Effects of Helicobacter pylori on intracellular Ca2+ signaling in normal human gastric mucous epithelial cells

Katie L. Marlink,1 Kathy D. Bacon,1 Brett C. Sheppard,1 Hassan Ashktorab,3 Duane T. Smoot,3 Timothy L. Cover,4 Clifford W. Deveney,1,2 and Michael J. Rutten1

1Department of Surgery and 2Veterans Affairs Medical Center, Oregon Health Sciences University, Portland, Oregon, 97201; 3Department of Medicine, Howard University, Washington, District of Columbia 20060; and 4Departments of Medicine, Microbiology, Immunology, and Veterans Affairs Medical Center, Vanderbilt University School of Medicine, Nashville, Tennessee 37232

Submitted 1 July 2002 ; accepted in final form 15 February 2003


    ABSTRACT
 TOP
 ABSTRACT
 MATERIALS AND METHODS
 RESULTS
 DISCUSSION
 REFERENCES
 
In stomach, Helicobacter pylori (Hp) adheres to gastric mucous epithelial cells (GMEC) and initiates several different signal transduction events. Alteration of intracellular Ca2+ concentration ([Ca2+]i) is an important signaling mechanism in numerous bacteria-host model systems. Changes in [Ca2+]i induced by Hp in normal human GMEC have not yet been described; therefore, we examined effects of Hp on [Ca2+]i in normal human GMEC and a nontransformed GMEC line (HFE-145). Cultured cells were grown on glass slides, porous filters, or 96-well plates and loaded with fura 2 or fluo 4. Hp wild-type strain 60190 and vacA, cagA, and picB/cagE isogenic mutants were incubated with cells. Changes in [Ca2+]i were recorded with a fluorimeter or fluorescence plate reader. Wild-type Hp produced dose-dependent biphasic transient [Ca2+]i peak and plateau changes in both cell lines. Hp vacA isogenic mutant produced changes in [Ca2+]i similar to those produced by wild type. Compared with wild type, cagA and picB/cagE isogenic mutants produced lower peak changes and did not generate a plateau change. Preloading cultures with intracellular Ca2+ chelator BAPTA blocked all Hp-induced [Ca2+]i changes. Thapsigargin pretreatment of cultures to release Ca2+ from internal stores reduced peak change. Extracellular Ca2+ removal reduced plateau response. Hp-induced peak response was sensitive to G proteins and PLC inhibitors. Hp-induced plateau change was sensitive to G protein inhibitors, src kinases, and PLA2. These findings are the first to show that H. pylori alters [Ca2+]i in normal GMEC through a Ca2+ release/influx mechanism that depends on expression of cagA and picB/cagE genes.

vacA; cagA; picB/cagE; bacteria; signal transduction; fura 2; fluo 4; cell culture; immunofluorescence; thapsigargin; genistein; herbimycin; G protein; stomach


HELICOBACTER PYLORI is associated with the induction of gastric inflammation and is a risk factor for peptic ulcer disease and distal gastric cancer (38). Two important virulence factors produced by H. pylori strains are a vacuolating cytotoxin (VacA) and products of a 40-kb genetic locus of ~31 genes termed the cag pathogenicity island (PAI) (8). VacA is a secreted toxin that produced multiple functional and morphological changes within gastric epithelial cells (36). The cag PAI encodes proteins that act to form a type IV secretion system that is responsible for translocation of the H. pylori CagA protein into gastric cells (2, 6, 12, 33, 51, 56). The picB/cagE gene, which encodes a homolog of the Agrobacterium VirB4 ATPase, is also necessary for the translocation of the H. pylori CagA protein into the gastric cell (6, 14, 17, 33). Also, products of the cag PAI act to induce synthesis and secretion of IL-8 (60), increase MAP kinase activity (20), induce gastric epithelial cell proliferation and apoptosis (18, 39), and induce transactivation of the epidermal growth factor receptor (EGFR) (21) and cyclooxygenase-2 mRNA expression (45). Other mutagenesis studies involving the cag PAI have found that disruption of the cagA gene resulted in a reduction in gastric cell arachidonic acid release and prostaglandin E2 synthesis (40), in a decreased stress kinase gene expression (30), and in reduced expression of the protooncogenes c-fos and c-jun (26). The presence of the cagA gene and its expressed product, the CagA protein, have also been reported as necessary for the induction of specific gastric cell morphological changes such as cell elongation, spreading, and scattering, which has been designated as the "hummingbird" phenotype (5, 16, 4951). Of interest is a recent study suggesting that just the presence of the CagA protein (an not necessarily phosphorylated CagA protein) can induce this hummingbird phenotype (27). Other H. pylori-induced morphological changes, such as gastric cell stress fiber formation, were shown to be cagA and vacA independent (49).

Despite the recent advances in H. pylori-host cell mutagenesis and transcriptional profiling (14), little is known about certain aspects of H. pylori signaling in normal gastric cells such as the regulation of intracellular Ca2+ concentrations ([Ca2+]i). In other model systems, bacterial adherence to the host cell has been shown to result in specific [Ca2+]i changes (10). For example, the adherence of certain Escherichia coli strains to intestinal epithelial cells results in increased [Ca2+]i and inositol trisphosphate levels (11). It has also been shown that Salmonella induces intracellular Ca2+ changes that were linked to the activation of an NF-{kappa}B-dependent inflammatory pathway (13). In this regard, a study using the intracellular Ca2+ chelator BAPTA along with calmodulin inhibitors found that H. pylori activation of NF-{kappa}B and IL-8 signaling in MKN45 human gastric cancer cells was Ca2+-calmodulin dependent (32). The reported H. pylori-induced hummingbird phenotype in gastric cells is similar to the morphological events seen with hepatocyte growth factor or scatter factor (HGF/SF) on MDCK cells or hepatocytes (44). It has also been reported that HGF/SF can induce changes in [Ca2+]i, which have been shown to be linked to changes in cell morphology and proliferation (1, 19, 31, 34).

However, despite the extensive work on various aspects of H. pylori-induced signaling in gastric cancer cells, the specific mechanism(s) of intracellular Ca2+ mobilization by H. pylori in normal human gastric mucous epithelial cells has not yet been thoroughly examined. Also, many H. pylori signaling studies have used either nongastric or gastric cancer cell lines as a model system, which always introduces a degree of uncertainty as to whether the events observed are applicable to normal gastric cells. As an alternative to nongastric gastric cancer cell lines, several in vitro model systems of normal human gastric mucous epithelial cells have been established (7, 48, 54, 61). The use of nontransformed cell culture models provides a more accurate representation of the environment that H. pylori may encounter in the normal human gastric mucosa. The aim of the present study, therefore, was to examine the effects of H. pylori on intracellular Ca2+ signaling in normal human gastric epithelial cells. We found for the first time that H. pylori produces specific transient [Ca2+]i changes in normal human gastric mucous epithelial cells and that these H. pylori-induced [Ca2+]i changes could also be replicated in a nontransformed gastric mucous epithelial cell line (HFE-145 cells). We also found that a G protein-dependent/PLC pathway primarily regulated H. pylori-induced intracellular Ca2+ release, whereas H. pylori-induced Ca2+ influx was primarily regulated by components of a G protein-, src kinase-, and PLA2-dependent pathway. Finally, we report that mutagenesis of picB/cagE and cagA genes (located within the cag PAI), but not the vacA gene, alters the capacity of H. pylori to produce a full [Ca2+]i response.


    MATERIALS AND METHODS
 TOP
 ABSTRACT
 MATERIALS AND METHODS
 RESULTS
 DISCUSSION
 REFERENCES
 
Chemicals and peptides. The Ca2+ probes fura 2-AM and fluo 4-AM (special packaging) as well as BAPTA-AM were purchased from Molecular Probes (Eugene, OR) and stored at –20°C until needed. All Ca2+ probes were freshly prepared as 5-mM stock solutions on the day of the experiment by dissolving preweighed aliquots in cultured-grade DMSO (Sigma, St. Louis, MO). The compounds methyl arachidonyl fluorophosphate (MAFP), thapsigargin, 4-amino-5-(4-chlorophenyl)-7-(t-butyl)pyrazolo[3,4-d] pyrinidine (PP2), pertussis toxin (PTX), U-73122, and U-73343 were purchased from Calbiochem (San Diego, CA). Type I collagenase, RIA grade BSA powder, Triton X-100, digitonin, and genistein were purchased from Sigma. Cell culture media were from GIBCO (San Diego, CA), and FBS was from Hyclone (Logan, UT). Unless noted otherwise, all Falcon cell culture plasticware was purchased from Fisher Scientific (San Francisco, CA).

