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Infection and Immunity, November 2002, p. 6494-6498, Vol. 70, No. 11
0019-9567/02/$04.00+0     DOI: 10.1128/IAI.70.11.6494-6498.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

A Comparison of Murine and Human Immunoproteomes of Helicobacter pylori Validates the Preclinical Murine Infection Model for Antigen Screening

Department of Molecular Biology,¹ Central Core Facility Protein Analysis, Max-Planck-Institute for Infection Biology, Berlin, Germany²

Received 12 February 2002/ Returned for modification 8 April 2002/ Accepted 22 July 2002

	ABSTRACT

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Preclinical mouse infection models are widely used for Helicobacter vaccine development, but how well such models mimic important aspects of human infections is unknown. A comparison of Helicobacter pylori immunoproteomes of infected mice with previously reported patient data reveals a high agreement in the antigens recognized, suggesting that H. pylori in vivo protein composition and recognition by the host immune system are comparable in mice and humans. Murine Helicobacter models may thus be valid to screen antigens for human vaccination.

	TEXT

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The gram-negative bacterium Helicobacter pylori is a major causative agent of chronic active gastritis as well as gastric and duodenal ulcers. Moreover, it contributes to the development of gastric adenocarcinoma and mucosa-associated lymphoid tissue lymphoma. There has been extensive work to develop a Helicobacter vaccine. Most preclinical studies have been performed using mouse Helicobacter infection models because of the practical advantages of small-animal models (15). H. pylori does not normally colonize mice, but some mouse-adapted strains that can infect the murine stomach have been identified. Little work on in vivo gene expression of H. pylori has been done, but transcript levels of four important Helicobacter genes are similar for human biopsy samples and mouse samples (23). However, there is no detectable phase variation of Lewis antigen expression (27), and the important virulence factors CagA and VacA are lost during mouse colonization (11, 25). Pathological changes in the murine system include gastritis and in some cases follicle formation and even low-grade mucosa-associated lymphoid tissue lymphoma in the gastric mucosa (5, 17), whereas ulcer formation and adenocarcinoma have not been observed. Various vaccines that induce protective immunity against a Helicobacter challenge in the mouse model have been developed, but clinical trials have revealed a poor efficacy of such vaccines in humans (21), suggesting that murine Helicobacter models might be of limited value for vaccine development. The failure to transfer mouse vaccination strategies to humans could be due to potential differences in Helicobacter protein expression, antigen exposure to the host immune system, vaccine delivery, and protective immune mechanisms (8). To address the first two issues (protein composition and antigen exposure to the immune system,) which could particularly affect the screening of protective antigens, we compared the H. pylori immunoproteome in infected mice with previous data from infected human patients. Helicobacter antigens that induce specific antibody responses are obviously expressed in situ (4, 9, 26) and become exposed to the host immune system.

Female, 6- to 8-week-old, C57BL/6 mice were infected by three sequential oral inoculations of 5 x 10⁹ H. pylori SS1 (16) cells as described previously (6). Mice were killed at 14 weeks postinfection, and H. pylori colonization was assessed by plating of stomach samples. Sera were obtained prior to infection and by terminal bleeding. Alternatively, mice were subcutaneously immunized with 550 µg of H. pylori P76 sonicate mixed with incomplete Freud's adjuvant and given two booster doses on days 14 and 28.

H. pylori SS1 proteins were resolved in two dimensions on small gels (7.0 by 8.5 cm) and blotted as described previously (12). The blots were incubated with mouse sera at a dilution of 1:200 and stained using a peroxidase-coupled polyvalent goat antibody to mouse immunoglobulins (Sigma) at a dilution of 1:10,000 and enhanced chemiluminescence detection (ECL kit; Amersham). To increase the detection range, films were exposed for 5 to 30 min. The 35 spots with the highest postinfection seroreactivity but low to nondetectable preinfection seroreactivity (specifically recognized) and the 14 spots with the highest preinfection seroreactivity (cross-reactive) were analyzed by matrix-assisted laser desorption ionization-mass spectrometry peptide mass fingerprinting using a minimum sequence coverage of 30% (12). Coomassie brilliant blue spot staining intensities were quantified using the gel analysis program TOPSPOT.

