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Previous Article | Next Article 
Infection and Immunity, September 1999, p. 4463-4468, Vol. 67, No. 9
Laboratory of Microbial Structure and
Function, Rocky Mountain Laboratories, National Institute of Allergy
and Infectious Diseases, National Institutes of Health, Hamilton,
Montana 59840
Received 29 March 1999/Returned for modification 18 May
1999/Accepted 14 June 1999
Fundamental to the virulence of microbial pathogens is their
capacity for adaptation and survival within variable, and often hostile, environments encountered in the host. We describe a novel, extragenomic mechanism of surface modulation which may amplify the
adaptive and pathogenic potential of numerous bacterial species, including Staphylococcus, Yersinia, and
pathogenic Neisseria species, as well as Helicobacter
pylori and Streptococcus pyogenes. The mechanism
involves specific bacterial recruitment of heparin, glycosaminoglycans,
or related sulfated polysaccharides, which in turn serve as universal
binding sites for a diverse array of mammalian heparin binding
proteins, including adhesive glycoproteins (vitronectin and
fibronectin), inflammatory (MCP-3, PF-4, and MIP-1 Infectious diseases typically
involve continuous interplay between microbial pathogenicity factors
and host defense systems. Commonly identified bacterial strategies for
surviving within the host include exploiting host cell receptors for
colonization of mucosal surfaces and tissue invasion, the production of
(cyto)toxins and proteases that undermine the host defense, and
phenotypic variation intended to evade the immune system. In
otherwise-healthy individuals, microbial pathogenic behavior is
classically considered to be an intrinsic property of the
microorganism, with individual sets of genes providing the necessary
tools to direct key events in the infectious process. This concept
however, is increasingly challenged by the recognition that host
factors may significantly contribute to the intrinsic virulence
capabilities of microbial pathogens. It has been demonstrated that
bacteria can utilize host matrix constituents, such as fibronectin and
vitronectin, to facilitate interactions with mammalian cells
(9-12, 15, 17, 23, 28, 38, 40) or use soluble molecules,
such as host-derived complement factor H and sialic acid precursors, to
protect against being killed by the immune system (29, 34).
These observations suggest that by synthesizing specific surface
antigens, microbial pathogens can increase their virulence potential by
interacting with relevant host molecules.
Recently, we discovered a novel mechanism for microbial exploitation of
host molecules in which the human pathogen Neisseria gonorrhoeae binds vitronectin without the involvement of a
specific gonococcal vitronectin receptor (10). In this
event, vitronectin binding is indirect and mediated through heparin or
functionally related sulfated polysaccharides. These molecules form a
stable molecular bridge between the bacterial surface adhesin OpaA and vitronectin, both of which are heparin binding proteins (2, 7, 18,
19, 40-42). The relevance of this system was demonstrated by the
ability of vitronectin-coated gonococci to invade certain types of
epithelial cells that were otherwise not susceptible to gonococcal
infection (10).
The ability of proteins to interact with heparin is widespread in both
the prokaryotic and eukaryotic worlds. This is due in large part to the
fact that heparin binding consensus sites within various proteins are
relatively ambiguous, requiring only clusters of six to eight
alternating basic and hydropathic amino acid residues (5, 6,
20). These sites interact with exposed sulfate groups present in
heparin and other sulfated polysaccharides, such as heparan sulfate and
dextran sulfate. Heparin has thus been shown to interact with
bacterial, viral, and parasitic pathogens (reviewed in reference
30), as well as with numerous mammalian proteins,
including cytokines, adhesive glycoproteins, growth factors, complement
components, plasma lipoproteins, and regulators of hemostasis
(20). This extensive binding capability led us to
hypothesize that binding of heparin and functionally related sulfated
polysaccharides is an efficient strategy utilized by microbial
pathogens to recruit a diverse array of mammalian heparin binding
proteins to their surfaces, bypassing the need to synthesize individual
receptors for each of these proteins. In the present study, we tested
this concept and evaluated its potential impact on key aspects of the
host-pathogen relationship.
Reagents.
