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Clinical Microbiology Reviews, October 2006, p. 597-613, Vol. 19, No. 4
0893-8512/06/$08.00+0 doi:10.1128/CMR.00006-06
Copyright © 2006, American Society for Microbiology. All Rights Reserved.
Departments of Medicine,1 Microbiology and Immunology, Vanderbilt University School of Medicine,2 Veterans Affairs Tennessee Valley Healthcare System, Nashville, Tennessee3
SUMMARY INTRODUCTION ANTIBACTERIAL PROPERTIES OF THE HUMAN STOMACH H. PYLORI FACTORS THAT CONTRIBUTE TO GASTRIC COLONIZATION IMMUNE RESPONSE TO H. PYLORI IN HUMANS Acute Infection Chronic Infection Factors Modulating the Immune Response to H. pylori in Humans INTERACTIONS BETWEEN H. PYLORI AND HOST DEFENSES IN ANIMAL MODELS H. pylori Infection of Wild-Type Animals H. pylori Infection of Knockout Mice Th1 and Th2 Responses in Mice Role of Regulatory T Cells Protective Immunity in Animal Models INTERACTIONS BETWEEN H. PYLORI AND IMMUNE CELLS IN VITRO Immune Recognition of H. pylori by Gastric Epithelial Cells Interactions of H. pylori with Neutrophils Interactions of H. pylori with Mast Cells Interactions of H. pylori with Macrophages Interactions of H. pylori with Dendritic Cells Interactions of H. pylori with B Lymphocytes Interactions of H. pylori with T Lymphocytes CONCLUDING REMARKS ACKNOWLEDGMENTS REFERENCES
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| INTRODUCTION |
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| ANTIBACTERIAL PROPERTIES OF THE HUMAN STOMACH |
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Multiple factors produced by the gastric mucosa limit the proliferation of bacteria (Fig. 1). Antibacterial peptides, including ß-defensins 1 and 2 and LL-37, are active against many different species of bacteria (74, 94). Lactoferrin inhibits bacterial growth by restricting the availability of extracellular Fe3+ (133) and can have direct effects on bacterial membrane permeability (13, 175, 253). Lactoferricin, a peptide derived from lactoferrin, also has antimicrobial properties (80). Lysozyme can degrade the peptidoglycan of many bacterial species. Surfactant protein D is capable of aggregating many different types of microorganisms in a calcium-dependent and lectin-specific manner (114, 158, 164). Finally, specific components of human gastric mucin can inhibit bacterial growth; alpha-1,4-GluNAC-capped O-glycans inhibit biosynthesis of cholesteryl-
-D-glucopyranoside, a component of the H. pylori cell wall (112).
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The antibacterial properties of the human stomach described above prevent most bacterial species from colonizing the stomach. Based on the high prevalence of H. pylori in humans throughout the world, it may be presumed that H. pylori possesses mechanisms to overcome these innate host defenses.
| H. PYLORI FACTORS THAT CONTRIBUTE TO GASTRIC COLONIZATION |
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H. pylori outer membrane proteins and other surface components are likely targets for recognition by host immune defenses. One mechanism by which H. pylori evades immune recognition may involve a form of antigenic disguise in which the bacteria are coated with host proteins. For example, H. pylori PgbA and PgbB proteins bind plasminogen, and the bacteria can thereby be coated with this host protein (108). Other mechanisms for evading immune recognition may involve phase variation and antigenic variation of surface components. Phase variation has been reported for multiple H. pylori surface components, including outer membrane proteins and lipopolysaccharide (LPS) antigens (14, 198, 210, 241). Genetic rearrangements contribute to antigenic variation in CagY (16), and intragenomic recombination may contribute to antigenic variation in outer membrane proteins (210).