Among the several hundred detectable protein species of H. pylori strain SS1 (12), only a few were recognized by preinfection sera (Fig. 1A). Sera from the same individual mice obtained at 14 weeks postinfection reacted with a much larger number of proteins, and the overall staining intensity was higher (Fig. 1B), which agrees with previously published human data (7, 14, 19, 20). Despite the facts that all mice were from a genetically homogenous inbred background and all were infected with the same cultures of a single H. pylori strain, there were marked differences between the recognition patterns of the individual sera. Immunostaining intensities of each of the 587 recognized protein species were determined in mice using a semiquantitative scale and average values from eight infected mice. Of the 35 species that were most strongly recognized by sera from infected mice but not by preinfection sera (specific recognition), 31 species corresponding to 21 different proteins could be identified (Table 1). In addition to these specifically recognized proteins, 14 protein species that were already strongly recognized prior to infection (cross-reactive) were analyzed, resulting in the identification of 13 protein species that corresponded to 10 proteins (Table 1).

View larger version (80K): [in this window] [in a new window]   FIG. 1. Typical immunoproteome of H. pylori strain SS1 as revealed by two-dimensional gel electrophoresis and immunoblotting with sera from the same mouse obtained either prior to infection (A) or 14 weeks after infection (B). The immunoblots were stained with a peroxidase-coupled antibody to mouse immunoglobulins followed by chemiluminescence detection. To enhance the detection of weakly cross-reactive antigens, film A was exposed for a longer time period (15 min) than film B (5 min). Abbreviations: SDS-PAGE, sodium dodecyl sulfate-polyacrylamide gel electrophoresis; IEF, isoelectric focusing.

Abundant Helicobacter proteins are overrepresented among the seroreactive antigens (Fig. 2), suggesting that dose-dependent responses may influence the recognition pattern. An alternative explanation is that spots containing rather small amounts of antigen might bind to a small amount of antibody and thus escape detection. However, on the basis of the least abundant species that was strongly recognized on the immunoblots (spot 59, a protein species yet to be identified), it can be estimated that this technical limitation probably affects only a minority of rare species (Fig. 2).

View larger version (17K): [in this window] [in a new window]   FIG. 2. Staining intensities of specifically recognized and cross-reactive (cross-r.) H. pylori antigens (top). The vertical lines represent the median values. For comparison, a histogram for the staining intensities of all detectable protein spots is shown at the bottom of the figure. Strongly immunogenic spots have higher staining intensities than those of all detectable spots (P < 0.001, t test), and cross-reactive species are significantly more intensely stained than specifically recognized species (P < 0.01, t test). a.u., arbitrary units.

It was thought that immunoblotting would be a good way to select promising vaccine antigen candidates (10, 14, 19, 20), although cellular instead of humoral immune responses seem to be relevant for protection against H. pylori at least in the mouse model (1, 3, 22). Interestingly, the combined data from infected mice (this study) and differentially immunized mice (this study) (10) show that all known protective antigens can be recognized by antibodies (Table 2), supporting a correlation between seroreactivity and cellular immune responses which could be related to the fact that optimal antibody responses depend on help from T cells. Interestingly, many protective H. pylori antigens, including the well-characterized urease, are cross-reactive in noninfected mice and patients, suggesting that specificity is not a prerequisite for protective efficacy. A comparison between the recognition patterns of infected (nonprotected) versus lysate-immunized (protected) mice might yield interesting information about individual, potentially protective antigens, but our preliminary data indicate a large number of differentially recognized antigens, suggesting that relevant candidates might be difficult to identify (not shown).

	FOOTNOTES

 
* Corresponding author. Mailing address: Abteilung Molekulare Biologie, Max-Planck-Institut für Infektionsbiologie, Schumannstraße 21/22, D-10117 Berlin, Germany. Phone: 49 30 28460 400. Fax: 49 30 28460 401. E-mail: meyer{at}mpiib-berlin.mpg.de.

Editor: E. I. Tuomanen

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