Heparin (sodium salt; 180 U/mg) was obtained from
ICN Biomedicals Inc. (Aurora, Ohio). Dextran sulfate (average molecular weight, 500,000) was obtained from Sigma (St. Louis, Mo.). Heparan sulfate was a generous gift from Cornelius Van Gorp (Celsus
Laboratories, Cincinatti, Ohio). Vitronectin was purified from adult
bovine serum as described previously (45), and the
vitronectin-specific polyclonal antiserum was obtained from Calbiochem
(San Diego, Calif.). Human fibronectin was obtained from Becton
Dickinson (Cockeysville, Md.). The fibronectin-specific monoclonal
antibody was purified from culture supernatants of hybridoma cell line HB91 (American Type Culture Collection, Rockville, Md.) as described previously (40). All human cytokines, acidic fibroblast
growth factor, and their respective polyclonal antisera were obtained from Peprotech, Inc. (Rocky Hill, N.J.). Human epidermal growth factor
(EGF) was obtained from Life Technologies, and the EGF-specific polyclonal antiserum was from Peprotech.
Bacterial strains, cell lines, and growth conditions.
N.
gonorrhoeae MS11 (nonpiliated/LOS type b), Neisseria
meningitidis B1940siaA (16), staphylococcal
strains, Streptococcus pyogenes NZ131, and Yersinia
pestis KIM6 and Yersinia enterocolitica "Tacoma"
were generously provided by John Swanson (Rocky Mountain Laboratories,
Hamilton, Mont.), Matthias Frosch (Institut für Hygiene und
Microbiologie, Würzburg, Germany), Michael Minnick (University of
Montana, Missoula), Michael Chaussee (Rocky Mountain Laboratories), and
Joseph Hinnebusch (Rocky Mountain Laboratories), respectively.
Helicobacter pylori MC903 was obtained from the American
Type Culture Collection. S. pyogenes and H. pylori were routinely grown on blood agar plates (BBL,
Cockeysville, Md.) at 37°C in 5% CO2 or under
microaerophilic conditions (using the Campypak Plus system
[BBL]), respectively. All other strains were maintained on GC agar
plates (composition [per liter]: 3.75 g of Trypticase peptone
[BBL], 7.5 g of Thiotone E [BBL], 4 g of K2HPO4, 1 g of
KH2PO4, 5 g of NaCl, 1 g of soluble
starch [BBL], and 1% Bacto Agar [Difco, Detroit, Mich.], pH 7.2)
containing 1% IsoVitaleX (BBL) at 37°C in 5% CO2.
CHO-pgs745 cells and HEK293/CCR1 cells were grown in RPMI-1640 and
Dulbecco's modified Eagle's media, respectively, enriched with 5%
fetal bovine serum plus 0.8 mg of geneticin per ml (HEK293/CCR1 cells only).
Binding assays.
For binding experiments, H. pylori was cultured for 3 days in 10 ml of serum-free Brucella
Albimi broth (BBL) supplemented with 1% IsoVitaleX without shaking
under microaerophilic conditions with the Campypak Plus
system, while S. pyogenes was grown to logarithmic phase in
5 ml of Todd-Hewitt-yeast extract broth in 15-ml polystyrene tubes
without shaking. All other bacteria were cultured overnight on HEPES
agarose plates as previously described (10). The bacteria
were suspended in 10 ml of HEPES-buffered saline (HBS; 10 mM HEPES, 145 mM NaCl, 5 mM KCl, 1 mM CaCl2, 1 mM MgCl2, 5 mM
glucose, pH 7.2), collected by centrifugation (1,800 × g;
6 min; 20°C), and diluted in HBS to an optical density of 0.13 at 550 nm. Two milliliters (approximately 108 organisms) of
this suspension was centrifuged again, and the bacterial pellets were
resuspended in 200 µl of HBS containing no sulfated polysaccharide or
in HBS containing heparin (5 µg/ml), dextran sulfate (5 µg/ml), or
heparan sulfate (15 µg/ml). After incubation for 10 min at 5°C, the
bacteria were washed twice by centrifugation (15,000 × g;
2 min; 20°C) with 200 µl of HBS and the pellets were
resuspended in 200 µl of HBS containing 5 µg of each purified
mammalian protein (Fig. 1 and
2)/ml or 50% pooled normal human serum
(Fig. 3) and incubated at 5°C for 10 min. After being washed three times by centrifugation, the pellets were
resuspended in 50 µl of deionized water and transferred to new tubes
containing 50 µl of sodium dodecyl sulfate-polyacrylamide gel
electrophoresis (SDS-PAGE) sample buffer (22), and 5 µl of
each sample was subjected to SDS-PAGE. The presence of
bacterium-associated mammalian proteins in the lysates was analyzed by
immunoblotting with specific antisera or monoclonal antibodies as
previously described for vitronectin binding (11). The
identity of each protein was confirmed by duplicate Western blots of
the purified proteins (data not shown).