LPS from most bacterial organisms serves as a potent signal for development of an inflammatory response. An important H. pylori adaptation is the synthesis of LPS that is less proinflammatory than LPSs from many other gram-negative species (114, 157, 181). In comparison to LPS from Escherichia coli or Salmonella enterica serovar Typhimurium, H. pylori LPS has approximately 500-fold-lower endotoxic activity (162), and its ability to stimulate macrophage production of proinflammatory cytokines, nitric oxide, and prostaglandins is relatively weak (35, 181). The low biological activity of H. pylori LPS is attributable to modifications of its lipid A component (157, 162). H. pylori strains commonly express LPS O antigens that are structurally related to Lewis blood group antigens found on human cells (19, 154). This similarity in structure between H. pylori LPS and Lewis blood group antigens may represent a form of molecular mimicry or immune tolerance that permits H. pylori LPS antigens to be shielded from immune recognition because of similarity to "self" antigens.
Many H. pylori strains contain a 40-kb region of chromosomal DNA known as the cag pathogenicity island (PAI) (5, 40). Some strains contain an incomplete cag PAI (less than 40 kb in size), and in other strains the cag PAI is completely absent (40, 166). One product of the cag pathogenicity island, CagA, is translocated into gastric epithelial cells and induces numerous alterations in cellular signaling (18, 98, 171, 204, 214). Multiple other products of the cag pathogenicity island have a role in secretion of CagA and in altering gene transcription in gastric epithelial cells (5, 40, 71, 87, 205). In comparison to cag PAI-negative H. pylori strains, cag PAI-positive strains stimulate gastric epithelial cells to produce high levels of proinflammatory cytokines such as interleukin-8 (IL-8) (5, 38, 71, 87, 125, 161, 205). Gastric cancer and peptic ulcer disease occur more commonly in persons infected with cag PAI-positive strains (particularly those strains containing an intact 40-kb cag PAI) than in persons infected with cag PAI-negative strains (33, 70, 166, 236).
Several H. pylori factors are known to interact directly with immune cells and modulate immune responses to H. pylori. These factors include a secreted toxin (VacA) (37, 46, 77, 219), neutrophil-activating protein (HP-NAP or NapA) (68, 197), arginase (83, 256), urease (93, 139, 140), Hsp60 (a GroEL heat shock protein) (81), SabA (235), HcpA (53), CagA (170, 234), and a proinflammatory peptide designated Hp(2-20) (29). Several of these factors act on multiple different types of immune cells. For example, VacA alters the function of T lymphocytes, B cells, macrophages, and mast cells (37, 49, 77, 152, 219, 220, 258), and HP-NAP acts on neutrophils, mast cells, and monocytes (155, 156, 197). The activities of H. pylori factors that interact directly with immune cells will be discussed in greater detail below.
| IMMUNE RESPONSE TO H. PYLORI IN HUMANS |
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More recently, 20 human volunteers were experimentally infected with 104 to 1010 CFU of an H. pylori strain (86). Symptoms occurred most frequently during the second week after infection and included dyspepsia (in >50% of subjects), headaches, anorexia, abdominal pain, belching, and halitosis. Gastric biopsies performed 2 weeks after infection showed infiltration of lymphocytes and monocytes, along with significantly increased expression of IL-1ß, IL-8, and IL-6 in the gastric antrum (86). Four weeks after infection, the numbers of gastric CD4+ and CD8+ T cells were increased compared to preinfection levels, indicating the development of an early adaptive immune response (168). These cases provide evidence that gastric inflammation develops within a short period of time after H. pylori infection and that the initial colonization of the stomach by H. pylori frequently results in upper gastrointestinal symptoms. Either innate immune responses to H. pylori or early adaptive immune responses could account for the gastric mucosal inflammatory responses and symptoms that accompany acute infection.
In contrast to the intestine, the stomach does not contain Peyer's patches or M cells (165). Therefore, there is some uncertainty about the location where priming of the immune response to H. pylori occurs. Gastric epithelial cells up-regulate expression of major histocompatibility complex (MHC) class II and costimulatory molecules during H. pylori infection (17, 255), and potentially these cells have a role in antigen presentation. Monocytes, macrophages, and dendritic cells in the lamina propria of the gastric mucosa also may play important roles in antigen presentation (115, 222, 240). Alternatively, priming of the immune response to H. pylori may occur within lymph nodes draining the stomach or may occur at intestinal sites in response to H. pylori antigens or intact organisms that are shed from the stomach.
