Houseflies Are an Unlikely Reservoir or Vector for Helicobacter pylori

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Journal of Clinical Microbiology, September 1998, p. 2786-2788, Vol. 36, No. 9
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Houseflies Are an Unlikely Reservoir or Vector for Helicobacter pylori

Michael S. Osato,^* Kamran Ayub, Hong-Hahn Le, Rita Reddy, and David Y. Graham

Department of Medicine, Veterans Affairs Medical Center and Baylor College of Medicine, Houston, Texas

Received 17 December 1997/Returned for modification 8 February 1998/Accepted 12 June 1998

	ABSTRACT

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The route of transmission of Helicobacter pylori from individual to individual remains undefined. It has recently been reportedthat the domestic housefly, Musca domestica, when fed pure culturesof H. pylori, was able to harbor the organism in its midgut forup to 30 h (P. Grubel, S. Hoffman, F. K. Chong, N. A. Barstein,C. Mepani, and D. R. Cave, J. Clin. Microbiol. 35:1300-1303, 1997).Our investigation examined whether houseflies could acquire H.pylori from fresh human feces. Domestic houseflies (40 flies/group)were exposed for 24 h to feces from an H. pylori-positive volunteer,feces from an H. pylori-negative volunteer, or feces from an H.pylori-negative volunteer to which a known amount of viable H.pylori had been added. At various intervals, flies were sacrificedand the midguts were excised, homogenized, and plated in duplicateonto selective horse blood agar plates. All plates were incubatedunder microaerobic conditions at 37°C for 14 days. Emergent coloniespresumptive of H. pylori were picked and tested biochemicallyto confirm the identity as H. pylori. H. pylori was not recoveredfrom houseflies fed human feces either naturally infected or artificiallyinfected with H. pylori. These results suggest that the domestichousefly is not a vector for transmission or a reservoir for H.pylori infection.

	TEXT

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It is recognized that gastritis, gastric ulcer, duodenal ulcer, gastric carcinoma, and primary gastric B-cell lymphoma areall associated with Helicobacter pylori infection (2, 3,7, 11, 20, 35). The rate at which a population acquiresH. pylori infection is greater in developing than in industrializedcountries (1, 9, 11, 24, 26, 29, 30). Risk factorsfor an increased prevalence of H. pylori seropositivity includelower socioeconomic strata (31), overcrowded living conditions(27), large sibship size (32), substandard sanitation (28),the presence of regurgitated gastric contents in the environment(23), the presence of children in the family (25), the presenceof a single parent in the household (29), and the consumptionof contaminated drinking water (5, 19, 22). H. pylori infectionclusters in families with children (4, 25), but the factthat the genetically unrelated spouse is at high risk of infectionfurther confirms the importance of environmental factors in H.pylori infection. While the natural habitat of H. pylori is thehuman stomach, transmission has been linked to consumption ofwater in Peru and consumption of vegetables grown in regions wherehuman feces is used as fertilizer (18). These conditions maypredispose to infestation by flies and other pests. Two physiologicalfactors make the fly an ideal vector and reservoir for H. pyloriinfection. First, the mid-midgut of flies is acidic (much likethe human stomach) and could possibly be selective for H. pylori.Second, flies can only ingest liquefied meals and must regurgitatetheir enzyme-laden gastric contents onto food to facilitate feeding(6, 13, 33). The postulated mechanism by which flies disseminateinfection involves the selective concentration of H. pylori inthe fly's midgut following ingestion of fecal material and thenregurgitation of H. pylori-contaminated digestive fluids or defecationonto foodstuffs which are subsequently consumed by humans (6,13, 34). Grubel et al. (14, 15) showed that flies fedpure cultures of H. pylori harbored viable bacteria in their midgutsfor as long as 30 h after the initial exposure. While these resultsdemonstrated the prolonged retention of H. pylori in the fly'salimentary tract, the study design failed to replicate adequatelythe "natural" conditions consistent with poor sanitation. Datafrom studies of fecal cultures to recover H. pylori suggest thatthis organism is present at significantly lower concentrationsin nature than in a lawn of bacterial growth on an agar plate(19, 21, 22). However, the fly as a vector for the spreadof infectious disease has already been established, as in thetransmission of blinding chlamydial infection, cholera, shigellosis,and salmonellosis (8, 12, 13). We designed our study toascertain whether the domestic housefly, Musca domestica, couldacquire H. pylori from fresh human fecal specimens.

