loss of billions of dollars each year (3). Thus, a thorough
understanding of the pathogenesis of staphylococcal disease could have
a profound impact on public health and agriculture in the United States
and worldwide.
The mechanism of persistence of staphylococci in its hosts, despite the
induction of seemingly sufficient levels of humoral and mucosal
antibodies, remains unexplained. This is an important issue for both
humans and animals, which can have repeated occurrences of
staphylococcal infections and toxigenic diseases such as toxic shock
syndrome (7). While there is some evidence that
immunosuppression induced by superantigens is partially responsible for
both the persistence of infection and reduced antibody levels against
some staphylococcal products, not all human and animal cases are
attributed to superantigen-producing organisms. For example, less than
half of bovine mastitis staphylococcal isolates produce known
superantigen exotoxins (26).
One confirmed mechanism employed by some bacteria to evade humoral
immunity is to become internalized in host cells. For example, organisms such as Listeria monocytogenes and
Mycobacterium tuberculosis are facultative intracellular
pathogens that require cell-mediated immunity to be eliminated most
efficiently; the presence of antibodies alone is ineffective during
infection by these pathogens. S. aureus is generally not
considered to be an intracellular pathogen of the magnitude associated
with classical facultative intracellular pathogens (i.e.,
Listeria, Mycobacterium, Salmonella,
and Shigella spp.). However, it is well documented that
S. aureus can be internalized in epithelial cells
(1) and endothelial cells (18, 37). Little is
known regarding the mechanisms involved in internalization, the
potential role of internalization of S. aureus by the host cell, or host cell responses.
The objective of this study was to investigate the invasion of mammary
epithelial cells by a strain of S. aureus known to cause
bovine mastitis. We now report that S. aureus cells
successfully invade epithelial cells, exist free in the cytoplasm after
effecting release from the endosome, and induce the host cells to
undergo apoptosis.
Bacterial strains and growth conditions.
S. aureus
Novel (36) was isolated from cows with clinical mastitis and
used throughout this study. Prior to each experiment, a single colony
from a Todd-Hewitt (TH) (Difco Laboratories, Detroit, Mich.) agar plate
was inoculated into 4 ml of TH broth and grown at 37°C with vigorous
shaking for 6 to 8 h. From this 4-ml culture, 100 µl was
transferred into 10 ml of TH broth and incubated overnight (16 h) at
37°C with vigorous shaking. The overnight culture was centrifuged,
and the pellet was washed once with sterile phosphate-buffered saline
(pH 7.2) and resuspended in 10 ml of invasion medium (see below) to
give a cell density of 1010 CFU/ml.
Cell culture.
An established bovine mammary epithelial cell
line, designated MAC-T (21), was used for all experiments.
The MAC-T cell growth medium was Dulbecco's modified Eagle medium
(Gibco BRL, Grand Island, N.Y.) containing 10% heat-inactivated fetal
bovine serum (HyClone, Logan, Utah), 5 µg of insulin/ml, 1 µg of
hydrocortisone/ml, 44 mM NaHCO3 (Sigma, St. Louis, Mo.),
100 U of penicillin G/ml and 100 µg of streptomycin sulfate (Gibco
BRL)/ml. Prior to use, cells were seeded at 6 × 104
cells/well and grown for 3 days at 37°C with 7% CO2.
Cells were grown in 24-well tissue culture plates (Costar, Cambridge,
Mass.) for invasion assays or 24-well tissue culture plates with 13-mm round Thermanox coverslip inserts (Nalge Nunc International;
Naperville, Ill.) for electron microscopy. Lab-Tek four-chambered glass
slides (Nalge Nunc International) were used for confocal microscopy.
Invasion assay.