0019-9567/99/$04.00+0
Sulfated Polysaccharide-Directed Recruitment of
Mammalian Host Proteins: a Novel Strategy in Microbial
Pathogenesis
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
) and
immunomodulatory (gamma interferon) intermediates, and fibroblast
growth factor. This strategy impacts key aspects of microbial
pathogenicity as exemplified by increased bacterial invasion of
epithelial cells and inhibition of chemokine-induced chemotaxis. Our
findings illustrate a previously unrecognized form of parasitism that
complements classical virulence strategies encoded within the microbial genome.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
View larger version (69K):
[in a new window]
FIG. 1.
Sulfated-polysaccharide-mediated binding of mammalian
proteins to N. gonorrhoeae producing the heparin binding
adhesin OpaA. Gonococci were preincubated with buffer alone ( 
),
heparin (Hp), or dextran sulfate (DS), washed, and subsequently
incubated in buffer containing the purified mammalian protein as
indicated next to each gel. Bacterium-associated proteins were detected
by SDS-PAGE and immunoblotting with polyclonal antisera or monoclonal
antibodies specific for each protein, as described in Materials and
Methods. Each gel shows the major band(s) recognized by the
corresponding antibody for each protein as determined by companion
Western blots for each purified protein: vitronectin (Vn), 78 and 68 kDa; fibronectin (Fn), 220 kDa; FGF, 15.8 kDa; EGF, 6.2 kDa; IFN-
,
16.7 kDa; PF-4, 8 kDa; MIP-1, 8 kDa; and MCP-3, 9 kDa. Fn,
Fn-specific monoclonal antibody; Vn, Vn-specific monoclonal
antibody.
View larger version (36K):
[in a new window]
FIG. 2.
Sulfated-polysaccharide-dependent recruitment of heparin
binding proteins by various bacterial pathogens. Each of the bacterial
strains was incubated in buffer containing either vitronectin (Vn),
IFN- , or MCP-3 after preincubation in the absence () or presence
(+) of dextran sulfate (DS), as described in Materials and Methods.
Shown are immunoblots probed with antisera specific for each protein as
indicated. N.g.
, N. gonorrhoeae producing no
Opa protein; N.g.A, N. gonorrhoeae producing
OpaA; N.m., N. meningitidis; H.p., H. pylori;
S.e., Staphylococcus epidermidis; S.a., Staphylococcus
aureus; Y.e., Y. enterocolitica; Y.p., Y. pestis; S.p., S. pyogenes.
View larger version (46K):
[in a new window]
FIG. 3.
Heparan sulfate-mediated recruitment of heparin binding
proteins from human serum. Gonococci were preincubated with buffer
alone ( ) or with heparan sulfate (HS), washed, and subsequently
incubated in buffer containing normal human serum. Bacterium-associated
proteins were detected by SDS-PAGE and immunoblotting with vitronectin
(Vn)- and fibronectin (Fn)-specific antisera as described in Materials
and Methods. The migrations and the sizes of molecular mass standards
in kilodaltons are indicated between the gels. The band migrating at
>200 kDa may represent cross-reactivity of the anti-vitronectin
(Vn) serum with fibronectin. The apparently exclusive binding of the
68-kDa vitronectin band represents the predominance of that band in
human serum (26). Fn, anti-fibronectin antibody.