One hundred fifty domestic housefly (M. domestica) pupae (American Biological Supply Company, Gainesville, Fla.) were allowedto emerge at room temperature for 5 days and fed sterilized sugarwater ad libitum until used. Fresh fecal specimens were obtainedfrom both H. pylori-infected and noninfected volunteers. The infectedvolunteer had asymptomatic gastritis and had a positive ¹³C-urea breath test (Meretek, Houston, Tex.) and a positive HM-CAPenzyme-linked immunosorbent assay immunoglobulin G antibody test(Enteric Products, Inc., Westbury, N.Y.). The H. pylori-negativevolunteer had negative results for all diagnostic tests (¹³C-urea breath test, culture, histology, and HM-CAP enzyme-linkedimmunosorbent assay immunoglobulin G antibody test). The H. pyloriused for the inoculum was recovered from a frozen stock and platedon brain heart infusion agar (Difco Laboratories, Detroit, Mich.)plates containing 0.25% yeast extract (Difco) and 5% horse blood(Cocalico Biologicals, Inc., Reamstown, Pa.) (HBA). The plateswere incubated at 37°C for 3 days under 12% CO₂. A bacterial suspensionequivalent in density to a no. 5 McFarland standard (approximately1.5 × 10⁹ CFU/ml) was prepared in sterile saline. Three milliliters ofthe bacterial suspension was then added to approximately 50 gof fresh stool from the H. pylori-negative volunteer. The flieswere divided into three groups and placed in separate caged enclosures.Group 1 was exposed to feces from the H. pylori-positive volunteer,group 2 was exposed to feces from the H. pylori-negative volunteer,and group 3 was exposed to feces from the H. pylori-negative volunteerto which viable H. pylori was added. The exposure period for allgroups was 24 h. At various intervals postexposure (0, 6, 12,18, 24, 36, and 48 h), five flies from each group were sacrificed.The flies were immersed in 70% ethanol prior to dissection toclean the external surfaces of any adherent bacteria. The midgutsof the flies were excised and placed in cold cysteine medium untilcultured. The midgut tissue was homogenized and then plated induplicate on selective HBA plates containing 10-mg/liter nalidixicacid, 5-mg/liter trimethoprim, 3-mg/liter vancomycin, and 2-mg/literamphotericin B (16). All plates were incubated at 37°C under12% CO₂ for up to 14 days. Emergent colonies were picked and testedto identify H. pylori. Criteria used to confirm the identity ofthe selected isolates as H. pylori included colony morphologyon plated media, Gram stain and cellular morphology, and positivebiochemical reactions to catalase, urease, and oxidase tests.Both the CLOtest (Tri-Med Specialties, Inc., Lenexa, Kans.) andhpfast (GI Supply, Camp Hill, Pa.) rapid urease tests (RUTs) wereused to detect H. pylori in fly midgut tissue homogenates. Testingwas only performed on tissues collected up to 24 h after exposureto the fecal samples. All testing was performed as instructedby the manufacturer. Results were based on reading after incubationat 25°C for 24 h. A change in the color of the gel from yellowto either red (CLOtest) or green (hpfast) was indicative of apositive result. Any change in the pH indicator after 24 h ofincubation was read as a negative RUT result.

After we confirmed that M. domestica will not light on human stool, we removed all other sources of water. The flies werethen observed to light on and consume stool. H. pylori were notrecovered from the midgut tissue from any of the flies at anytime point (Table 1). Although other contaminating organismswere recovered (gram-positive cocci and bacilli), none of thecolonies resembling H. pylori and selected for subculture wereconfirmed as H. pylori following subsequent testing using biochemicaland morphologic criteria.

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TABLE 1. Microbiological recovery of H. pylori from the alimentary tracts of domestic houseflies after exposure to human stool for 24 h

Both the CLOtest and hpfast RUTs detected urease-producing bacteria in the remnant midgut tissues (Table 2). However, allalkaline responses occurred after 24 h of incubation at room temperature,suggesting the presence of non-H. pylori urease-positive organisms,and correlated with the presence of Proteus species in the fecalspecimen used as the negative control. None of the tissues fromflies exposed to feces from the H. pylori-positive volunteer producedan alkaline RUT result.