Gastric epithelial cell culture. Human gastric mucous cells were isolated and cultured as previously described (48). The Oregon Health Sciences University (OHSU) Human Studies Subcommittee approved all procedures and handling of human tissue. Briefly, H. pylori-free gastric tissues were obtained from patients undergoing surgical gastrectomy. The surgical specimens were washed twice in serum-free media and pinned down on polymerized Sylgard, and the epithelium was removed by scraping the surface with a glass slide. The scraped tissue pieces were minced by using razor blades then washed three times at 100 g for 3 min in serum-free media. The pellets were then transferred to siliconized 125-ml screw-cap Erlenmeyer flasks containing 20 ml of serum-free culture media with 20 mg/ml of type I collagenase and 0.1% bovine serum albumin. The flasks were then gassed with 95% O2-5% CO2, put into a 37°C shaking water bath, and gyrated at 120 oscillations/min for 45 min. At the end of the incubation period, the collagenase-digested mixture was put into a 50-ml syringe with an attached 15-gauge luer-stub adapter, and the contents were pushed through a 200-µm nylon mesh screen. The mesh-filtered suspension was washed twice in serum-free media and centrifuged at 100 g for 3 min, then the pellet was resuspended in 15 ml of serum-free culture media and a 200-µl aliquot was taken for cell counts in a Coulter Counter. The 15-ml suspension was divided into three 5-ml aliquots in 16 x 125-cm Falcon round-bottom tubes, then 5 ml of isosmotic Percoll was added to each tube. The tubes were centrifuged for 15 min at 100 g at 24°C, and the bottom pellet, containing the gastric mucous epithelial cells, was removed. The pellet was washed three times and centrifuged at 20 g for 3 min in serum-free cell culture media, then the cells were plated on 0.45-µm Falcon porous filters (catalog no. 353180; 12 mm, 0.45-µm pore size), 25 mm round glass coverslips, or 96-well plastic dishes.

The HFE-145 human gastric mucous epithelial cell line (provided by D. Smoot) were plated and grown under the same experimental conditions as the above human primary gastric mucous epithelial cells. The HFE-145 cells were originally developed from normal human gastric epithelial cells by the transfection of normal cells with SV40 Large T-antigen and human telomerase vectors (53). The cells have a doubling time of ~24 h and are strongly positive for cytokeratin-10,11,18 and weakly positive for cytokeratin-13,16,20, which is almost identical to cytokeratin staining of the parental cell line. These cells also stain positive for neutral mucin using periodic acid-Schiff and negative for alcian blue (acidic mucin), which is consistent with normal gastric epithelial cells. Growth of these cells was inhibited when cells were placed in soft agar, suggesting that these cells are not tumorigenic. The cells constitutively express mRNA from Muc-5ac, Muc-5b, and Muc-6 genes, which is consistent with normal gastric epithelial cells. Electron microscopy shows that these cells form tight junctions when grown as monolayers on plastic tissue culture dishes and on glass slides (53).

H. pylori culture. The H. pylori bacteria used in this study were the wild-type vacA+, cag+ 60190 (ATCC 49503), an isogenic vacA mutant, isogenic cagA mutant, and an isogenic picB/cagE mutant. H. pylori 60190 contains a type s1a/m1 vacA allele (59). The vacA, cagA, and picB-/cagE mutants have been previously described (39, 52, 59). The bacteria were grown on blood agar plates (trypticase soy agar with 5% sheep blood; PML Microbiologicals, Tualatin, OR) under microaerobic conditions using a CampyPak jar (Fisher Scientific) at 36°C. Unless noted otherwise, all bacteria were harvested at 24 h by using a sterile cotton swab and 3 ml of PBS (pH 7.1). The bacterial suspensions were put into 12-ml Falcon round-bottom tubes, and the H. pylori was resuspended by gentle inversion. A 1-ml aliquot of the suspension was put into a cuvette, and the H. pylori concentration was determined by using optical density 600 nm (OD600) where an OD of 1 = 1.2 x 109 colony-forming units (CFU)/ml. All final bacterial suspensions (1 x 105–1 x 109 CFU/ml) were adjusted with the appropriate mammalian Ringer solution. The mammalian Ringer solution consisted of (in mM): 137 NaCl, 4 KCl, 25 NaHCO3, 2 KH2PO4, 15 HEPES, 1 MgSO4, 2 CaCl2, and 25 glucose, pH 7.4. Periodically, the bacteria were plated in serial dilutions on agar plates and H. pylori concentrations were checked by counting the bacterial colonies after 3 days of incubation.

H. pylori sonicates were made by growing the bacteria on agar plates for 24 h and then harvesting the bacteria in PBS as indicated above. The bacteria were washed twice in PBS by centrifugation at 10,000 g for 15 min, and then the pellet was resuspended in mammalian Ringer (pH 7.4). The bacterial suspensions were disrupted by sonication (10 30-s pulses), the sonicates were filtered through a 0.2-µm filter, and the protein content was determined by using a Bio-Rad protein assay. Aliquots were frozen and stored at –80°C until needed. For control studies, both live bacteria and bacterial sonicates were heated to 70°C for 30 min to generate heat-inactivated bacteria and sonicates.

H. pylori and gastric cell [Ca2+]i using fura 2. Primary cultures of gastric mucous epithelial cells, the HFE-145 cell line, and AGS gastric cancer cells were grown on either permeable Falcon filters or 25-mm round glass coverslips. After 24 h in serum-free media, the cells were loaded with fura 2-AM according to modifications of previously described techniques (47). Briefly, the cells were loaded with 2.5 µM fura 2-AM in fresh serum-free media for 45 min at 37°C. After fura 2-AM loading, the cells were washed twice with fresh serum-free media, then twice with mammalian Ringer. When extracellular Ca2+-free Ringer solutions were used, the CaCl2 was replaced with NaCl and the solution was characterized as nominally Ca2+-free Ringer. In preliminary experiments, we found that the use of our nominally Ca2+-free Ringer solution did not affect H. pylori adherence. However, the addition of 1 mM EDTA and 1 mM EGTA to the nominally Ca2+-free Ringer solution decreased H. pylori adherence and disrupted monolayer integrity over the experimental time period and therefore could not be used (data not shown). Solutions were oxygenated with 5% CO2–95% O2, kept warm at 37°C in a heated water bath, and perfused into the chamber by using a variable Millipore pump.

After fura 2 loading, the gastric cultures were transferred to a horizontal open perfusion chamber that had been modified to hold either a permeable Falcon filter or a glass coverslip (46). The chamber was then placed on the stage of a Nikon Diaphot TMD inverted microscope equipped with a fluorescence objective (Nikon Fluor-phase-3DM, numerical aperature 60/0.7, 160-mm working distance). [Ca2+]i measurements were made at 340/380 nm excitation and 510 nm emission wavelengths from an SLM-Aminco spectrophotometer (Rochester, NY). The effects of nonspecific H. pylori fluorescence scatter and cell autofluorescence were determined by placing an unloaded gastric cell monolayer with varying doses of H. pylori (1 x 105–1 x 109 CFU/ml) on the microscope stage, then emission ratios were recorded and subtracted from the final fura 2 tracings. In preliminary experiments, we found light scattering by the bacteria and cellular autofluorescence did not exceed 5% of the total fura 2 fluorescence.

In some experiments, the rates of H. pylori-induced intracellular Ca2+ release and influx were estimated by using the "Ca2+ add-back technique" (43). For these experiments, fura 2-loaded gastric cells are initially incubated in the absence of extracellular Ca2+, then H. pylori is added and [Ca2+]i is recorded as intracellular Ca2+ release, then extracellular Ca2+ (2.0 mM) is "added back" and the [Ca2+]i change is measured as Ca2+ influx.

The final calibration of the fura 2 signal was done at the end of each experiment by adding 5 µM ionomycin for 10 min to saturate fura 2 with Ca2+ to obtain maximal fluorescence (Fmax), then 10 mM EGTA and 10 mM EDTA plus 60 mM Tris·HCl, pH 10.5, was added to chelate the Ca2+ from fura 2 to determine the minimal fluorescence (Fmin). Additional points on the calibration curve were determined by using a series of defined Ca2+-calibration solutions (Kit #1, C-3008; Molecular Probes), and [Ca2+]i was calculated (58). The fluorescence tracing analysis and data smoothing were done with software provided by the manufacturer (SLM-Aminco).

H. pylori and gastric cell [Ca2+]i using a fluo 4 96-well assay. In some experiments we wanted a quicker throughput assay to measure the relative change in [Ca2+]i produced by H. pylori with different kinase inhibitors. For these experiments, measurement of [Ca2+]i was done using a modification of a 96-well fluorescence assay (25). Cultures of normal human gastric epithelial cells were grown to confluence in 96-well plates and loaded with 2.5 µM fluo 4-AM for 45 min at 37°C. After being loaded, the cultures were washed twice with mammalian Ringer and then incubated for another 30 min with fresh 37°C Ringer solution. Fluo 4 fluorescence was recorded using a 96-well fluorescence plate reader (FluoStar; BMG Technologies, Durham, NC) equipped with excitation (485 ± 20 nm) and emission (530 ± 20 nm) filters. After the addition of H. pylori or drugs, fluorescence measurements were made every 2 s. The Fmax measurement for the human gastric epithelial cells was obtained by adding a solution of 5 µM ionomycin and 100 µM digitonin to the gastric cells for 15 min. After this, the Fmin measurement was obtained by adding a solution of 10 mM EGTA-10 mM EDTA in 60 mM Tris·HCl, pH 10.5, for 15 min. The values for Fmax and Fmin were graphed, and individual fluorescence values were obtained by using a single wavelength equation for fluo 4 (58).

Statistics. All data are expressed as means ± SE. The differences between means were considered significant when the P value calculated from Students' t-test for paired cultures was <0.05. Multiple cell culture comparisons were analyzed by using ANOVA and Duncan's multiple-range tests. Unless stated otherwise, n represents the total number of different "individual" cell preparations isolated from different surgical specimens. All statistical calculations were made using SigmaStat statistical software (SPSS, San Rafael, CA).