H. pylori-specific CD4+ T cells are detectable in the gastric mucosae of H. pylori-infected persons but not uninfected persons (52, 54, 132). One study reported that about 15% of CD4+ T-cell clones isolated from the stomachs of H. pylori-infected persons were H. pylori specific, whereas the other T-cell clones did not proliferate in response to antigens in H. pylori lysate (52). Some T-cell clones from H. pylori-infected patients recognize epitopes on parietal cell H+,K+-ATPase (9), and it has been suggested that recognition of H+,K+-ATPase by gastric T cells may contribute to the development of autoimmune gastritis (51).
Levels of numerous cytokines, including gamma interferon (IFN-
), tumor necrosis factor (TNF), IL-1ß, IL-6, IL-7, IL-8, IL-10, and IL-18, are increased in the stomachs of H. pylori-infected humans compared to uninfected humans (47, 126). IL-4 has not been detected in the gastric mucosae of most H. pylori-infected persons (110, 126, 184). The Th1-defining cytokine, IFN-, is expressed by a higher proportion of gastric T cells from H. pylori-infected persons than gastric T cells from uninfected persons (22, 91, 110, 126, 211). In one study, 83% of H. pylori-specific gastric T-cell clones produced IFN- but not IL-4 upon stimulation with H. pylori antigens, compared to 17% of clones that produced IL-4 (22, 52). Based on the relative abundance of IFN--producing T cells and the relative scarcity of IL-4-producing gastric T cells in the setting of H. pylori infection, it has been concluded that H. pylori infection leads to a Th1-polarized response (22, 211). In the setting of H. pylori infection, multiple cytokines in the gastric mucosa (including TNF, IFN-, IL-1ß, IL-6, IL-8, and IL-18) are predicted to have proinflammatory effects, whereas IL-10 is an immunoregulatory cytokine that may limit the inflammatory response.
A humoral immune response to H. pylori is elicited in nearly all H. pylori-infected humans (180). In a study of H. pylori-infected human volunteers, H. pylori-specific serum IgM antibodies were present by 4 weeks postinfection (168). Serum IgA and IgG antibodies in persons with chronic H. pylori infection are directed toward many different H. pylori antigens (147, 180). Antibody-secreting cells producing H. pylori-specific IgA or IgM antibodies are detectable in the gastric mucosae of H. pylori-infected persons (147), and secretory IgA antibodies to H. pylori are detectable in gastric juice, which suggests that H. pylori infection elicits a local secretory IgA response in the stomach (96, 147).
The gastric inflammatory response to H. pylori also may be modulated by characteristics of the human host. H. pylori-associated gastric inflammation in adults is characterized by infiltration of mononuclear cells and neutrophils, whereas in children the inflammatory response often is predominantly lymphocytic with relatively few neutrophils (246). Adults who are persistently colonized with H. pylori for many decades may develop atrophic gastritis (an inflammatory process characterized by loss of glandular structures and parietal cells in the gastric mucosa), which is considered a preneoplastic lesion (45, 117).
No immunodeficiency diseases are known to result in enhanced severity of H. pylori-associated inflammation. For example, gastric inflammation is not more severe in H. pylori-infected humans with IgA deficiency than in immunocompetent hosts (36). However, single-nucleotide polymorphisms in several genes encoding proinflammatory cytokines can influence the clinical outcome of H. pylori infection (Table 1). Polymorphisms that result in elevated levels of IL-1ß and TNF- and reduced levels of IL-10 have been associated with an increased risk of atrophic gastritis and gastric cancer (64, 66, 101, 134, 232, 248). A polymorphism in the promoter region of IL-1 receptor antagonist that leads to reduced expression of IL-1 receptor antagonist has also been associated with an increased incidence of atrophic gastritis and gastric cancer (64, 135, 187). The exact mechanisms by which these polymorphisms affect the risk for gastric cancer are not yet completely understood. Some of the TNF- and IL-10 polymorphisms associated with increased risk for gastric cancer are considered proinflammatory genotypes (66, 134), and IL-1ß is known to be a potent inhibitor of gastric acid secretion (254). These polymorphisms may predispose individuals to develop gastric atrophy and gastric cancer by pathways involving enhancement in the severity of gastric inflammation and a reduction in gastric acid secretion (254).