Cell invasion assay. The CHO-pgs745 cell line was kindly provided by Jeffrey Esko (University of California San Diego, La Jolla). Infection assays with these cells have been described previously (10). Vitronectin was bound to S. pyogenes via dextran sulfate as described above, and approximately 107 bacteria were added to nearly confluent monolayers of CHO-pgs745 cells grown on glass coverslips in 24-well plates. The infections were allowed to proceed for 2 h in serum-free Dulbecco's modified Eagle's medium (Life Technologies) at 37°C and 5% CO2. The numbers of extracellular and intracellular streptococci were enumerated microscopically after differential immunogold-silver staining with a polyclonal antiserum specific for group A streptococci (dilution, 1/500; Biodesign, Kennebunk, Maine) as previously described for gonococcal invasion assays (43).
Cell migration assays. The human embryonic kidney cell line HEK293 transfected with the CCR1 receptor (HEK293/CCR1) was a generous gift from Ji Ming Wang (Frederick Cancer Research and Development Center, Frederick, Md.). Migration of these cells through polyvinylpyrrolidone-free polycarbonate filters with 10-µm pores (Osmonics, Livermore, Calif.) was assayed essentially as described previously (3), except that after trypsinization, the cells were diluted in 10 ml of RPMI medium containing 5% fetal calf serum in 50-ml polypropylene centrifuge tubes (Corning, Corning, N.Y.) and allowed to recover for 2 h at 37°C and 5% CO2. The cells were then washed three times by centrifugation (400 × g; 5 min; 20°C) and resuspended in HBS to a concentration of 3 × 105/ml before addition to the chambers. A total of 108 organisms from logarithmic broth cultures of S. pyogenes or N. gonorrhoeae MS11-OpaA+ grown overnight on HEPES agarose plates were preincubated in HBS alone or in HBS containing 5 µg of dextran sulfate/ml as described for the binding assays above. After being washed by centrifugation (15,000 × g; 2 min; 20°C), the bacteria (3 × 107 streptococci and 108 gonococci) were resuspended in 100 µl of HBS and added to the lower compartment of blind-well chemotaxis chambers (NeuroProbe, Gaithersburg, Md.) with or without MCP-3 (200 ng/ml). The chambers were centrifuged (450 × g; 5 min; 20°C) before assembly and addition of 100 µl of the HEK293/CCR1 cell suspension to the upper chambers. Migration was allowed to proceed for 60 min at 37°C and 5% CO2, after which migrating cells adherent to the underside of the filter were fixed (30 min; 2% paraformaldehyde-0.1% glutaraldehyde), stained for 5 min in 0.05% crystal violet, and counted. The data represent the mean number of cells migrating to the lower side of the filter in 20 high-power fields (final magnification, ×1,000) ± standard errors. The experiments were performed in duplicate and repeated at least three times. Statistical significance was determined by the paired t test.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
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Sulfated-polysaccharide-mediated binding of bioactive mammalian
proteins by N. gonorrhoeae.
The ability of heparin and
functionally related molecules to facilitate the recruitment of diverse
mammalian heparin binding proteins to bacterial surfaces was initially
assayed with N. gonorrhoeae MS11 producing the heparan
sulfate-specific adhesin OpaA. For these experiments, gonococci were
grown on medium solidified with agarose to avoid interference by
agar-derived polysaccharides, which have been shown to bind to OpaA
(10, 41). The binding assays involved preincubation of the
bacteria in buffer alone or in buffer containing either heparin or the
functionally related molecule dextran sulfate in order to saturate OpaA
with sulfated polysaccharide. This was followed by incubation in fresh
buffer containing one of the following proteins: vitronectin,
fibronectin, gamma interferon (IFN-), platelet factor 4 (PF-4),
macrophage inflammatory protein 1 (MIP-1), monocyte chemotactic
protein 3 (MCP-3), or acidic fibroblast growth factor (FGF). Although these proteins have very different functional and structural
characteristics, they all share the ability to bind to heparin. After
removal of unbound protein, the bacteria were lysed and associated
proteins were detected by electrophoresis and immunoblotting with
antibodies specific for each protein.
Binding of mammalian proteins by various bacterial species.