    RESULTS
 TOP
 ABSTRACT
 MATERIALS AND METHODS
 RESULTS
 DISCUSSION
 REFERENCES
 
H. pylori mobilizes intracellular Ca2+ in normal gastric mucous epithelial cells. For the first series of experiments, we used a modified horizontal chamber on an inverted microscope connected to a spectrophotometer. This particular setup has the advantage that smaller volumes can be used, allowing a quicker rate of H. pylori settling and adherence to the gastric cells. Before the addition of H. pylori, a baseline fluorescence measurement was taken of the fura 2-loaded gastric mucous cell cultures, then varying doses of H. pylori (1 x 105–1 x 109 CFU/ml) were added and [Ca2+]i was measured. As shown in the composite tracings in Fig. 1, we found that wild-type H. pylori (strain 60190) induced a dose-dependent change in [Ca2+]i in primary cultures of human gastric mucous epithelial cells. Over the time course of 60 min, the wild-type strain produced a characteristic biphasic [Ca2+]i increase (transient "peak") that was followed by a decline and then a return to above [Ca2+]i baseline values ("plateau" phase) (Fig. 1). At the highest H. pylori concentration used (1 x 109 CFU/ml), there was a change in [Ca2+]i from a basal level of 104 ± 2 nM to a peak of 184 ± 4 nM, followed by a decline and then a rise again to a plateau level of 145 ± 4 nM (n = 14; Table 1).



View larger version (24K):
[in this window]
[in a new window]
 
Fig. 1. Graphs showing representative tracings of intracellular Ca2+ concentration ([Ca2+]i) changes with varying concentrations [1 x 106–1 x 109 colony-forming units (CFU)/ml] of wild-type (60190) Helicobacter pylori (Hp) on fura 2-loaded primary cultures of human gastric mucous epithelial cells (A) and the HFE-145 gastric mucous epithelial cell line (B). Note that the addition of H. pylori (thick arrow) produced a concentration-dependent biphasic change in [Ca2+]i, which was followed by a return to baseline [Ca2+]i levels in both cell types. Heat-killed wild-type H. pylori produced no detectable [Ca2+]i change in either the primary gastric cultures or the HFE-145 gastric cell line. For all tracings, n = 14 independent experiments.

 

View this table:
[in this window]
[in a new window]
 
Table 1. Helicobacter pylori-induced [Ca2+]i changes in gastric mucous epithelial cells

 

To independently validate the previous results, we tested the effects of H. pylori on [Ca2+]i in the nontumorigenic HFE-145 human gastric mucous epithelial cell line. The HFE-145 cell line has morphological and phenotypic properties similar to those seen in primary gastric mucous epithelial cells (53). Compared with the primary gastric mucous epithelial cell cultures, we found that H. pylori produced similar [Ca2+]i changes in the HFE-145 cell line (Fig. 1B). That is, H. pylori dose-dependently produced the characteristic biphasic peak and plateau changes in [Ca2+]i (Fig. 1B; Table 1). For example, H. pylori (1 x 109 CFU/ml) produced a change in baseline [Ca2+]i from 106 ± 2 nM to a peak of 177 ± 4 nM, which was followed by a decline and then an increase to plateau levels of 140 ± 4 nM (n = 14; Table 1). Although some quantitative differences in H. pylori-induced intracellular Ca2+ signaling existed between the primary human gastric mucous epithelial cell cultures and the HFE-145 cell line, overall the qualitative patterns of H. pylori-induced [Ca2+]i changes were similar in both cell types. It should be noted that after several passages (>25) of the HFE-145 cell line, we began to lose the characteristic H. pylori-induced intracellular Ca2+ response that was observed in early cultures (data not shown).

In addition to live bacteria, we also tested the capacity of H. pylori sonicates (0–5 µg/ml) to induce changes in [Ca2+]i in normal gastric mucous epithelial cells. However, we found that the H. pylori sonicates, even at the highest concentration used (5 µg/ml), produced only a small, slow, steady change in [Ca2+]i from a baseline level of 103 ± 3 nM to 119 ± 4 nM over a 60-min time course (n = 9). Because the bacterial sonicates did not reproduce the [Ca2+]i changes observed with live intact H. pylori, they were not used for the remainder of our experiments. Compared with the untreated control cultures, we also found that heat-killed H. pylori produced no significant change (P > 0.05) in [Ca2+]i over the 60-min time period (control = 106 ± 3 nM; heat-killed bacteria = 108 ± 4 nM; n = 9; Fig. 1). We also found that the pretreatment of the gastric mucous epithelial cell cultures with the Ca2+ chelator BAPTA completely abolished the wild-type H. pylori-induced [Ca2+]i changes over 60 min (control = 106 ± 3 nM; H. pylori-treated = 107 ± 3 nM; n = 7). These data confirm that intact live H. pylori are able to induce a specific [Ca2+]i change in normal gastric mucous epithelial cells. In addition, the H. pylori-induced [Ca2+]i change is characterized by an initial transient peak [Ca2+]i increase followed by a sustained plateau [Ca2+]i phase that can be specifically blocked by the Ca2+ chelator BAPTA.

The role of vacA, cagA, and picB/cagE genes in H. pylori-induced [Ca2+]i changes. It is well established that the VacA toxin secreted by H. pylori is an important virulence factor in the pathogenesis of peptic ulcer disease (36). In addition, the CagA protein encoded by the cagA gene within the H. pylori cag PAI is involved in gastric host cell cytoskeletal responses (5, 16, 4951). Also, residing within the cag PAI is the picB/cagE gene, which encodes a structural component of the type IV secretion system that is important in translocating the CagA protein as well as activation of signaling mechanisms involved in immune responses and cell growth and apoptosis (37). We therefore were interested in testing the role of the H. pylori vacA, cagA, and picB/cagE genes on intracellular Ca2+ signaling. Using a vacA isogenic mutant strain on primary cultures of human gastric mucous epithelial cells, we found that the vacA isogenic mutant produced peak and plateau [Ca2+]i changes that were nearly identical to those seen in the wild-type 60190 strain (Fig. 2A; Table 2). The heat-killed H. pylori vacA isogenic mutant strain produced no change in [Ca2+]i in the gastric cells (Fig. 2A). In contrast to the wild-type and vacA isogenic mutant strains, the cagA and picB/cagE isogenic strains produced markedly attenuated [Ca2+]i changes (Fig. 2B). That is, the wild-type strain (1 x 109 CFU/ml) produced a peak [Ca2+]i response of 184 ± 4 nM compared with the significantly (P < 0.05) smaller peak responses of 157 ± 4 and 143 ± 5 nM, respectively, from the cagA and picB/cagE isogenic mutants (Table 2). Of the two mutant strains, the picB/cagE-induced [Ca2+]i peak response of 143 ± 5 nM was also found to be significantly (P < 0.05) lower than the cagA-induced [Ca2+]i peak response of 157 ± 4 nM (Table 2). We also found that after treating the gastric cells for 15 min with either the cagA or picB/cagE mutant strains we could no longer detect a [Ca2+]i change over the remainder of the 60-min time course (Fig. 2B; Table 2). That is, the cagA and picB/cagE isogenic mutants did not generate the typical prolonged plateau phase as seen with the H. pylori wild-type strain or vacA isogenic mutant (compare Fig. 2, B to A; Table 2). We have also found this same attenuated [Ca2+]i response using other independent picB/cagE and cagA mutant strains derived from wild-type 60190 strain (M. J. Rutten and T. L. Cover, unpublished data). These data suggest that the expressed products of the cagA and picB/cagE genes (but not vacA) contribute to H. pylori-induced [Ca2+]i changes.



View larger version (22K):
[in this window]
[in a new window]
 
Fig. 2. Graph showing the comparative effects of wild-type H. pylori 60190 and the vacA, cagA, and picB/cagE isogenic strains on [Ca2+]i changes in fura 2-loaded primary cultures of normal human gastric mucous epithelial cells. The addition of the vacA strain (1 x 109 CFU/ml) produced nearly identical [Ca2+]i changes compared with the wild-type strain (A). Compared with the wild-type strain, the addition of the cagA and picB/cagE isogenic strains (1 x 109 CFU/ml) to the cultures produced only small [Ca2+]i peak changes with no [Ca2+]i plateau change (B). Heat-killed vacA cagA, and picB/cagE isogenic strains produced no change in [Ca2+]i. For all tracings, n = 14 independent experiments.

 

View this table:
[in this window]
[in a new window]
 
Table 2. Effects of H. pylori wild-type and isogenic strains on [Ca2+]i changes in primary cultures of normal human gastric mucous epithelial cells

 

H. pylori-induced [Ca2+]i: intracellular Ca2+ release vs. Ca2+ influx. One of the main intracellular Ca2+ stores within most cells is the thapsigargin-sensitive sarcoendoplasmic reticular (SERCA) Ca2+ store (43, 58). Thapsigargin inhibits the Ca2+-ATPase on the SERCA membrane, which then leads to the release of Ca2+ and depletion of the intracellular Ca2+ store (43). As a first step in identifying the source(s) of the H. pylori-induced [Ca2+]i change, fura 2-loaded gastric mucous epithelial cells grown on glass slides were pretreated with 500 nM thapsigargin, and then H. pylori (1 x 109 CFU/ml) was added and [Ca2+]i was measured. In thapsigargin-pretreated gastric cells, H. pylori wild-type and vacA, cagA, and picB/cagE mutant strains all had reduced [Ca2+]i peak levels [from 184 ± 4, 177 ± 5, 157 ± 4, and 143 ± 3 nM to 117 ± 4, 115 ± 3, 112 ± 4, and 110 ± 3 nM, respectively (n = 9; Fig. 3A)]. The H. pylori-induced wild-type and vacA [Ca2+]i plateau change was only slightly diminished by the thapsigargin pretreatment (Fig. 3A). Because the cagA and picB/cagE H. pylori strains were previously found to produce no [Ca2+]i plateau change (see Fig. 2), the thapsigargin pretreatment of the gastric cells was without effect on this portion of the [Ca2+]i response (Fig. 3B).