Approximately 16 h prior to invasion
experiments, the MAC-T cell growth medium was replaced with 1 ml of
invasion medium (growth medium without antibiotics or fetal bovine
serum). The morning of the experiment, the medium was removed and MAC-T
cells were washed once with invasion medium and given 1 ml of fresh
invasion medium. Appropriate wells of MAC-T cells were then inoculated with 107 CFU of washed S. aureus and incubated
at 37°C with 7% CO2. After 2 h, supernatants of the
cocultures were removed and replaced with 1 ml of invasion medium
containing 100 µg of gentamicin (Sigma) per ml. After the incubation
of cocultures at 37°C with 7% CO2 had continued for the
specified times, the supernatants were removed and discarded. MAC-T
cell monolayers were washed three times with sterile phosphate-buffered
saline, treated with 0.25% trypsin in Hanks balanced salt solution
(Gibco BRL), and further lysed with 0.025% Triton X-100 (United States
Biochemicals, Cleveland, Ohio) in sterile distilled water. Cell lysates
were serially diluted 10-fold and plated in triplicate on TH agar
plates; the plates were incubated overnight at 37°C, and CFU were
counted. To test the inhibition of S. aureus invasion by
cytochalasin D, experiments were carried out as described for the
invasion assays except that prior to inoculation with bacteria, MAC-T
cell monolayers were incubated at 37°C with 7% CO2 for
2 h with invasion medium containing 0.5 µg of cytochalasin D
(Sigma) per ml.
Assessment of apoptosis.
The occurrence of apoptosis in
MAC-T cells was evaluated by three different methods: (i) DNA
laddering, (ii) a terminal deoxynucleotidyl transferase-mediated dUTP
nick end labeling (TUNEL) assay (12, 17, 33, 38), and (iii)
microscopic observation of morphological changes in the cells.
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Intracellular Staphylococcus aureus
Escapes the Endosome and Induces Apoptosis in Epithelial
Cells
ABSTRACT
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
20°C in 1/10
volume of 3 M sodium acetate (pH 5.1) and 2 volumes of 100% ethanol.
DNA was collected by centrifugation, and the pellet was washed once
with 70% ethanol, dried, resuspended in sterile water, and treated
with 20 µg of DNase-free RNase A (Sigma) per ml for 30 min at 37°C.
DNA samples were separated by electrophoresis at 5 V/cm in 1.8%
agarose, stained with ethidium bromide, visualized with UV light, and
photographed. DNA fragments were sized by comparison with a 100-bp DNA
ladder (Gibco BRL).
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RESULTS |
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Abstract
Introduction
Materials & Methods
Results
Discussion
References
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S. aureus invasion of MAC-T cells. To study the internalization of S. aureus in more detail, we examined the ability of a highly transmissible S. aureus bovine mastitis isolate, designated Novel (36), to invade a well-established bovine mammary epithelial MAC-T cell line (21). The invasion assay employed is based on the principle that bacteria inside host cells are protected from the antimicrobial effects of gentamicin added to the medium (22). The Novel strain of S. aureus invaded the MAC-T cells in a dose-dependent fashion (Fig. 1). A linear increase in the number of surviving bacteria was observed up to a multiplicity of infection (MOI) of 53. Above this dose, substantial increases in bacterial survival were not observed, indicating that saturation of the internalization mechanism had occurred. We confirmed the results of other investigators working with different systems (1, 18) by demonstrating that treatment with 0.5 µg of cytochalasin D per ml reduced the survival of S. aureus approximately 10-fold (Fig. 1).
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Cellular effects of invasion. Several time course experiments were performed to evaluate the morphological events that were induced by the presence of intracellular S. aureus. MAC-T monolayers were infected with 107 bacteria (MOI = 34) prior to killing the extracellular bacteria with gentamicin. The number of intracellular bacteria increased continuously for 2 h, after which time the numbers began to decline gradually (data not shown). We attributed the initial increase in numbers to staphylococcal replication following the addition of gentamicin. Although many MAC-T cells were observed to contain large numbers of viable and dividing staphylococci for at least 3 days following the addition of S. aureus, an accurate assessment of the extent of intracellular replication was not possible, and numbers of viable bacteria eventually declined (data not shown).