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Mongolian gerbils can be experimentally infected with H. pylori and develop gastric inflammation characterized by infiltration of mononuclear cells and neutrophils (149, 172, 247). An attractive feature of the Mongolian gerbil model is that these animals may develop gastric mucosal ulceration or gastric adenocarcinoma in response to H. pylori infection (73, 100, 172, 244), and they thus provide a model for two important H. pylori-associated diseases that occur in humans. Several studies suggest that products of the H. pylori cag pathogenicity island contribute to gastric pathology in the gerbil model (105, 172, 192). Limitations of this model include the relative paucity of gerbil-specific immunologic reagents and the fact that Mongolian gerbils are outbred.
The mouse model is frequently utilized because of low cost, availability of relevant reagents, and the potential for development of knockout mice (142). H. pylori can persistently colonize the stomachs of wild-type mice for periods of at least 15 months. However, wild-type mice do not develop gastric mucosal ulceration or gastric adenocarcinoma in response to H. pylori. One limitation of the mouse model is that only a few human isolates of H. pylori have been successfully adapted to permit efficient colonization of the mouse stomach (20). Infant mice and certain types of knockout mice (e.g., IL-12 knockout mice) seem to be more permissive hosts than are wild-type adult mice and tolerate infection with a broader range of H. pylori strains (89, 99). A different Helicobacter species, H. felis, also can colonize conventional inbred mice and causes more severe gastric inflammation than does H. pylori (196). However, H. felis does not express several important H. pylori virulence factors (249).
The gastric mucosal inflammation that develops in wild-type mice infected with H. pylori consists primarily of lymphocytes and other mononuclear cells. Most of the infiltrating cells are CD4+ T cells, but CD8+ T cells, B cells, dendritic cells, and monocytes are also present (167, 199, 207, 237). The intensity of inflammation that develops in H. pylori-infected mice is relatively mild compared to that which develops in H. pylori-infected humans and is also relatively mild compared to that which develops in H. pylori-infected Mongolian gerbils (121). Neutrophils are typically present in the gastric mucosae of H. pylori-infected humans (194, 246) and gerbils (100) but are less commonly observed in the gastric mucosae of H. pylori-infected mice (138).
C57BL/6 mice have been commonly used for studies of H. pylori. Gastric levels of IFN-, IL-12, TNF, and IL-6 are increased in H. pylori-infected C57BL/6 mice compared to uninfected mice, whereas gastric levels of IL-4 are not increased in response to H. pylori infection (150, 212). Upon antigen stimulation ex vivo, splenocytes from H. pylori-infected C57BL/6 mice produce substantially more IFN- than IL-4 (107, 127, 207). These patterns of cytokine expression are indicative of a predominantly Th1 response, which is similar to the response which occurs in H. pylori-infected humans.
There is variability among different strains of inbred mice in susceptibility to H. pylori infection (138, 231) and in host responses to H. pylori. Inbred mice are known to have default T-helper responses, and therefore, the genetic backgrounds of inbred mice may influence the T-cell response to H. pylori. C57BL/6 mice have a default Th1 response, whereas BALB/c mice have a default Th2 response (113). This difference may be a factor that helps to explain why BALB/c mice are relatively resistant to H. pylori colonization and why H. pylori-infected BALB/c mice develop relatively mild gastric inflammation compared to H. pylori-infected C57BL/6 mice (109, 196).
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µ-MT (B-cell-deficient) mice infected with H. pylori develop gastritis that is more severe than that which occurs in wild-type mice, and subsequently H. pylori infection is cleared from the stomachs of the B-cell-deficient mice (3). There are several possible reasons why H. pylori-induced gastritis may be more severe in B-cell-deficient mice than in wild-type mice. For example, antibodies produced by wild-type mice may engage the inhibitory IgG receptor (FcRIIb) on leukocytes and increase expression of anti-inflammatory cytokines such as IL-10 (3).