View larger version (24K):
[in this window]
[in a new window]
 
Fig. 3. Effects of intracellular Ca2+ depletion on H. pylori-induced [Ca2+]i changes in primary cultures of human gastric mucous epithelial cells. Fura 2-loaded human gastric mucous epithelial cell cultures were pretreated for 30 min with 500 nM thapsigargin to release intracellular Ca2+. The appropriate H. pylori strains (1 x 109 CFU/ml) were then added, and [Ca2+]i changes were recorded. Compared with untreated control cultures, thapsigargin pretreatment of the gastric cells primarily affected the wild-type and vacA H. pylori-induced [Ca2+]i peak response with only small reductions in the [Ca2+]i plateau change (A). Thapsigargin pretreatment also reduced the cagA and picB/cagE H. pylori-induced [Ca2+]i peak changes (B). Because the cagA and picB/cagE H. pylori strains were found to produce no [Ca2+]i plateau change, the thapsigargin pretreatment of the gastric cells was without effect on this portion of the cagA and picB/cagE [Ca2+]i response (B). For all tracings, n = 10 independent experiments.

 

In addition to the release of intracellular Ca2+ stores, the opening of Ca2+ channels in the plasma cell membrane can also contribute to the change in [Ca2+]i (43). A general experimental approach in examining the contribution of Ca2+ channels to the total agonistinduced [Ca2+]i change is to use the Ca2+ add-back technique (see MATERIALS AND METHODS; Ref. 43). For these experiments, fura 2-loaded primary gastric mucous epithelial cells were first pretreated with extracellular Ca2+-free Ringer solution, H. pylori was added, and [Ca2+]i was recorded, followed 30 min later by the readdition of extracellular Ca2+ to the Ringer. We found that there was only a small, nonsignificant (P > 0.05) reduction in the wild-type and vacA H. pylori-induced [Ca2+]i peak responses using extracellular Ca2+-free buffer (Fig. 4A). However, the extracellular Ca2+ treatment greatly reduced the wild-type and vacA H. pylori-induced [Ca2+]i plateau response from control levels of 145 ± 4 and 141 ± 3 nM to 103 ± 4 and 100 ± 4 nM, respectively (n = 10; Fig. 4A). When extracellular Ca2+ was added back to the Ringer solution, we found that the [Ca2+]i in the H. pylori wild-type and vacA-treated gastric cultures rose to near control plateau levels (Fig. 4A). The extracellular Ca2+ treatment also did not significantly (P > 0.05) reduce the cagA- and picB/cagE-induced [Ca2+]i peak response from control levels of 157 ± 4 and 151 ± 4 nM to 143 ± 5 and 138 ± 4 nM, respectively (n = 10; Fig. 4B). Because the cagA or picB/cagE mutant strains do not produce an [Ca2+]i plateau change (see Fig. 2), the effect of readdition of extracellular Ca2+ to the Ringer solution to detect Ca2+ influx was without effect on this portion of the [Ca2+]i response (Fig. 4B). Overall, these experiments suggest that the H. pylori-induced peak [Ca2+]i change is dependent primarily on release of intracellular thapsigargin-sensitive Ca2+ stores, whereas the H. pylori-induced plateau [Ca2+]i change is primarily dependent on extracellular Ca2+ influx.



View larger version (26K):
[in this window]
[in a new window]
 
Fig. 4. Effects of extracellular Ca2+-free Ringer on H. pylori-induced [Ca2+]i changes in primary cultures of human gastric mucous epithelial cells. Fura 2-loaded human gastric mucous epithelial cell cultures were first exposed to extracellular Ca2+-free Ringer for 15 min to minimize Ca2+ influx; then the appropriate H. pylori strains (1 x 109 CFU/ml) were introduced and [Ca2+]i was recorded. Later, 2.0 mM Ca2+ was returned to the extracellular Ringer and [Ca2+]i was measured again. We found that Ca2+-free Ringer pretreatment of the gastric cells primarily affected the wild-type and vacA H. pylori-induced [Ca2+]i plateau response with only small reductions in the [Ca2+]i peak change (A). When extracellular Ca2+ was "added back" to the Ringer solution (double arrows), there was an immediate rise in [Ca2+]i to plateau levels like that seen H. pylori-treated gastric cells in Ringer with Ca2+ (A; compare with Fig. 1A). In contrast, the Ca2+-free Ringer pretreatment of the gastric cells only slightly reduced the cagA and picB/cagE [Ca2+]i peak changes (B). Because there is no H. pylori-induced [Ca2+]i plateau change produced by either the cagA or picB/cagE mutant strains, the effect of the removal and readdition of extracellular Ca2+ to the Ringer solution (double arrows) was without effect on this portion of the [Ca2+]i response (B). For all tracings, n = 10 independent experiments.

 

H. pylori-induced Ca2+ release is regulated by a PLC-dependent mechanism. Several agonists as well as certain bacterial pathogens have been shown to induce Ca2+ release from intracellular stores through a PLC-mediated process (42). In the next series of experiments, we used the PLC inhibitor U-73122 to test whether PLC activation is involved in H. pylori-induced [Ca2+]i changes. In the wild-type and vacA isogenic strains, the U-73122 pretreatment considerably reduced the [Ca2+]i peak increase with less of an effect on the [Ca2+]i plateau change (Fig. 5, A and B). Compared with untreated controls, the U-73122 also significantly reduced the cagA or picB/cagE peak change in [Ca2+]i (Fig. 5, C and D). Because the cagA and picB/cagE isogenic strains do not generate a plateau [Ca2+]i change, U-73122 was without effect on this portion of the [Ca2+]i response (Fig. 5, C and D). As a control, cultures were pretreated with the structurally related but ineffective PLC drug U-73343, and it did not alter any of the [Ca2+]i changes produced by the wild-type, vacA, cagA, and picB/cagE strains on the gastric cells (data not shown). However, it should be noted that the control compound U-73343 used at concentrations >2.5 µM actually inhibited H. pylori-induced Ca2+ signaling, indicating that at >2.5 µM both U-73122 and U-73343 exhibit nonspecific inhibitory effects (data not shown). These data suggest that H. pylori-induced intracellular Ca2+ release (but not Ca2+ influx) is under the control of a PLC-dependent mechanism.



View larger version (28K):
[in this window]
[in a new window]
 
Fig. 5. Graph showing the effects of the PLC inhibitor U-73122 on H. pylori-induced [Ca2+]i changes in primary cultures of human gastric mucous epithelial cells. Fluo 4-loaded human gastric mucous epithelial cells were first pretreated with 2 µM U-73122 for 30 min, then the appropriate H. pylori strains (1 x 109 CFU/ml) were added and [Ca2+]i was recorded. In the wild-type (A) and vacA isogenic (B) strains, the U-73122 pretreatment considerably reduced the [Ca2+]i peak increase with less of an effect on the [Ca2+]i plateau change. Compared with untreated controls, U-73122 also significantly reduced the cagA (C) or picB/cagE (D) peak change in [Ca2+]i. Because the cagA and picB/cagE isogenic strains do not generate a plateau [Ca2+]i change, U-73122 was without effect on this portion of the [Ca2+]i response (C and D). Data are from 10 independent experiments and expressed as means ± SE; *P < 0.05 vs. control peak and plateau levels.

 

H. pylori-induced [Ca2+]i changes are regulated by src kinases. It has now been well documented that the src kinases play an important signaling role in the phosphorylation of the translocated CagA protein as well as participation of H. pylori-induced cytoskeletal changes (2, 16, 50, 55). It has also been shown in other cell types that src kinases play a modulatory role in agonist-induced [Ca2+]i changes (9). We therefore wanted to examine the role of src kinases in H. pylori-induced intracellular Ca2+ signaling in gastric cells where src kinase activity was inhibited by using PP2. Pretreatment of the primary human gastric mucous epithelial cell cultures with PP2 produced a dose-dependent differential decrease in H. pylori wild-type and vacA isogenic [Ca2+]i peak and plateau changes (Fig. 6). That is, PP2 pretreatment (0.5–5.0 µM) of the gastric cells was most effective in reducing the H. pylori wild-type and vacA mutant [Ca2+]i plateau response (Fig. 6, A and B). Only at higher concentrations of PP2 (15 µM) did we observe a reduction in both the H. pylori wild-type strain and vacA mutant [Ca2+]i peak and plateau changes to baseline levels (Fig. 6, A and B). We also found that only at the highest PP2 concentration used (15 µM) was the cagA and picB/cagE [Ca2+]i peak change reduced to baseline levels (Fig. 6, C and D). Because the cagA and picB/cagE isogenic strains do not generate an [Ca2+]i plateau change (see Fig. 2), the PP2 was without effect on this portion of the [Ca2+]i response (Fig. 6, C and D). Overall, these results with the various concentrations of PP2 suggest that the src kinases are more likely to have a regulatory role in controlling the H. pylori wild-type and vacA mutant-induced [Ca2+]i "plateau" (Ca2+ release) than the [Ca2+]i "influx" change.