As shown in Fig. 2, a dramatic difference in the morphology of MAC-T cells between infected and uninfected cells was observed. Some infected cells detached from the plates within 2 h after staphylococci were added to the monolayers. Detachment from the substrate was accompanied by an overall rounding of the cells and a mottled appearance of the cell membrane (Fig. 2C and D), morphological changes consistent with apoptosis. By 18 h of incubation with gentamicin, the majority of the MAC-T cells (typically at least 80% of the population) were apoptotic. This correlated with the high percentage of infection, which was also estimated to be approximately 80%. The uninfected cells (to which gentamicin, but not S. aureus, had been added) maintained normal adherence and cellular morphology (Fig. 2A and B). An examination of electron micrographs of the infected cells (Fig. 3) also revealed several additional features of S. aureus invasion at the ultrastructural level. Bacteria that were in close contact with the MAC-T cell surface were associated with pseudopod-like structures (Fig. 3A and C); these structures were presumably involved in engulfing the bacteria, leading to the formation of membrane-bound endosomes. The membrane was clearly evident surrounding the bacteria in endosomes that had recently entered the cell (Fig. 3A and C). However, vacuoles farther from the cytoplasmic membrane of the host cell, presumably those internalized for longer periods of time, began to degrade. Some bacteria were observed to be partially surrounded by vacuolar fragments, while others were entirely free in the cytoplasm (Fig. 3A and B). Another interesting feature was the cytoplasmic membrane contortions that were associated with many of the infected cells (Fig. 3D). These contortions are also characteristic of apoptosis (35).
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Infection by S. aureus induces apoptosis. As described above, the morphological features of the infected MAC-T cells (Fig. 2 and 3) were reminiscent of those of cells undergoing apoptosis (27, 29). One hallmark of apoptotic cells is the fragmentation of the DNA by specific endonucleases (29, 32, 39). This phenomenon can be visualized as a characteristic ladder pattern where the size of each band increases by approximately 180 bp. As shown in Fig. 4, laddering of the DNA occurred in S. aureus-infected MAC-T cells (Fig. 4, lane B) but not in uninfected MAC-T control cells also treated with gentamicin (Fig. 4, lane A). In some experiments, samples of the growth media containing detached, rounded cells were collected separately from the remaining attached MAC-T cells and lysed and the DNA was visualized on agarose gels for fragmentation. DNA fragmentation laddering was observed predominately in samples from growth media containing detached cells (data not shown). This would be expected since it is characteristic of apoptotic cells to be released from the culture substrate into the growth medium (35). Additionally, some S. aureus-infected MAC-T cells were observed to exhibit an intense green positive fluorescence by using the TUNEL method (Fig. 5D), which is based on the specific staining of the 3' hydroxyl ends of the fragmented DNA within apoptotic cells (12, 17, 33, 38). Figures 5A and C show uninfected and infected cells, respectively, visualized by red propidium iodide fluorescence. Panels B and D show the same fields as panels A and C, respectively, visualized by green fluorescein fluorescence. Apoptotic cells are visualized as intensely green fluorescent cells, easily recognized above background levels (Fig. 5D).
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DISCUSSION |
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Abstract
Introduction
Materials & Methods
Results
Discussion
References
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While S. aureus has not traditionally been considered an intracellular pathogen, previous studies have revealed that S. aureus cells may be actively internalized by phagocytosis and are capable of intracellular survival (1, 18, 37). In characterizing S. aureus invasion further, we have observed that many of the internalization events are consistent with the cellular events that are induced by other well-established facultative intracellular pathogens (13). First, electron photomicrographs show that S. aureus cells interact or bind with the cell surface of the MAC-T host cell and induce membrane pseudopod formation. Which S. aureus adhesion factor(s) is responsible for the signal transduction initiating pseudopod formation and endocytosis is currently unknown. However, one or more of the group of specific cell surface proteins, collectively termed MSCRAMMs (for microbial surface components recognizing adhesive matrix molecules) (31) could be involved. Second, although the S. aureus cells were observed to be internalized initially within a membrane-bound endosome, the S. aureus cells eventually came to reside directly in the host cytoplasm, in this respect mimicking Rickettsia, Shigella, and Listeria cells.