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TABLE 2. RUT results of housefly alimentary tract tissue after exposure to human stool for 24 h

M. domestica is a classical eusyanthropic fly species; i.e., it is trophically linked to the human habitat (12, 13). Originally,M. domestica was coprophagous and was adapted to feeding on theexcreta of ungulate mammals. Its presence in areas of decayingorganic matter and its repute as a vector for disease transmissionmade M. domestica a likely candidate as a vector for transmittingH. pylori infection. However, its extended association with humankindhas broadened its food range, and as a result, synanthropic populationsof this species have become trophically adapted, instead, to nonfecalhuman waste such as kitchen offal, decaying organic material,and decomposing proteins of animals. The original trophic adaptationof M. domestica to feces has gradually disappeared and is nowpreserved only in the subtropical asynanthropic populations ofM. domestica, e.g., M. domestica vicina (12, 13). Evidencefor this trophic shift was shown in our study when the recentlyemerged M. domestica would not alight on the fecal specimens unlessall other sources of nutrient were removed from the cage enclosures.

Our conclusions conflict with those of Grubel et al. (14, 15), who suggested that M. domestica could be a vector for thespread of infection and also serve as a reservoir for H. pylori.The fact that we were unable to recover H. pylori from housefliesthat were exposed to stool containing approximately 9 × 10⁷ CFU of H. pylori per g of stool indicates that even higher levelsof viable organisms must be present in nature to ensure positiverecovery from flies. Previous data have shown that such high levelsof viable H. pylori may not be present in the extragastric environment(5, 17, 19, 21, 34, 36). Therefore, it appears unlikelythat the domestic housefly is a vector for transmission of H.pylori infection or is an extragastric reservoir of H. pylori.

	ACKNOWLEDGMENTS

This work was supported by the Department of Veterans Affairs and the generosity of Hilda Schwartz.

	FOOTNOTES

^* Corresponding author. Mailing address: Gastroenterology Microbiology Laboratory, Veterans Affairs Medical Center (111-D),2002 Holcombe Boulevard, Rm. 3A-351, Houston, TX 77030. Phone:(713) 794-7901. Fax: (713) 790-1040. E-mail: mosato{at}bcm.tmc.edu.

REFERENCES

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Abstract
Text
References

1. Al-Moagel, M. A., D. G. Evans, M. E. Abdulghani, E. Adams, D. J. Evans, Jr., H. M. Malaty, and D. Y. Graham. 1990. Prevalence of Helicobacter (formerly Campylobacter) pylori infection in Saudi Arabia and comparison of those with and without upper gastrointestinal symptoms. Am. J. Gastroenterol. 85:944-948[Medline].

2. Blaser, M. J. 1992. Helicobacter pylori: its role in disease. Clin. Infect. Dis. 15:386-391[Medline].

3. Correa, P., J. Fox, E. Fontham, B. Ruiz, Y. P. Lin, D. Zavala, N. Taylor, D. Mackinley, E. De Lima, H. Portilla, and G. Zarama. 1990. Helicobacter pylori and gastric carcinoma. Serum antibody prevalence in populations with contrasting cancer risks. Cancer 66:2569-2574[Medline].

4. Drumm, B., G. I. Perez Perez, M. J. Blaser, and P. M. Sherman. 1990. Intrafamilial clustering of Helicobacter pylori infection. N. Engl. J. Med. 322:359-363[Abstract].

5. Enroth, H., and L. Engstrand. 1995. Immunomagnetic separation and polymerase chain reaction for detection of Helicobacter pylori in water and stool specimens. J. Clin. Microbiol. 33:2162-2165[Abstract].

6. Espinoza-Fuentes, F. P., and W. R. Terra. 1987. Physiological adaptations for digesting bacteria. Water fluxes and distribution of digestive enzymes in Musca domestica larval midgut. Insect Biochem. 6:809-817.

7. The Eurogast Study Group. 1993. An international association between Helicobacter pylori infection and gastric cancer. Lancet 341:1359-1362[Medline].

8. Fotedar, R., U. Banerjee, S. Singh, S. Shriniwas, and A. K. Verma. 1992. The housefly (Musca domestica) as a carrier of pathogenic microorganisms in a hospital environment. J. Hosp. Infect. 20:209-215[Medline].

9. Graham, D. Y., E. Adam, G. T. Reddy, J. P. Agarwal, R. Agarwal, D. J. Evans, Jr., H. M. Malaty, and D. G. Evans. 1991. Seroepidemiology of Helicobacter pylori in India: comparison of developing and developed countries. Dig. Dis. Sci. 36:1084-1088[Medline].

10. Graham, D. Y., H. M. Malaty, D. G. Evans, D. J. Evans, Jr., P. D. Klein, and E. Adam. 1991. Epidemiology of Helicobacter pylori in an asymptomatic population in the United States: effect of age, race and socioeconomic status. Gastroenterology 100:1495-1501[Medline].