View larger version (35K):
[in this window]
[in a new window]
 
Fig. 6. Dose-response effects of src kinase inhibitor 4-amino-5-(4-chlorophenyl)-7-(t-butyl)pyrazolo[3,4-d] pyrimidine (PP2) on H. pylori-induced [Ca2+]i changes in cultures of human gastric mucous epithelial cells. Fluo 4-loaded human gastric mucous epithelial cell cultures were pretreated for 30 min with varying doses of PP2; then the appropriate H. pylori strains (1 x 109 CFU/ml) were added and [Ca2+]i was recorded. In the wild-type (A) and vacA isogenic (B) strains, low to intermediate doses of PP2 (0.5–5.0 µM) primarily attenuated the [Ca2+]i plateau change, with higher doses (15 µM) of PP2 completely reducing both the peak and plateau changes to control levels. Compared with untreated controls, PP2 also dose-dependently reduced the cagA (C) and picB/cagE (D) [Ca2+]i peak change. Because the cagA and picB/cagE isogenic strains do not generate an [Ca2+]i plateau response, PP2 was without effect on this portion of the [Ca2+]i response (C and D). Data are from 10 independent experiments and expressed as means ± SE; *P < 0.05 vs. control peak and plateau levels.

 

H. pylori-induced Ca2+ influx is regulated by G proteins and a PLA2-dependent mechanism. In several cell types, agonist-induced changes in [Ca2+]i can be altered by PTX-sensitive G proteins as well as PLA2 activity (23, 28). In addition, it has been reported that H. pylori-induced arachidonic acid release from the human cervical adenocarcinoma HeLa cell line could be abolished by PTX and the PLA2 inhibitor MAFP (40). For the next series of experiments, we were therefore interested in determining the effects of PTX treatment on H. pylori-induced Ca2+ release and Ca2+ influx in cultures of normal human gastric mucous epithelial cells. We found that PTX pretreatment of the gastric cells caused a reduction in both the wild-type and vacA H. pylori-[Ca2+]i peak and plateau changes to baseline [Ca2+]i levels (Fig. 7, A and B). The effect of PTX pretreatment also caused a reduction of the cagA and picB/cagE mutant [Ca2+]i peak change to near baseline levels (Fig. 7, C and D). Because the cagA and picB/cagE isogenic strains do not generate a [Ca2+]i plateau change, the PTX pretreatment had no effect on this portion of the [Ca2+]i response (Fig. 7, C and D).



View larger version (28K):
[in this window]
[in a new window]
 
Fig. 7. Effects of the G protein inhibitor pertussis toxin (PTX) on H. pylori-induced [Ca2+]i changes in cultures of normal human gastric mucous epithelial cells. The cultures were preincubated for 3 h with PTX (250 ng/ml), loaded with fluo 4, and then treated with the appropriate H. pylori wild-type or isogenic strain (1 x 109 CFU/ml), and [Ca2+]i was recorded. Compared with untreated cultures, PTX pretreatment caused a reduction of the wild-type (A) and vacA (B) H. pylori-[Ca2+]i peak and plateau changes to baseline levels. The effect of PTX pretreatment also caused a reduction of the cagA (C) and picB/cagE (D) [Ca2+]i peak change to near baseline levels. Because the cagA and picB/cagE isogenic strains do not generate a [Ca2+]i plateau change, the PTX pretreatment had no effect on this portion of the [Ca2+]i response (C and D). Data are from 9 independent experiments and expressed as means ± SE; *P < 0.05 vs. control peak and plateau levels.

 

We next investigated the effects of inhibiting cPLA2 on H. pylori-induced intracellular Ca2+ signaling in primary cultures of normal human gastric mucous epithelial cells. We found no significant effect (P > 0.05) of MAFP on the wild-type and vacA H. pylori-induced [Ca2+]i peak change, whereas MAFP had a significant effect (P < 0.05) on the wild-type and vacA H. pylori-induced [Ca2+]i plateau change (Fig. 8 A and B). Also, MAFP had no significant effect (P > 0.05) on the cagA or picB/cagE-induced [Ca2+]i peak change (Fig. 8, C and D). Because the cagA and picB/cagE isogenic strains do not generate a [Ca2+]i plateau change, MAFP was without effect on this portion of the [Ca2+]i response (Fig. 8, C and D). Overall, these results suggest that the H. pylori-induced plateau phase (Ca2+ influx) is under the regulation of a G protein/cPLA2-dependent pathway.



View larger version (27K):
[in this window]
[in a new window]
 
Fig. 8. Effects of PLA2 inhibitor methyl arachidonyl fluorophosphate (MAFP) on H. pylori-induced [Ca2+]i changes in cultures of normal human gastric mucous epithelial cells. The cultures were preincubated for 30 min with MAFP, then treated with the appropriate H. pylori wild-type or isogenic strain (1 x 109 CFU/ml), and [Ca2+]i was recorded. We found no significant effect (P > 0.05) of MAFP on the wild-type (A) and vacA (B) H. pylori-induced [Ca2+]i peak change, whereas MAFP had a signifi-cant effect (P < 0.05) on the wild-type and vacA H. pylori-induced [Ca2+]i plateau change. Also, MAFP had no significant effect (P > 0.05) on the cagA (C)or picB/cagE-(D) induced [Ca2+]i peak change. Because the cagA and picB/cagE isogenic strains do not produce an [Ca2+]i plateau change, MAFP was without effect on this portion of the [Ca2+]i response (C and D). Data are from 9 independent experiments and are expressed as means ± SE; *P < 0.05 vs. control peak and plateau levels.

 


    DISCUSSION
 TOP
 ABSTRACT
 MATERIALS AND METHODS
 RESULTS
 DISCUSSION
 REFERENCES
 
Pathogenic bacteria have developed a variety of mechanisms to survive and interact with their respective host cells, where they exploit their respective host cell signaling pathways (11). H. pylori has also been shown to activate or use several different signaling pathways within the host gastric cell that eventually lead to the development of ulcers or gastric cancer (38, 57). However, the effect of H. pylori on intracellular Ca2+ signaling in normal human gastric epithelial cells has not been investigated. The present study is the first to describe the effects of H. pylori on the regulation of [Ca2+]i changes in this cell type. We found that wild-type H. pylori produced a dose-dependent biphasic [Ca2+]i change within primary human gastric mucous epithelial cells and in a nontransformed gastric mucous epithelial cell line (HFE-145 cells). The changes in [Ca2+]i by H. pylori were dependent on the presence of intact live bacteria, since bacterial sonicates or heat-killed bacteria produced no change in [Ca2+]i. The wild-type H. pylori-induced [Ca2+]i response was also found to consist of two phases, the first being the release of Ca2+ from intracellular Ca2+ stores (peak phase) followed by the activation of a Ca2+-influx mechanism (plateau phase).

In the present study, we also examined a role for the H. pylori vacA, cagA, and picB/cagE genes on intracellular Ca2+ signaling. The H. pylori VacA toxin has been shown to produce several membrane permeability events in gastric cells, and it is also an important virulence factor in the pathogenesis of peptic ulcer disease (36). However, from our studies we conclude that the H. pylori VacA toxin has no direct role in mediating H. pylori-induced [Ca2+]i changes. That is, we found no difference between our H. pylori wild-type strain and a vacA isogenic mutant in their abilities to produce an [Ca2+]i change. This finding is in contrast to other pathogens in which extracellular toxins have been shown to have a role in host cell Ca2+ signaling. For example, the pore-forming toxin aerolysin, from Aeromonas hydrophila, has been shown to activate G protein-dependent intracellular Ca2+ release in human granulocytes (24). In contrast to the vacA mutant, we found that the [Ca2+]i response was greatly reduced when the gastric cells were treated with either a cagA or picB/cagE isogenic mutant strain. Specifically, we found that the [Ca2+]i peak change was markedly reduced with the cagA and picB/cagE isogenic mutants, and these mutant stains did not generate the typical prolonged plateau phase as seen with the H. pylori wild-type strain or vacA mutant. In addition, the picB/cagE-induced [Ca2+]i peak response was found to be significantly lower than the cagA-induced [Ca2+]i peak response.

Role of signaling intermediates on H. pylori-induced [Ca2+]i changes. After identifying the initial H. pylori-induced [Ca2+]i response, the mechanistic components for each of the H. pylori-induced [Ca2+]i phases were examined by using different kinase or drug inhibitors. We found, for example, that the pretreatment of the gastric cells with the PLC inhibitor U-73122, and not the structural control U-73343 analog, attenuated the wild-type H. pylori-induced [Ca2+]i peak phase to near control levels. Even more effective was the Gi{alpha} protein inhibitor PTX, which completely reduced the H. pylori-induced [Ca2+]i peak phase to baseline control levels in all of the H. pylori wild-type and mutant strains tested. PTX pretreatment was also effective in reducing the wild-type and vacA mutant H. pylori-induced [Ca2+]i plateau (Ca2+ influx) phase. However, because the cagA and picB/cagE mutants produced no [Ca2+]i plateau phase, the use of PTX pretreatment with these mutants on [Ca2+]i plateau changes were redundant. The src kinase inhibitor PP2 was found to produce dose-dependent differential effects on H. pylori-induced [Ca2+]i changes. That is, low concentrations of PP2 were most effective in attenuating wild-type and vacA mutant H. pylori-induced [Ca2+]i plateau changes, with only high concentrations reducing H. pylori-induced [Ca2+]i peak changes. These data suggest that a range of src kinase activity is likely to control the final H. pylori-induced intracellular Ca2+ signal. We also found that pretreatment of gastric cells with the cytoplasmic PLA2 (cPLA2) inhibitor MAFP was able to reduce (but not to control levels) the H. pylori-induced [Ca2+]i plateau response in the gastric cells. In this regard, it has been shown the activity of cPLA2 is Ca2+ dependent and that the increase in cPLA2 activity will increase arachidonic acid, which can modulate Ca2+ influx (23). It is possible that the first H. pylori-induced phase of intracellular Ca2+ mobilization will secondarily activate cPLA2, which in turn could generate arachidonic acid and modulate Ca2+ influx (Fig. 9).