In comparison to H. pylori-infected wild-type mice, H. pylori-infected mice with defects in IFN- expression (IFN-–/– mice or interferon response factor 1–/– mice) develop less severe gastric inflammation and have higher bacterial colonization densities (2, 169, 199, 207, 212, 251). This suggests that IFN- contributes to increased severity of H. pylori-induced gastric inflammation while also contributing to reducing bacterial colonization. In support of this view, H. pylori-infected SCID mice reconstituted with splenocytes that express IFN- developed more severe gastritis than did mice reconstituted with IFN--deficient splenocytes (60). IFN- may indirectly modulate the severity of gastritis by activating macrophages to secrete proinflammatory cytokines and also may down-regulate the expression of anti-inflammatory factors such as the anti-inflammatory cytokine transforming growth factor ß (215).
In comparison to Helicobacter-infected mice that express IL-10, infected IL-10–/– mice develop more severe gastritis (26, 43). IL-10 is known to be a potent anti-inflammatory and immunoregulatory cytokine, and therefore it seems likely that IL-10 has a role in down-regulating H. pylori-induced inflammation (43). One study reported that H. pylori-infected IL-4–/– mice developed more severe gastritis than did H. pylori-infected wild-type C57BL/6 mice (207). Similarly, H. felis-infected IL-4–/– mice developed significantly more severe gastric inflammation than did H. felis-infected IL-4+/+ mice (151). Although the results of studies analyzing IL-4–/– mice have not been entirely uniform (42, 109), these data suggest that both IL-10 and IL-4 have a role in down-regulating gastric inflammation (26, 72, 151, 207, 257).
A general theme that emerges from studies of H. pylori in mouse models is that there is a reciprocal relationship between the intensity of gastric mucosal inflammation and bacterial load (or colonization density) (32, 43, 61, 188, 199, 251). For example, IFN-–/– mice have relatively high bacterial loads and mild gastritis, whereas IL-10–/– mice have relatively low bacterial loads and severe gastritis (43). As will be discussed later in this review, these observations are relevant to understanding the immunologic basis for protective immunity to H. pylori.
(a Th1 cytokine) contributes to enhanced gastric inflammation, whereas expression of certain Th2 cytokines (IL-10 and possibly IL-4) contributes to diminished inflammation. To investigate further the role of Th1 and Th2 responses in modulating gastric inflammation, C57BL/6 mice were initially infected with a nematode that induces a strong Th2 response and then were challenged with H. felis (72). In comparison to mice infected with H. felis alone, the mice coinfected with H. felis and the nematode had reduced gastric expression of Th1 cytokines (IFN-, TNF, and IL-1ß), increased gastric expression of Th2 cytokines (IL-4, IL-10, and transforming growth factor ß), and reduced gastric inflammatory scores (72). These data provide support for the hypothesis that a Th2-polarized response down-regulates the severity of H. pylori-induced gastric inflammation.
Several cytokines affect the expression of gastric hormones that control gastric acid secretion. Expression of gastrin, a hormone that stimulates gastric acid secretion, is stimulated by IFN- (257), and expression of somatostatin, a hormone that inhibits gastric acid secretion, is stimulated by IL-4 and inhibited by IFN- and TNF (25, 257). Increased expression of IFN- (a Th1 response) is expected to result in increased gastrin production, whereas expression of IL-4 (a Th2 response) is expected to result in increased somatostatin production and reduced gastrin secretion. One study used a mouse model of H. felis infection to investigate the effects of IL-4-induced alterations on gastrin and somatostatin expression (257). As expected, administration of IL-4 resulted in increased somatostatin expression and reduced gastrin expression. These changes were accompanied by a reduction in the severity of H. felis-induced gastritis. The modulatory effects of IL-4 on the severity of gastric inflammation were observed in H. felis-infected wild-type mice but not in infected somatostatin knockout mice, which suggested that the IL-4-induced alterations in inflammation were mediated through effects of IL-4 on somatostatin production by D cells (257).
production compared to mice reconstituted with an unsorted T-cell population (188). These data indicate that Tregs have an important role in regulating the gastric mucosal inflammatory response to H. pylori. Several early studies suggested that protection might be mediated by Helicobacter-specific antibodies (30, 48, 69, 122). Subsequently, it was shown that immunization of µ-MT mice (which are unable to produce antibodies) or IgA-deficient mice can result in protective immunity against H. pylori or H. felis infection (3, 31, 67, 76, 84, 221). Therefore, there is now a general consensus that H. pylori-specific antibodies are not required for protective immunity.