11. Graham, D. Y. 1991. Helicobacter pylori: its epidemiology and its role in duodenal ulcer disease. J. Gastroenterol. Hepatol. 6:105-113[Medline].

12. Greenberg, B. 1965. Flies and disease. Sci. Am. 213:92-99[Medline].

13. Greenberg, B. 1971. Flies and diseases. Princeton University Press, Princeton, N.J.

14. Grubel, P., and D. R. Cave. 1997. Flies $---$ reservoirs and vectors of Helicobacter pylori. Fortschr. Med. 115:35-36[Medline].

15. Grubel, J. P., S. Hoffman, F. K. Chong, N. A. Burstein, C. Mepani, and D. R. Cave. 1997. Vector potential of houseflies (Musca domestica) for Helicobacter pylori. J. Clin. Microbiol. 35:1300-1303[Abstract].

16. Hachem, C. Y., J. E. Clarridge, D. G. Evans, and D. Y. Graham. 1995. Comparison of agar based media for primary isolation of Helicobacter pylori. J. Clin. Pathol. 48:714-716[Abstract/Free Full Text].

17. Hazell, S. L., H. M. Mitchell, M. Hedges, X. Shi, P. J. Hu, Y. Y. Li, A. Lee, and E. Reiss-Levy. 1994. Hepatitis A and evidence against the community dissemination of Helicobacter pylori via feces. J. Infect. Dis. 170:686-689[Medline].

18. Hopkins, R. J., P. A. Vial, C. Ferreccio, J. Ovalle, P. Prado, V. Sotomayor, R. G. Russell, S. S. Wasserman, and J. Morris, Jr. 1993. Seroprevalence of Helicobacter pylori in Chile: vegetables may serve as one route of transmission. J. Infect. Dis. 163:222-226.

19. Hulten, K., S. W. Han, H. Enroth, P. D. Klien, A. R. Opekun, R. H. Gilman, D. G. Evans, L. Engstrand, D. Y. Graham, and F. A. K. El-Zaatari. 1996. Helicobacter pylori in the drinking water in Peru. Gastroenterology 110:1031-1035[Medline].

20. Isaacson, P. G., and J. Spencer. 1993. Is gastric lymphoma an infectious disease? Hum. Pathol. 24:569-570[Medline].

21. Kelly, S. M., M. C. L. Pitcher, S. M. Farmery, and G. B. Gibson. 1994. Isolation of Helicobacter pylori from feces of patients with dyspepsia in the United Kingdom. Gastroenterology 107:1671-1674[Medline].

22. Klein, P. D., D. Y. Graham, A. Gaillour, A. R. Opekun, and E. O. Smith. 1991. Water source as risk factor for Helicobacter pylori infection in Peruvian children. Gastrointestinal Physiology Working Group. Lancet 337:1503-1506[Medline].

23. Langenberg, W., E. A. Rauws, J. H. Qudbier, and G. N. Tytgat. 1990. Patient-to-patient transmission of Campylobacter pylori infection by fiberoptic gastroduodenoscopy and biopsy. J. Infect. Dis. 161:507-511[Medline].

24. Malaty, H. M., D. G. Evans, D. J. Evans, Jr., and D. Y. Graham. 1992. Helicobacter pylori infection in Hispanics: comparison with Blacks and Whites of similar age and socioeconomic class. Gastroenterology 103:813-816[Medline].

25. Malaty, H. M., D. Y. Graham, P. D. Klein, D. G. Evans, E. Adam, and D. J. Evans, Jr. 1991. Transmission of Helicobacter pylori infection: studies in families of healthy individuals. Scand. J. Gastroenterol. 9:927-932.

26. Megraud, F., M. P. Brassens-Rabbë, F. Denis, A. Belbouri, and D. Q. Hoa. 1989. Seroepidemiology of Campylobacter pylori infection in various populations. J. Clin. Microbiol. 27:1870-1973[Abstract/Free Full Text].

27. Mendall, M. A., P. M. Goggin, N. Molineaux, J. Levy, T. Toosy, D. Strachan, and T. C. Northfield. 1992. Childhood living conditions and Helicobacter pylori seropositivity in adult life. Lancet 339:896-897[Medline].