View larger version (45K):
[in this window]
[in a new window]
 
Fig. 9. Proposed model for wild-type H. pylori-induced Ca2+ signaling in normal gastric mucous epithelial cells. Wild-type and vacA H. pylori strains produce [Ca2+]i changes through activation of G protein-coupled PLC and PLA2. Activation of PLC leads to the formation of inositol trisphosphate (IP3) and diacylglycerol (DAG), and IP3 binds to its receptor (IP3R) on an intracellular Ca2+ store to release Ca2+. The H. pylori-induced intracellular Ca2+ increase can then stimulate Ca2+-dependent PLA2 to produce arachidonic acid (AA) regulating Ca2+ influx (gray arrows). It is also possible that the H. pylori-translocated CagA protein, which becomes phosphorylated by src kinases, will directly or indirectly control Ca2+ influx.

 

H. pylori, Ca2+ signaling, and host cell pathogenesis. It is now known that H. pylori can initiate multiple signaling pathways within the host gastric cell by using a variety of effector stimuli, ranging from small extracellular molecules, such as urease-generated ammonia, to the VacA toxin or the use of specialized injected molecules such as the CagA protein (57). As a focus for our own study, we chose to look at what role the VacA toxin, the CagA protein, and a functional type IV injection system may have on intracellular Ca2+ signaling in normal human gastric mucous epithelial cells. We also chose to use a buffered urea-free Ringer solution (pH 7.4) to help minimize the potential effects that H. pylori-generated urease activity or ammonia might have on the overall H. pylori-induced [Ca2+]i change (4). However, we cannot rule out in our study the contribution of other H. pylori-secreted/shed factors that may contribute to the overall [Ca2+]i response (29). In addition, some of the H. pylori extracellular shed/secreted proteins, such as HP0305, have been reported to have sequence homology to regulators of G protein signaling, which makes it possible that these proteins could modulate or contribute to the overall H. pylori host cell [Ca2+]i response (22). However, because H. pylori was able to increase [Ca2+]i within minutes after the addition of the bacteria, we believe that soon after bacteria adherence, certain signaling intermediates are immediately activated, such as G proteins and PLC, which were both found to be important in the H. pylori-induced [Ca2+]i peak change (Fig. 9). In other cell types, it is well established that agonists or pathogens can quickly increase PLC activity and the formation of inositol trisphosphate, which releases Ca2+ from intracellular Ca2+ stores (3). Our time-course and inhibitor studies suggest that H. pylori is likely to involve a similar PLC pathway that produced the characteristic rise and fall of [Ca2+]i observed within the first 15 min after the addition of bacteria. It should be emphasized again that our cagA isogenic mutant produced only a small [Ca2+]i peak response (and no [Ca2+]i plateau change) and that this cagA-induced peak [Ca2+]i change was further reduced to baseline [Ca2+]i levels by the PLC inhibitor U-73122. These data indicate that there may be CagA-dependent and CagA-independent pathways for PLC activation, but overall, increases in PLC activity along with the physical translocation of the CagA protein are likely to be the major contributing factors to the initial H. pylori-induced [Ca2+]i change. It is noteworthy that other studies (2) have shown that phosphorylated CagA protein can be detected as early as 15 min after the addition of H. pylori to gastric cells, which is well within the time course of our [Ca2+]i peak response.

Another facet of intracellular Ca2+ signaling is the potential for cross-talk between different receptor systems (9). For example, it has been reported that H. pylori can transactivate the EGFR (21, 62). Although the role of H. pylori transactivation of the EGFR and Ca2+ signaling was not examined in our study, it has been reported that Salmonella can transactivate the EGFR to produce an increase in [Ca2+]i that was important for bacterial entry (35). H. pylori can also activate adenylate cyclase and increase intracellular cAMP within AGS gastric cancer cells, and the H. pylori-induced cAMP increase is independent of the vacA, cagA, and cag PAI genes (63). In this regard, intracellular Ca2+ release has also been shown to be regulated by cAMP and PKA (3), suggesting that H. pylori is capable of activating multiple receptor systems that are in turn capable of coordinating host cell Ca2+ signaling.

Our study also suggests that the translocated CagA protein may be necessary for the continuation of the Ca2+ signal for the induction of a [Ca2+]i plateau (Ca2+ influx) change. That is, in addition to the inability of our cagA mutant to produce the [Ca2+]i peak phase, we also found that the src kinase inhibitor PP2 (which has been shown to block CagA protein phosphorylation; Ref. 50) was also capable of inhibiting the H. pylori-induced [Ca2+]i peak phase. It has been suggested that the ability of the CagA protein to perturb host cell functions is dependent on the number and sequences of tyrosine sites that are phosphorylated (15, 41). At this time we do not know to what degree the CagA protein has to be phosphorylated to induce the H. pylori [Ca2+]i changes.

Several studies have also implicated a link between an H. pylori-induced [Ca2+]i change and a biological response. That is, pretreatment of MKN45 gastric cancer cells with the intracellular Ca2+ chelator BAPTA was shown to completely block wild-type H. pylori-induced IL-8 secretion (32). It has also been reported that BAPTA was able to block H. pylori-induced arachidonic acid release that is involved in the production of prostaglandin E2 (40). Of interest, however, was the fact that the expression of the CagA protein was not important for the above-mentioned Ca2+-dependent H. pylori-induced IL-8 release (32), whereas the CagA protein was necessary for Ca2+-dependent H. pylori-induced arachidonic acid synthesis (40). One might propose that, depending on the final H. pylori-induced [Ca2+]i change, different signaling pathways could be activated based on a specific [Ca2+]i threshold. That is, even in the presence of a cagA mutant, which we have shown generates only a small [Ca2+]i peak change, this small [Ca2+]i response may be sufficient enough to release IL-8, but a larger [Ca2+]i threshold and the CagA protein are both needed for activation of the arachidonic acid/prostaglandin signaling pathway. In this context, it is also possible that the various components of the H. pylori-induced biphasic [Ca2+]i signal, i.e., the peak and plateau phases, may be utilized differently depending on the nature of the Ca2+-dependent signaling molecule within the host gastric cell. It also appears that differential signaling by H. pylori may hold true for other gastric host cell responses. That is, H. pylori-induced MAP kinase activity has also been reported to be induced in a "biphasic" manner over several hours (27). In addition, recent microarray transcriptional studies of H. pylori-treated AGS gastric cancer cells found that many H. pylori-induced signaling genes are transiently expressed within 1 h (14). It is also highly likely that there are other genes inside or outside the H. pylori cag PAI, as well certain structural components from H. pylori itself, that could participate in the H. pylori-induced [Ca2+]i response. For example, it has been suggested that the direct binding of the defective picB/cagE type IV injection apparatus to the plasma cell membrane itself is enough to activate other receptors, as well as translocate other unknown molecules through the type IV injection apparatus that can participate in host cell responses (51).

In summary, we found that H. pylori produces specific transient [Ca2+]i changes in normal human gastric mucous epithelial cells and that these H. pylori-induced [Ca2+]i changes could also be replicated in a nontransformed gastric mucous epithelial cell line (HFE-145 cells). A G protein/PLC-dependent pathway primarily regulated the H. pylori-induced intracellular Ca2+ release, whereas H. pylori-induced Ca2+ influx was under the control of a G protein-, src kinase-, and PLA2-dependent pathway (Fig. 9). Finally, we report that mutagenesis of picB/cagE and cagA genes (located within the cag PAI), but not the vacA gene, alters the capacity of H. pylori to produce a full [Ca2+]i response. For future studies, it will be important to look at other genes inside and outside the cag PAI to determine their effects on H. pylori-induced [Ca2+]i changes.


    ACKNOWLEDGMENTS
 
We thank Richard Bumgarden (Veterans Affairs Microbiology Lab) and Patrick Muller [Department of Surgery, Oregon Health Sciences University (OHSU)] for advice on growing H. pylori, and we thank Jodi Engstrom of the OHSU Department of Molecular Microbiology/Immunology for her great expertise in confocal microscopy. We also give special thanks to the chair of the OHSU Department of Molecular Microbiology/Immunology, Dr. Magdalene So, for her helpful discussions on bacterial pathogenesis.

Portions of these data were presented in abstract form at Digestive Disease Week, May 20–23, 2001, Atlanta, GA.

These studies were supported in part by the Medical Research Service of the Department of Veterans Affairs (to M. J. Rutten and C. W. Deveney) and by National Institutes of Health Grants R01-AI-39657 and DK-53623 (to T. L. Cover).