Cellular immune responses seem to have an important role in protective immunity against H. pylori. Mice deficient in CD8+ T cells (MHC class I–/– mice) can be successfully immunized and protected against colonization with H. pylori (177), whereas mice deficient in CD4+ T cells (MHC class II–/– mice) were not protected by prophylactic immunization against H. pylori (177). CD4+ T cells from H. felis-immunized mice can mediate protective immunity if adoptively transferred into immunodeficient Rag1–/– mice (84). These data suggest that CD4+ T cells, but not CD8+ cells, are necessary for protection (67, 177).
Several lines of evidence suggest that Th2-type responses might be required for protective immunity against H. pylori. Specifically, persistent H. pylori infections in humans and mice typically result in Th1-polarized responses, whereas successful Helicobacter immunization of animals typically results in Th2-polarized responses (1, 50). In addition, adoptive transfer of Th2 cells from H. felis-infected C57BL/6 mice into infected C57BL/6 mice significantly reduced the bacterial load compared to when Th1 cells were adoptively transferred (151). Conversely, there is evidence that a Th2 response may not be required for protection. Specifically, IL-4 and IL-5 knockout C57BL/6 mice were successfully protected from H. pylori infection following immunization (76). In addition, studies with IL-4 receptor -chain-deficient BALB/c mice (which lack both IL-4 and IL-13 signaling) suggested that IL-4 and IL-13 are not required for a protective immune response (129). Whether IFN--producing Th1 cells are required for protective immunity is not yet completely clear (75, 199). However, immunization studies using IL-12 and IL-18 knockout mice indicate that these two Th1 cytokines are required for effective protection against H. pylori and suggest that the establishment of an active Th1-type response is required for protection (2, 4, 75). In summary, the role of Th1-type versus Th2-type immune responses in protective immunity to H. pylori infection remains incompletely understood. Differences in the mouse strain backgrounds used in various studies potentially complicate interpretation of the data.
There is evidence that protective immunity against H. pylori in prophylactically immunized mice may require mast cells. In contrast to immunized wild-type mice, immunized mast cell-deficient mice (W/W v mice) were not protected from challenge with H. felis (238). Reconstitution of W/W v mice with bone marrow-derived mast cells restored the ability of W/W v mice to develop a protective immune response following prophylactic vaccination (238). The mechanism by which the mast cells contribute to protective immunity is undefined, but it may be hypothesized that mast cells modulate the activity of T cells or neutrophils through secretion of cytokines or that mast cells have antibacterial activity via the production of nitric oxide or antimicrobial peptides.
Further insight into protective immunity against H. pylori can be gleaned by analyzing levels of H. pylori colonization (bacterial load or bacterial density) in persistently infected knockout mouse models. The levels of H. pylori colonization in SCID mice are significantly higher than those in wild-type mice (61). Conversely, the levels of H. pylori colonization in IL-10 knockout mice are about 100-fold lower than those in wild-type mice (43), and in some cases, H. pylori is completely eradicated from IL-10 knockout mice (104). Control of H. pylori proliferation in IL-10 knockout mice is associated with development of a gastric mucosal inflammatory response that is more severe than that in infected wild-type mice. Therefore, it may be hypothesized that protective immune responses leading to eradication of H. pylori are associated with relatively severe gastric mucosal inflammatory responses.
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Several studies have sought to characterize the interactions of H. pylori PAMPs with TLRs in vitro. These studies have used many different cell types, including primary gastric epithelial cells, gastric epithelial cell lines, and cell lines transfected with plasmids that express TLRs and/or TLR accessory proteins. It is possible that some of the gastric epithelial cell lines used in these experiments do not express certain TLR accessory proteins such as CD14 and MD-2, which are required for TLR4 signaling. Different sources of H. pylori PAMPs have been used, including intact bacteria, purified LPS, and flagellin. Because of the many variations in experimental design, the results of these studies have not been uniform. Nevertheless, several general conclusions can be drawn from these studies.