It is noteworthy that not all intracellular parasites escape from the vacuole; Coxiella burnetii, for example, has evolved to thrive in the phagolysosome, while Salmonella, Mycobacterium, and Legionella spp. inhibit phagolysosomal fusion (15). Thus, it is of interest to establish the fate of S. aureus once it is within a host cell. The studies of Almeida et al. (1), who examined the invasion of S. aureus into primary and established bovine mammary epithelial cell lines, showed that the bacteria were localized in membrane-bound vacuoles. This apparent conflict with our observations might be explained as follows. First, it is possible that infected cells that were analyzed by TEM in their study were harvested at too early a time point to observe lysis of the endosomal membrane and access to the cytoplasm. Second, it has been shown that only a small fraction of internalized L. monocytogenes cells escape from the vacuoles (15). A similarly small fraction of S. aureus cells might escape from the vacuoles, making them difficult to locate. Regardless of this apparent conflict, our results are in agreement with those of Hudson et al. (20), who demonstrated that S. aureus cells were able to invade and appeared free in the cytoplasm of cultured chick osteoblast cells. Furthermore, our data are also consistent with the assumption of Proctor et al. (34) that intracellular S. aureus cells must reside in the host cell cytoplasm since this compartment would provide the biochemical environment that allows the survival of small-colony variants during persistent, recurring staphylococcal infections.
Since S. aureus was seen to escape from vacuoles in MAC-T cells, it becomes important to ask how this was achieved. Listeria and Shigella cells produce specific hemolysins (listeriolysin O and IpaB, respectively) that enzymatically degrade the endosomal membrane (15). The role of listeriolysin was elegantly demonstrated by expressing this hemolysin in the nonpathogenic species Bacillus subtilis, which allowed these bacteria to survive and replicate in the cytoplasm of phagocytic cells (2). We hypothesize that the release of S. aureus from the vacuole is mediated by one (or more) of at least four different staphylococcal hemolysins known to damage membranes (alpha-, beta-, gamma-, and delta-toxins) (4). Experiments are under way to test this hypothesis.
The ability of S. aureus to survive intracellularly could explain several aspects of host-pathogen relationships as they pertain to chronic recurrent staphylococcal diseases and long-term colonization. Internalization may be an important component of mastitis and other staphylococcal diseases, perhaps by providing protection against host defenses and antibiotic treatment. In fact, Craven and Anderson (8) demonstrated intracellular S. aureus in experimental mastitis in mice. As a species, S. aureus comprises a heterogeneous group of strains, each with the potential to elaborate its own set of virulence factors. Because of this diversity, many types of infectious diseases are associated with this organism. Although diseases such as toxic shock syndrome require the expression of immunomodulating superantigen exotoxins, the effect of the toxins must be preceded by colonization on mucosal surfaces. The most common types of staphylococcal diseases are pyogenic infections that are often a direct result of long-term colonization of the host by an endogenous organism. Furthermore, many types of staphylococcal infections that tend to become chronic, such as osteomyelitis and mastitis, are associated with multiple recurrences and do not resolve even in the presence of a seemingly adequate humoral immune response. Our results suggest that the chronic nature of S. aureus disease and/or its long-term persistence may be dependent on the ability of S. aureus to survive within host cells.
A further important finding of this study was that internalized S. aureus cells induced the bovine epithelial host cells to become apoptotic. Interestingly, the ability of Shigella flexneri to induce apoptosis in macrophages, T cells, and B cells has been shown (42). Invasion and cell killing were inhibited by cytochalasin D, indicating that the bacteria must be within the cell to induce apoptosis (41). It has been shown that the induction of apoptosis by ingested S. flexneri cells is mediated by the binding of IpaB invasin to interleukin-1-converting enzyme, which promotes apoptosis in macrophages (5). Although no IpaB-like invasin has been identified for S. aureus, it is important to note that in primary lymphocyte cultures, purified staphylococcal alpha-toxin and superantigens can induce apoptosis (24, 25). However, it is unlikely that a similar type of induction mechanism, mediated from the outside of the MAC-T cells, played a significant role in causing apoptosis in our cell cultures for several reasons. First, the S. aureus cells were carefully washed to remove extracellular proteins before infecting the MAC-T cells and the MAC-T cells were carefully washed after being infected with S. aureus. Second, the length of time that the MAC-T cells were exposed to viable staphylococcal prior to the addition of gentamicin was very short. Most secreted proteins are regulated by the products of the agr global transcriptional regulatory locus and are expressed late in the growth cycle (28). Finally, observations using microscopy revealed that following infection with S. aureus, MAC-T cells exhibiting normal (nonapoptotic) morphology were observed in the presence of apoptotic MAC-T cells at every time point; the presence of extracellular inducers of apoptosis would be expected to be able to affect all cells similarly.