The ability to bind heparin and related sulfated polysaccharides is
widespread in the microbial world. Thus, we hypothesized that the
sulfated polysaccharide-mediated binding of mammalian proteins observed
for N. gonorrhoeae may represent a novel form of phenotypic
modulation that can be exploited by any microorganism with heparin
binding capabilities. This hypothesis was tested by examining the
binding of vitronectin, IFN-, or MCP-3 to nine different bacterial
species, including H. pylori, S. pyogenes, and
Yersinia, Staphylococcus, and pathogenic
Neisseria species. For these assays, the microorganisms were
cultured in media free of agar-derived sulfated polysaccharides, as
described above. Preincubation of every bacterial species with dextran
sulfate resulted in efficient binding of all three of these heparin
binding proteins (Fig. 2). In contrast, none of the proteins bound
significantly to bacteria that had been preincubated without dextran
sulfate. Furthermore, Opa N. gonorrhoeae,
which has been shown to exhibit negligible heparin binding capabilities
(7, 42), also lacked the ability to bind significant amounts
of protein. These data indicate that sulfated polysaccharides are
absolutely required for the binding of vitronectin, IFN-, and MCP-3
to the tested bacterial species and confirm that the recruitment of
mammalian proteins through sulfated-polysaccharide intermediates is a
common feature among bacterial pathogens that bind heparin.
Heparan sulfate-mediated recruitment of proteins from a complex biological fluid. During a natural infection, microbial pathogens encounter highly complex and changing host environments containing various polysaccharides and mixtures of proteins, only some of which may have heparin binding properties. To investigate the efficiency of the microbial sulfated-polysaccharide-mediated recruitment mechanism in a more native biological setting, we tested OpaA+ gonococci for their ability to recruit proteins from human serum, which contains measurable amounts of fibronectin and vitronectin (25, 33). In these experiments, the bacteria were preincubated in buffer with or without heparan sulfate, a natural heparin-like molecule which makes up the side chains of many cell surface proteoglycans and is shed into the environment during tissue damage (21). After incubation of the heparan sulfate-coated bacteria in 50% normal human serum (10 min; 5°C), the bacteria were washed and proteins bound to the gonococcal surface were assayed by Western blotting with vitronectin- and fibronectin-specific antibodies as described for Fig. 1. This procedure demonstrated that gonococci that had been preincubated with heparan sulfate efficiently recruited both fibronectin and vitronectin from human serum (Fig. 3). In contrast, virtually no binding was detected for bacteria that lacked heparan sulfate at their surfaces. These data show that bacterial pathogens can utilize natural glycosaminoglycans (i.e., heparan sulfate) to simultaneously recruit multiple heparin binding proteins from a biological fluid, even though numerous other proteins are present in the mixture.
Polysaccharide-mediated recruitment of vitronectin enhances the invasive potential of bacterial pathogens. A key question regarding the glycosaminoglycan-mediated interaction of host proteins with microbial pathogens lies in the impact of the event on both bacterial behavior and the host's physiology. To address these issues, we first analyzed the effect of sulfated polysaccharide-mediated vitronectin binding on the interaction between S. pyogenes and Chinese hamster ovary (CHO) cells, in keeping with the increasingly appreciated role of vitronectin and related adhesive glycoproteins as mediators of bacterial colonization and invasion of eukaryotic cells. In these experiments, epithelial cells deficient in heparan sulfate proteoglycan biosynthesis (CHO-pgs745) were utilized in order to eliminate any influence of proteoglycan molecules that are present at the cell surface or shed into the medium during the assay (33). Preincubation of S. pyogenes in buffer lacking dextran sulfate and vitronectin resulted in virtually no interaction between the bacteria and CHO-pgs745 cells (Fig. 4). After sequential preincubation of the streptococci with dextran sulfate (5 µg/ml) and then with vitronectin (5 µg/ml), however, a mean internalization level of 14.1 bacteria per cell was achieved. These results are fully in line with the observed vitronectin binding under these conditions (Fig. 2). Similar experiments with N. gonorrhoeae producing OpaA gave comparable results (reference 10 and data not shown). Together, these data indicate that sulfated-polysaccharide-dependent binding of vitronectin to bacterial surfaces is an effective bacterial strategy to enhance invasive potential.