Analyses of the interactions of purified H. pylori LPS with TLRs suggest that, in contrast to LPSs from most other gram-negative bacteria, H. pylori LPS is not well recognized by TLR4 (21, 103, 206). One study provided evidence that H. pylori LPS may act as an antagonist for TLR4 (124). H. pylori LPS induced NF-
B activation in HEK293 cells that expressed TLR2 but not in HEK293 cells that expressed TLR4 (206). These data suggest that H. pylori LPS may be recognized by TLR2 instead of by TLR4. H. pylori Hsp60 also is reported to be recognized by TLR2 (224).
Unlike flagellins from gram-negative organisms such as Salmonella enterica serovar Typhimurium, H. pylori flagellin is not recognized by TLR5 (12, 79, 123). This evasion of TLR5 recognition is attributable to alterations in H. pylori FlaA amino acid sequences in the TLR5 recognition site. If the corresponding amino acids are mutated in FlaA from Salmonella, the resulting Salmonella mutant strain is not recognized by TLR5 (12). Thus, H. pylori expresses at least two PAMPs (LPS and flagellin) that are recognized relatively poorly by TLRs and that may not trigger a strong innate immune response.
Recognition of intact H. pylori organisms by cultured epithelial cells appears to be dependent on TLR2 and TLR5 and to be independent of TLR4 (136, 141, 206). In one study, dominant negative forms of TLR2, TLR4, and TLR5 were expressed in the human gastric cancer cell line MKN45, and the cells then were incubated with H. pylori (206). The expression of chemokines (MIP3, IL-8, and GRO) in these cells in response to H. pylori was dependent on TLR2 and TLR5 signaling but not on TLR4 signaling. These studies suggest that intact H. pylori organisms can be recognized by TLR5, despite poor recognition of H. pylori flagellin by TLR5. Potentially H. pylori components other than flagellin are recognized by TLR5, or perhaps the results are influenced by variations in the methodology used in different studies.
In addition to recognition of H. pylori PAMPs by TLRs, H. pylori peptidoglycan can be recognized by Nod1 (CARD4), an intracellular pathogen recognition molecule (239). There is evidence that the type IV secretion system encoded by the H. pylori cag PAI delivers H. pylori peptidoglycan into epithelial cells. Intracellular recognition of H. pylori peptidoglycan by Nod1 leads to activation of NF-B and altered gene transcription in host cells (239). Compared to gastric epithelial cells from wild-type mice, gastric epithelial cells from Nod1-deficient mice produced significantly less macrophage inflammatory protein-2 in response to H. pylori (239).
In summary, H. pylori can be recognized in vitro by TLRs as well as the Nod1 receptor, and such recognition probably contributes to initiation of an innate immune response in vivo (Fig. 3). There is no evidence that H. pylori can evade detection by TLRs, but certain H. pylori PAMPs, such as LPS and flagellin, seem to be poorly recognized by TLRs. This may represent a mechanism by which H. pylori down-regulates the intensity of the innate immune response.
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H. pylori produces a 150-kDa oligomeric protein known as neutrophil-activating protein (HP-NAP), which is chemotactic for neutrophils and activates neutrophils in vitro (68). HP-NAP stimulates neutrophils to produce reactive oxygen intermediates, and in response to HP-NAP, neutrophils release Ca2+ and phosphorylate cytosolic cellular signaling molecules (197). In addition, HP-NAP induces expression of ß2-integrins on the surface of neutrophils (197).
An H. pylori outer membrane protein, SabA, also has an important role in human neutrophil activation (235). Wild-type strains of H. pylori expressing SabA activate neutrophils, whereas mutant and wild-type strains lacking SabA do not (235). There is evidence that binding of H. pylori to neutrophils through SabA-mediated adhesion may stimulate a G-protein-linked signaling pathway and downstream activation of phosphatidylinositol 3-kinase (235).