An alternative hypothesis involves recent evidence implicating the sphingomyelin cycle as a key component in the induction of apoptosis (19). It has been demonstrated that certain extracellular agents that lead to apoptosis, such as tumor necrosis factor alpha, activate endogenous sphingomyelinase activity (10), cleaving membrane sphingomyelin to yield cellular ceramide. Evidence implicating ceramide as a mediator of apoptosis was reported by Jarvis et al. (23), who showed that apoptosis was induced in human leukemia and murine fibrosarcoma cell lines after the addition of exogenous sphingomyelinase or synthetic ceramide. Thus, the production of beta-toxin, a known sphingomyelinase (9, 11), by intracellular S. aureus cells could result in an increased level of ceramide, leading to the induction of apoptosis in the bovine mammary epithelial cells. It should be noted that we have demonstrated that beta-toxin is produced by S. aureus Novel (data not shown). Furthermore, other beta-toxin-producing S. aureus strains, including standard laboratory strains 8325-4 and RN6390, also invade MAC-T cells and induce apoptosis (data not shown). Interestingly, beta-toxin has been shown to be an important virulence factor for infection by using a mouse model for staphylococcal mastitis (16).
Does the ability of bacteria to induce apoptosis imply that there is some benefit to the bacteria? In some cases, as when S. flexneri cells are internalized and induce the death of macrophages by apoptosis (6), one can speculate that the induction of apoptosis in leukocytes is a mechanism for suppressing the immune response. Alternatively, the biological consequences of apoptosis were hypothesized to be the release of interleukin-1 prior to cell death (40), which in turn initiates an acute inflammatory response characteristic of bacillary dysentery. The ability of S. aureus to induce apoptosis in cultured bovine mammary epithelial cells also has profound implications for the possible role of programmed cell death during the pathogenesis of bovine mastitis. One hypothesis is that the induction of apoptosis produces a vehicle by which the bacteria could enter macrophages without stimulating bactericidal activities, while simultaneously being provided with a protective barrier against exogenous host immune defenses and/or antibiotics. This is supported by the observation that phagocytes isolated from infected udders often contain viable S. aureus cells (8). We are currently investigating this possibility.
This report demonstrates that S. aureus becomes intracellular following contact with the cell surfaces of bovine mammary epithelial cells, escapes the endosome to reside and possibly multiply in the host cell cytoplasm, and induces the host cell to become apoptotic. The observation that intracellular S. aureus induces programmed cell death in epithelial cells, orchestrating normal host cell processes for its own advantage, suggests that S. aureus might be a more versatile and adaptive pathogen than previously believed.
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ACKNOWLEDGMENTS |
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We thank Raquel Brown and Chris Davitt for the electron microscopic examination of S. aureus invasion, Ann Norton for technical support with the confocal microscopy, and Katarzyna Dziewanowska for her characterization of S. aureus Novel.
This work was funded in part by NIH grant no. R29-AI38901 (K.W.B.), NRICGP USDA grant no. 9402399 (G.A.B.), Public Health Service grant no. AI28401 (G.A.B.), the United Dairymen of Idaho (G.A.B.), and an Organization for Economic Co-operation and Development sabbatical fellowship (W.R.T.).
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Microbiology, Molecular Biology and Biochemistry, College of Agriculture, University of Idaho, Moscow, ID 83844-3052. Phone: (208) 885-8977. Fax: (208) 885-6518. E-mail: btrumble{at}uidaho.edu.
Editor: V. A. Fischetti
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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