    FOOTNOTES
 

Address for reprint requests and other correspondence: M. J. Rutten, Oregon Health Sciences Univ., Dept. of Surgery/L223A, 3181 Sam Jackson Park Rd., Portland, OR 97201 (E-mail: ruttenm{at}ohsu.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.


    REFERENCES
 TOP
 ABSTRACT
 MATERIALS AND METHODS
 RESULTS
 DISCUSSION
 REFERENCES
 

  1. Adachi T, Nakashima S, Saji S, Nakamura T, and Nozawa Y. Possible involvement of pertussis toxin-sensitive G protein in hepatocyte growth factor-induced signal transduction in cultured rat hepatocytes: pertussis toxin treatment inhibits activation of phospholipid signaling, calcium oscillation, and mitogenactivated protein kinase. Hepatology 26: 295–300, 1997.[ISI][Medline]
  2. Asahi M, Azuma T, Ito S, Ito Y, Suto H, Nagai Y, Tsubokawa M, Tohyama Y, Maeda S, Omata M, Suzuki T, and Sasakawa C. Helicobacter pylori CagA protein can be tyrosine phosphorylated in gastric epithelial cells. J Exp Med 191: 593–602, 2000.[Abstract/Free Full Text]
  3. Ashby MC and Tepikin AV. Polarized calcium and calmodulin signaling in secretory epithelia. Physiol Rev 82: 701–734, 2002.[Abstract/Free Full Text]
  4. Athmann C, Zeng N, Kang T, Marcus EA, Scott DR, Rektorschek M, Buhmann A, Melchers K, and Sachs G. Local pH elevation mediated by the intrabacterial urease of Helicobacter pylori cocultured with gastric cells. J Clin Invest 106: 339–347, 2000.[Abstract/Free Full Text]
  5. Backert S, Moese S, Selbach M, Brinkmann V, and Meyer TF. Phosphorylation of tyrosine 972 of the Helicobacter pylori CagA protein is essential for induction of a scattering phenotype in gastric epithelial cells. Mol Microbiol 42: 631–644, 2001.[ISI][Medline]
  6. Backert S, Ziska E, Brinkmann V, Zimny-Arndt U, Fauconnier A, Jungblut PR, Naumann M, and Meyer TF. Translocation of the Helicobacter pylori CagA protein in gastric epithelial cells by a type IV secretion apparatus. Cell Microbiol 2: 155–164, 2000.[ISI][Medline]
  7. Basque JR and Menard D. Establishment of culture systems of human gastric epithelium for the study of pepsinogen and gastric lipase synthesis and secretion. Microsc Res Tech 48: 293–302, 2000.[ISI][Medline]
  8. Censini S, Lange C, Xiang Z, Crabtree JE, Ghiara P, Borodovsky M, Rappuoli R, and Covacci A. cag, A pathogenicity island of Helicobacter pylori, encodes type I-specific and disease-associated virulence factors. Proc Natl Acad Sci USA 93: 14648–14653, 1996.[Abstract/Free Full Text]
  9. Exton JH. Regulation of phosphoinositide phospholipases by hormones, neurotransmitters, and other agonists linked to G proteins. Annu Rev Pharmacol Toxicol 36: 481–509, 1996.[ISI][Medline]
  10. Fasano A. Toxins and the gut: role in human disease. Gut 50, Suppl 3: III9–III14, 2002.[Medline]
  11. Finlay BB. Interactions of enteric pathogens with human epithelial cells. Bacterial exploitation of host processes. Adv Exp Med Biol 412: 289–293, 1997.[ISI][Medline]
  12. Fischer W, Puls J, Buhrdorf R, Gebert B, Odenbreit S, and Haas R. Systematic mutagenesis of the Helicobacter pylori cag pathogenicity island: essential genes for CagA translocation in host cells and induction of interleukin-8. Mol Microbiol 42: 1337–1348, 2001.[ISI][Medline]
  13. Gewirtz AT, Rao AS, Simon PO Jr, Merlin D, Carnes D, Madara JL, and Neish AS. Salmonella typhimurium induces epithelial IL-8 expression via Ca2+-mediated activation of the NF-kappaB pathway. J Clin Invest 105: 79–92, 2000.[Abstract/Free Full Text]
  14. Guillemin K, Salama NR, Tompkins LS, and Falkow S. Cag pathogenicity island-specific responses of gastric epithelial cells to Helicobacter pylori infection. Proc Natl Acad Sci USA 99: 15136–15141, 2002.[Abstract/Free Full Text]
  15. Higashi H, Tsutsumi R, Fujita A, Yamazaki S, Asaka M, Azuma T, and Hatakeyama M. Biological activity of the Helicobacter pylori virulence factor CagA is determined by variation in the tyrosine phosphorylation sites. Proc Natl Acad Sci USA 99: 14428–14433, 2002.[Abstract/Free Full Text]
  16. Higashi H, Tsutsumi R, Muto S, Sugiyama T, Azuma T, Asaka M, and Hatakeyama M. SHP-2 tyrosine phosphatase as an intracellular target of Helicobacter pylori CagA protein. Science 295: 683–686, 2002.[Abstract/Free Full Text]
  17. Hofreuter D, Odenbreit S, and Haas R. Natural transformation competence in Helicobacter pylori is mediated by the basic components of a type IV secretion system. Mol Microbiol 41: 379–391, 2001.[ISI][Medline]
  18. Jones NL, Day AS, Jennings HA, and Sherman PM. Helicobacter pylori induces gastric epithelial cell apoptosis in association with increased Fas receptor expression. Infect Immun 67: 4237–4242, 1999.[Abstract/Free Full Text]
  19. Kawanishi T, Kato T, Asoh H, Uneyama C, Toyoda K, Momose K, Takahashi M, and Hayashi Y. Hepatocyte growth factor-induced calcium waves in hepatocytes as revealed with rapid scanning confocal microscopy. Cell Calcium 18: 495–504, 1995.[ISI][Medline]
  20. Keates S, Keates AC, Warny M, Peek RM Jr, Murray PG, and Kelly CP. Differential activation of mitogen-activated protein kinases in AGS gastric epithelial cells by cag+ and cag-Helicobacter pylori. J Immunol 163: 5552–5559, 1999.[Abstract/Free Full Text]
  21. Keates S, Sougioultzis S, Keates AC, Zhao D, Peek RM Jr, Shaw LM, and Kelly CP. cag+ Helicobacter pylori induce transactivation of the epidermal growth factor receptor in AGS gastric epithelial cells. J Biol Chem 276: 48127–48134, 2001.[Abstract/Free Full Text]
  22. Kim N, Weeks DL, Shin JM, Scott DR, Young MK, and Sachs G. Proteins released by Helicobacter pylori in vitro. J Bacteriol 184: 6155–6162, 2002.[Abstract/Free Full Text]
  23. Kramer RM and Sharp JD. Structure, function and regulation of Ca2+-sensitive cytosolic phospholipase A2 (cPLA2). FEBS Lett 410: 49–53, 1997.[ISI][Medline]
  24. Krause KH, Fivaz M, Monod A, and van der Goot FG. Aerolysin induces G-protein activation and Ca2+ release from intracellular stores in human granulocytes. J Biol Chem 273: 18122–18129, 1998.[Abstract/Free Full Text]
  25. Lin K, Sadee W, and Quillan JM. Rapid measurements of intracellular calcium using a fluorescence plate reader. Biotechniques 26: 318–326, 1999.[ISI][Medline]
  26. Meyer-ter-Vehn T, Covacci A, Kist M, and Pahl HL. Helicobacter pylori activates mitogen-activated protein kinase cascades and induces expression of the proto-oncogenes c-fos and c-jun. J Biol Chem 275: 16064–16072, 2000.[Abstract/Free Full Text]
  27. Mimuro H, Suzuki T, Tanaka J, Asahi M, Haas R, and Sasakawa C. Grb2 is a key mediator of Helicobacter pylori CagA protein activities. Mol Cell 10: 745–755, 2002.[ISI][Medline]
  28. Muallem S and Wilkie TM. G protein-dependent Ca2+ signaling complexes in polarized cells. Cell Calcium 26: 173–180, 1999.[ISI][Medline]
  29. Munzenmaier A, Lange C, Glocker E, Covacci A, Moran A, Bereswill S, Baeuerle PA, Kist M, and Pahl HL. A secreted/shed product of Helicobacter pylori activates transcription factor nuclear factor-kappa B. J Immunol 159: 6140–6147, 1997.[Abstract]
  30. Naumann M, Wessler S, Bartsch C, Wieland B, Covacci A, Haas R, and Meyer TF. Activation of activator protein 1 and stress response kinases in epithelial cells colonized by Helicobacter pylori encoding the cag pathogenicity island. J Biol Chem 274: 31655–31662, 1999.[Abstract/Free Full Text]
  31. Nebe B, Sanftleben H, Pommerenke H, Peters A, and Rychly J. Hepatocyte growth factor enables enhanced integrincytoskeleton linkage by affecting integrin expression in subconfluent epithelial cells. Exp Cell Res 243: 263–273, 1998.[ISI][Medline]
  32. Nozawa Y, Nishihara K, Peek RM, Nakano M, Uji T, Ajioka H, Matsuura N, and Miyake H. Identification of a signaling cascade for interleukin-8 production by Helicobacter pylori in human gastric epithelial cells. Biochem Pharmacol 64: 21–30, 2002.[ISI][Medline]