Whether H. pylori can resist phagocytosis by neutrophils is not yet completely resolved (7, 170), but one study reported that uptake of unopsonized H. pylori by neutrophils was inefficient compared to uptake of latex-coated beads and that H. pylori could inhibit phagocytosis of latex-coated beads or Neisseria gonorrhoeae (189). If nonopsonized H. pylori organisms are phagocytosed by neutrophils, the bacteria are able to resist intracellular killing (7, 227). One mechanism by which nonopsonized H. pylori evades intracellular killing may involve disruption of NADPH oxidase targeting, such that superoxide anions generated in the oxidative burst do not accumulate in the phagosome but instead are released into the extracellular space (7). A catalase-dependent pathway also may have a role in allowing nonopsonized H. pylori to evade intracellular killing (189).
The migration of neutrophils in response to chemokines IL-8 and Gro is mediated through the chemokine receptors CXCR1 and CXCR2 (163). H. pylori can down-regulate the expression of CXCR1 and CXCR2 in human neutrophils in vitro, and this is predicted to have an inhibitory effect on neutrophil migration (202). In summary, multiple H. pylori factors can activate neutrophils, and there is also evidence that H. pylori can interfere with the proper functioning of neutrophils.
Although not all studies have reached identical conclusions (170), at least one study reported that H. pylori is able to inhibit its own uptake by macrophages (190). When nonopsonized H. pylori organisms are internalized by macrophages, they initially localize in phagosomes, which then coalesce into "megasomes" that contain multiple bacteria (8, 193). Ingested H. pylori cells have at least some ability to resist intracellular killing (8). One study reported that phagolysosomal fusion is impaired in H. pylori-infected macrophages through retention of the tryptophan aspartate-containing coat protein on phagosomes, a phenomenon that is expected to result in increased intracellular survival of the bacteria (258).
Phagocytosis of bacteria by macrophages typically results in localization of the microorganisms within phagosomes that contain protein kinase C (PKC) isoform (39). PKC activation plays a role in the respiratory burst and phagosome-lysosome fusion (120). Upon phagocytosis of nonopsonized H. pylori by macrophages, PKC isoforms 
and 
accumulate on the forming phagosomes, but the conventional PKC isoform does not (6). Experiments using specific PKC inhibitors suggest that PKC regulates actin rearrangement and H. pylori engulfment (6) and that phagocytosis of nonopsonized H. pylori by macrophages may occur via a novel PKC -regulated pathway. The ability of nonopsonized H. pylori to resist macrophage killing may be attributable to features of this PKC -mediated phagocytic process. Opsonized H. pylori is phagocytosed by a PKC -independent process, which is likely to involve conventional pathways (6).
One mechanism by which H. pylori impairs the antimicrobial activity of macrophages involves expression of catalase. In comparison to a wild-type catalase-positive H. pylori strain, an isogenic, catalase-deficient strain was more susceptible to macrophage-mediated killing (23). Another mechanism by which H. pylori resists macrophage killing is by blocking the production of nitric oxide. This effect is mediated by H. pylori arginase, which competes with nitric oxide synthase for arginine (83). In addition to resisting killing by macrophages, in vitro experiments indicate that H. pylori can induce macrophage apoptosis (41, 44, 82). H. pylori-induced apoptosis of macrophages may result in impaired innate and adaptive immune responses.
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H. pylori arginase also contributes to inhibition of T-cell proliferation. One study reported that incubation of T cells with a wild-type H. pylori strain, but not an arginase mutant strain, caused decreased expression of the CD3 chain of the T-cell receptor (256). In addition to VacA and arginase, an uncharacterized low-molecular-weight protein of H. pylori has been reported to inhibit proliferation of T lymphocytes (78). This low-molecular-weight H. pylori factor is reported to block cell cycle progression at the G1 phase.
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| ACKNOWLEDGMENTS |
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This work was supported by NIH grants R01 AI39657, R01 DK53623, and T32 AI 07474 and by the Department of Veterans Affairs.
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), DCs, mast cells, and gastric epithelial cells. Innate immune recognition of H. pylori is mediated at least in part through TLRs. In addition, H. pylori peptidoglycan (PG) can be recognized by intracellular Nod receptors (