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Bacterial recruitment of chemokines inhibits efficient migration of CCR1-expressing cells. Biological effects resulting from the glycosaminoglycan-mediated bacterial recruitment of chemokines were evaluated by employing the well-documented ability of the chemokine MCP-3 to induce chemotaxis of monocytes and other cells producing the C-C chemokine receptor, CCR1 (1, 3, 39). Through the use of blind-well chemotactic chambers, we assayed the directed migration of human embryonic kidney cells transfected with cDNA encoding CCR1 (HEK293/CCR1) toward MCP-3 in the absence and presence of N. gonorrhoeae or S. pyogenes after preincubation of the bacteria with dextran sulfate. Fig. 4 shows that the presence of MCP-3 alone in the lower chamber stimulated the migration of HEK293/CCR1 cells at levels approximately 8.4-fold (S. pyogenes) and 14.1-fold (N. gonorrhoeae) over migration in buffer alone. When MCP-3 plus bacteria that had been preincubated without dextran sulfate were included in the lower chamber, similar levels of migration were observed. However, when dextran sulfate-coated bacteria were added to the lower chamber along with MCP-3, migration was inhibited by 65% for S. pyogenes (P < 0.002) and 71% for N. gonorrhoeae (P < 0.001) compared to that toward uncoated bacteria plus MCP-3. In the absence of MCP-3, there was no substantial migration toward bacteria present in the lower chamber whether or not they were preincubated with dextran sulfate. These results indicate that bacteria coated with sulfated polysaccharides inhibited migration of CCR1-expressing cells, presumably by sequestering MCP-3 and preventing the formation of an effective chemotactic gradient.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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In this report, we describe a novel, common bacterial strategy by which pathogens, including H. pylori, S. pyogenes, and Yersinia, Staphylococcus, and pathogenic Neisseria species, may amplify their pathogenic potential without the requirement for complex genetic machineries. The mechanism, schematically presented in Fig. 5, enables bacteria to recruit structurally and functionally diverse bioactive host proteins, including inflammatory mediators, adhesive glycoproteins, growth factors, and cytokines, without producing separate receptors for each protein. The bacteria accomplish this by binding heparin or functionally related sulfated polysaccharides to their surfaces, which in turn serve as secondary binding sites for mammalian heparin binding proteins. Recruitment of these factors profoundly impacts bacterial behavior, as illustrated by observed increases in bacterial invasiveness and inhibition of chemokine-induced chemotaxis.
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A key aspect of the described mechanism lies in the property of single sulfated polysaccharide molecules to interact simultaneously with multiple proteins. This allows the formation of a stable molecular bridge between heparin binding proteins present on the surfaces of most pathogens (7, 8, 24, 27, 32, 37, 41, 42) and mammalian heparin binding proteins (10). Sulfated polysaccharides, such as glycosaminoglycans, appear to be particularly suited for this system, as they contain multiple binding sites that recognize clusters of only six to eight alternating basic and hydropathic amino acid residues that are typical of heparin binding consensus sequences (5, 6, 20). The relatively low level of binding specificity enables promiscuous binding of a number of different microbial and mammalian heparin binding proteins, thus providing the microbes with a tremendous capacity for altering the protein composition of their surfaces (Fig. 1 and 2). Additional variation may be achieved through the variable molecular characteristics of different types of sulfated polysaccharides, which may exhibit slightly different heparin binding properties (10, 31, 36). Our data indicate that heparin, glycosaminoglycans, and dextran sulfate can act as bridging molecules but that they interact with different repertoires of heparin binding proteins (Fig. 1). Thus, under natural conditions, the bacterial phenotype may largely depend on the availability and nature of the sulfated polysaccharides as well as on heparin binding proteins present at the various infection niches.
A remarkable feature of the recruitment strategy is that it provides a rapid and efficient instrument for responding to environmental changes through the production of a single heparin binding protein. This is in contrast to most classical genomic systems of surface variation and adaptation, which often consume considerable amounts of time, energy, and genetic space (13). An additional major difference between the two strategies is that the genomic systems provide programmed bacterial phenotypes while the extragenomic recruitment strategy has a less predictable outcome that largely depends on environmental conditions. This flexibility, however, appears to nicely complement the genetically encoded pathogenic potential and may enable optimal adaptation to the highly dynamic environment encountered in each host.