  33. Odenbreit S, Puls J, Sedlmaier B, Gerland E, Fischer W, and Haas R. Translocation of Helicobacter pylori CagA into gastric epithelial cells by type IV secretion. Science 287: 1497–1500, 2000.[Abstract/Free Full Text]
  34. Osada S, Saji S, Nakamura T, and Nozawa Y. Cytosolic calcium oscillations induced by hepatocyte growth factor (HGF) in single fura-2-loaded cultured hepatocytes: effects of extracellular calcium and protein kinase C. Biochim Biophys Acta 1135: 229–232, 1992.[ISI][Medline]
  35. Pace J, Hayman MJ, and Galan JE. Signal transduction and invasion of epithelial cells by S. typhimurium. Cell 72: 505–514, 1993.[ISI][Medline]
  36. Papini E, Zoratti M, and Cover TL. In search of the Helicobacter pylori VacA mechanism of action. Toxicon 39: 1757–1767, 2001.[ISI][Medline]
  37. Peek RM Jr. Microbes and Microbial Toxins: Paradigms for Microbial-Mucosal Interactions. IV. Helicobacter pylori strain-specific activation of signal transduction cascades related to gastric inflammation. Am J Physiol Gastrointest Liver Physiol 280: G525–G530, 2001.[Abstract/Free Full Text]
  38. Peek RM Jr and Blaser MJ. Helicobacter pylori and gastrointestinal tract adenocarcinomas. Nat Rev Cancer 2: 28–37, 2002.[Medline]
  39. Peek RM Jr, Blaser MJ, Mays DJ, Forsyth MH, Cover TL, Song SY, Krishna U, and Pietenpol JA. Helicobacter pylori strain-specific genotypes and modulation of the gastric epithelial cell cycle. Cancer Res 59: 6124–6131, 1999.[Abstract/Free Full Text]
  40. Pomorski T, Meyer TF, and Naumann M. Helicobacter pylori-induced prostaglandin E(2) synthesis involves activation of cytosolic phospholipase A(2) in epithelial cells. J Biol Chem 276: 804–810, 2001.[Abstract/Free Full Text]
  41. Puls J, Fischer W, and Haas R. Activation of Helicobacter pylori CagA by tyrosine phosphorylation is essential for dephosphorylation of host cell proteins in gastric epithelial cells. Mol Microbiol 43: 961–969, 2002.[ISI][Medline]
  42. Rhee SG. Regulation of phosphoinositide-specific phospholipase C. Annu Rev Biochem 70: 281–312, 2001.[ISI][Medline]
  43. Ribeiro CM, Reece J, and Putney JW Jr. Role of the cytoskeleton in calcium signaling in NIH-3T3 cells. An intact cytoskeleton is required for agonist-induced [Ca2+]i signaling, but not for capacitative calcium entry. J Biol Chem 272: 26555–26561, 1997.[Abstract/Free Full Text]
  44. Ridley AJ, Comoglio PM, and Hall A. Regulation of scatter factor/hepatocyte growth factor responses by Ras, Rac, and Rho in MDCK cells. Mol Cell Biol 15: 1110–1122, 1995.[Abstract]
  45. Romano M, Ricci V, Memoli A, Tuccillo C, Di Popolo A, Sommi P, Acquaviva AM, Del Vecchio Blanco C, Bruni CB, and Zarrilli R. Helicobacter pylori up-regulates cyclooxygenase-2 mRNA expression and prostaglandin E2 synthesis in MKN 28 gastric mucosal cells in vitro. J Biol Chem 273: 28560–28563, 1998.[Abstract/Free Full Text]
  46. Rutten MJ. Use of commercially available cell culture inserts for primary culture and electrophysiological studies of guinea pig gastric mucous epithelial cells. J Tissue Culture Methods 14: 235–246, 1992.
  47. Rutten MJ, Bacon KD, Marlink KL, Stoney M, Meichsner CL, Lee FP, Hobson SA, Rodland KD, Sheppard BC, Trunkey DD, Deveney KE, and Deveney CW. Identification of a functional Ca2+-sensing receptor in normal human gastric mucous epithelial cells. Am J Physiol Gastrointest Liver Physiol 277: G662–G670, 1999.[Abstract/Free Full Text]
  48. Rutten MJ, Campbell DR, Luttropp CA, Fowler WM, Hawkey MA, Boland CR, Krauss ER, Sheppard BC, Crass RA, Deveney KE, and Deveney CW. A method for the isolation of human gastric mucous epithelial cells for primary cell culture; A comparison of biopsy vs. surgical tissue. Methods Cell Sci 18: 269–281, 1996.
  49. Segal ED, Cha J, Lo J, Falkow S, and Tompkins LS. Altered states: involvement of phosphorylated CagA in the induction of host cellular growth changes by Helicobacter pylori. Proc Natl Acad Sci USA 96: 14559–14564, 1999.[Abstract/Free Full Text]
  50. Selbach M, Moese S, Hauck CR, Meyer TF, and Backert S. Src is the kinase of the Helicobacter pylori CagA protein in vitro and in vivo. J Biol Chem 277: 6775–6778, 2002.[Abstract/Free Full Text]
  51. Selbach M, Moese S, Meyer TF, and Backert S. Functional analysis of the Helicobacter pylori cag pathogenicity island reveals both VirD4-CagA-dependent and VirD4-CagA-independent mechanisms. Infect Immun 70: 665–671, 2002.[Abstract/Free Full Text]
  52. Sharma SA, Tummuru MK, Blaser MJ, and Kerr LD. Activation of IL-8 gene expression by Helicobacter pylori is regulated by transcription factor nuclear factor-kappa B in gastric epithelial cells. J Immunol 160: 2401–2407, 1998.[Abstract/Free Full Text]
  53. Smoot DT, Allen CR, Barnes P, Brown M, Phadnis S, Gold B, and Ashktorab H. Human gastric epithelial cell lines derived from primary cultures of normal gastric epithelial cells (Abstract). Gastroenterology 118: A540, 2000.
  54. Smoot DT, Sewchand J, Young K, Desbordes BC, Allen CR, and Naab T. A method for establishing primary cultures of human gastric epithelial cells. Methods Cell Sci 22: 133–136, 2000.[Medline]
  55. Stein M, Bagnoli F, Halenbeck R, Rappuoli R, Fantl WJ, and Covacci A. c-Src/Lyn kinases activate Helicobacter pylori CagA through tyrosine phosphorylation of the EPIYA motifs. Mol Microbiol 43: 971–980, 2002.[ISI][Medline]
  56. Stein M, Rappuoli R, and Covacci A. Tyrosine phosphorylation of the Helicobacter pylori CagA antigen after cag-driven host cell translocation. Proc Natl Acad Sci USA 97: 1263–1268, 2000.[Abstract/Free Full Text]
  57. Suerbaum S and Michetti P. Helicobacter pylori infection. N Engl J Med 347: 1175–1186, 2002.[Free Full Text]
  58. Takahashi A, Camacho P, Lechleiter JD, and Herman B. Measurement of intracellular calcium. Physiol Rev 79: 1089–1125, 1999.[Abstract/Free Full Text]
  59. Tummuru MK, Cover TL, and Blaser MJ. Mutation of the cytotoxin-associated cagA gene does not affect the vacuolating cytotoxin activity of Helicobacter pylori. Infect Immun 62: 2609–2613, 1994.[Abstract]
  60. Tummuru MK, Sharma SA, and Blaser MJ. Helicobacter pylori picB, a homologue of the Bordetella pertussis toxin secretion protein, is required for induction of IL-8 in gastric epithelial cells. Mol Microbiol 18: 867–876, 1995.[ISI][Medline]
  61. Wagner S, Enss ML, Cornberg M, Mix H, Schumann S, Kirchner G, Jahne J, Manns MP, and Beil W. Morphological and molecular characterization of human gastric mucous cells in long-term primary culture. Pflügers Arch 436: 871–881, 1998.[ISI][Medline]
  62. Wallasch C, Crabtree JE, Bevec D, Robinson PA, Wagner H, and Ullrich A. Helicobacter pylori-stimulated EGF receptor transactivation requires metalloprotease cleavage of HB-EGF. Biochem Biophys Res Commun 295: 695–701, 2002.[ISI][Medline]
  63. Wessler S, Rapp UR, Wiedenmann B, Meyer TF, Schoneberg T, Hocker M, and Naumann M. B-Raf/Rap1 signaling, but not c-Raf-1/Ras, induces the histidine decarboxylase promoter in Helicobacter pylori infection. FASEB J 16: 417–443, 2002.[Abstract/Free Full Text]




This Article
Abstract
Full Text (PDF)
All Versions of this Article:
285/1/G163    most recent
00257.2002v1
Alert me when this article is cited
Alert me if a correction is posted
Citation Map
Services
Email this article to a friend
Similar articles in this journal
Similar articles in ISI Web of Science
Similar articles in PubMed
Alert me to new issues of the journal
Download to citation manager
Search for citing articles in:
ISI Web of Science (3)
Google Scholar
Articles by Marlink, K. L.
Articles by Rutten, M. J.
Articles citing this Article
PubMed
PubMed Citation
Articles by Marlink, K. L.
Articles by Rutten, M. J.


HOME HELP FEEDBACK SUBSCRIPTIONS ARCHIVE SEARCH TABLE OF CONTENTS
Visit Other APS Journals Online
Copyright © 2003 by the American Physiological Society.