The potential impact of the recruitment strategy on pathogenesis was substantiated by the observed increased bacterial invasion of epithelial cells in the presence of heparin and vitronectin. Microbial invasion of mammalian cells is considered to be an important virulence trait, providing pathogens with access to deeper tissues and temporary protection against inflammatory and immunological responses. Adhesive glycoproteins, such as vitronectin and fibronectin, have been implicated as intermediates in bacterial interactions with host cell integrin receptors, resulting in bacterial colonization and invasion of epithelial cells (9-12, 15, 17, 23, 28, 38, 40). Our data indicate that pathogens which lack the intrinsic ability to synthesize specific vitronectin receptors can still acquire the invasive capabilities associated with this protein through the glycosaminoglycan bridge mechanism of protein recruitment. This expansion of pathogenic potential was observed for S. pyogenes and N. gonorrhoeae, emphasizing the universality and significance of the recruitment mechanism.
The broad range of mammalian proteins that can be recruited to the bacterial cell surface (Fig. 1), which includes several cytokines and inflammatory mediators, opens the possibility that microorganisms also exploit this system to manipulate the host defense. Support for this concept is provided by the effect of bacterial recruitment of the chemokine MCP-3. MCP-3 is a heparin binding member of the C-C chemokine subfamily that induces the directed migration of cells producing its receptor, CCR1 (1), and stimulates the specific infiltration of monocytes into tissues (39, 44, 46). Our data demonstrate that sulfated polysaccharides mediate MCP-3 binding to N. gonorrhoeae and S. pyogenes and that this recruitment significantly inhibits the migration of CCR1-expressing cells toward MCP-3. This is most likely due to the sequestering of MCP-3 by sulfated polysaccharides bound to the microbial surface, preventing the establishment of an effective chemotactic gradient. The bacterial modulation of chemokine activity is to some extent reminiscent of chemokine sequestering through overexpression of viral C-C chemokine receptor homologs in cytomegalovirus-infected fibroblasts, although chemotaxis was not specifically assayed in these studies (4). Chemokine-directed infiltration of leukocytes during inflammatory responses is a primary host defense mechanism against microbial pathogens (35). Considering the intricate networks of overlapping gradients involving multiple chemoattractants in the control of leukocyte homing into target tissues (14), it is likely that minute disturbances in these gradients caused by microbes coated with sulfated polysaccharides profoundly influence the appropriate infiltration of effector cells to sites of infection and thus the progression of disease.
In mammals, the polysaccharide molecules which participate in the bridge mechanism are unknown. One candidate class of molecules are heparan sulfate glycosaminoglycans. The regulated shedding of heparan sulfate-containing proteoglycans during tissue damage (21), in conjunction with the efficient bacterial recruitment of both vitronectin and fibronectin from serum through heparan sulfate, supports this notion and confirms that the glycosaminoglycan bridge mechanism is functional in a highly complex biological setting. However, it should be noted that bacteria, viruses, and parasites can often bind heparan sulfate and heparin as well as related polysaccharides, indicating that additional undefined sulfated polysaccharides (41) may operate in vivo. This, combined with the fact that many mammalian heparin binding proteins function as adhesive, inflammatory, and immunomodulatory intermediates, led us to suggest that appreciation of the polysaccharide-mediated recruitment mechanism will greatly impact our views regarding microbial pathogenesis and the prospects for the use of glycosaminoglycan derivatives as prophylactic or therapeutic reagents.
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ACKNOWLEDGMENTS |
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We extend our appreciation to Ji Ming Wang for providing the CCR1-transfected cells, Jeffrey Esko for the CHO-pgs745 mutant cell line, and Cornelius Van Gorp (Celsus Laboratories) for the heparan sulfate. We also thank Tom Schwan, Joe Hinnebusch, and Kit Tilly for critical reading of the manuscript.
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FOOTNOTES |
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* Corresponding author. Mailing address: Rocky Mountain Laboratories, 903 South Fourth St., Hamilton, MT 59840. Phone: (406) 363-9307. Fax: (406) 363-9204. E-mail: jos_van_putten{at}nih.gov.
Present address: Cellomics, Pittsburgh, PA 15238.
Editor: E. I. Tuomanen
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Abstract
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Materials and Methods
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Discussion
References
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