28. Nowotty, U., and K. Heilmann. 1990. Epidemiology of Helicobacter pylori infection. Leber Magen Darm 20:183-186.

29. Perez-Perez, G. I., D. N. Taylor, L. Bodhidatta, J. Wongsrichanalai, W. B. Baze, B. E. Dunn, P. D. Echeverria, and M. J. Blaser. 1990. Seroprevalence of Helicobacter pylori infections in Thailand. J. Infect. Dis. 161:1237-1241[Medline].

30. Radhakrishnan, S., B. al Nakib, M. Kalaoui, and J. Patric. 1993. Helicobacter pylori-associated gastritis in Kuwait: endoscopy-based study in symptomatic and asymptomatic children. J. Pediatr. Gastroenterol. Nutr. 16:126-129[Medline].

31. Sitas, F., D. Forman, J. W. Yarnell, M. L. Burr, P. C. Elwood, S. Pedley, and K. J. Marks. 1991. Helicobacter pylori infection rates in relation to age and social class in a population of Welsh men. Gut 32:25-28[Abstract/Free Full Text].

32. Teh, B. H., J. T. Lin, W. H. Pan, S. H. Lin, L. Y. Wang, T. K. Lee, and C. J. Chen. 1994. Seroprevalence and associated risk factors of Helicobacter pylori infection in Taiwan. Anticancer Res. 14:1389-1392[Medline].

33. Terra, W. R., F. P. Espinoza-Fuentes, A. T. Ribeiro, and C. Ferreira. 1988. The larval midgut of the housefly (Musca domestica): ultrastructure, fluid fluxes and ion secretion in relation to the organization of digestion. J. Insect. Physiol. 34:463-472.

34. Thomas, J. E., G. R. Gibson, M. K. Darboe, A. Dale, and L. T. Weaver. 1988. Isolation of Helicobacter pylori from human feces. Lancet 340:1194-1195.

35. Tytgat, G. N. J., A. Lee, D. Y. Graham, M. F. Dixon, and T. Rokkas. 1993. The role of infectious agents in peptic ulcer disease. Gastroenterol. Int. 6:76-89.

36. van Zwet, A. A., J. C. Thijs, A. M. D. Kooistra-Smid, J. Schirm, and J. A. M. Snijder. 1994. Use of PCR with feces for detection of Helicobacter pylori infections in patients. J. Clin. Microbiol. 32:1346-1348[Abstract/Free Full Text].

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1.	Al-Moagel, M. A., D. G. Evans, M. E. Abdulghani, E. Adams, D. J. Evans, Jr., H. M. Malaty, and D. Y. Graham. 1990. Prevalence of Helicobacter (formerly Campylobacter) pylori infection in Saudi Arabia and comparison of those with and without upper gastrointestinal symptoms. Am. J. Gastroenterol. 85:944-948[Medline].
2.	Blaser, M. J. 1992. Helicobacter pylori: its role in disease. Clin. Infect. Dis. 15:386-391[Medline].
3.	Correa, P., J. Fox, E. Fontham, B. Ruiz, Y. P. Lin, D. Zavala, N. Taylor, D. Mackinley, E. De Lima, H. Portilla, and G. Zarama. 1990. Helicobacter pylori and gastric carcinoma. Serum antibody prevalence in populations with contrasting cancer risks. Cancer 66:2569-2574[Medline].
4.	Drumm, B., G. I. Perez Perez, M. J. Blaser, and P. M. Sherman. 1990. Intrafamilial clustering of Helicobacter pylori infection. N. Engl. J. Med. 322:359-363[Abstract].
5.	Enroth, H., and L. Engstrand. 1995. Immunomagnetic separation and polymerase chain reaction for detection of Helicobacter pylori in water and stool specimens. J. Clin. Microbiol. 33:2162-2165[Abstract].
6.	Espinoza-Fuentes, F. P., and W. R. Terra. 1987. Physiological adaptations for digesting bacteria. Water fluxes and distribution of digestive enzymes in Musca domestica larval midgut. Insect Biochem. 6:809-817.
7.	The Eurogast Study Group. 1993. An international association between Helicobacter pylori infection and gastric cancer. Lancet 341:1359-1362[Medline].
8.	Fotedar, R., U. Banerjee, S. Singh, S. Shriniwas, and A. K. Verma. 1992. The housefly (Musca domestica) as a carrier of pathogenic microorganisms in a hospital environment. J. Hosp. Infect. 20:209-215[Medline].
9.	Graham, D. Y., E. Adam, G. T. Reddy, J. P. Agarwal, R. Agarwal, D. J. Evans, Jr., H. M. Malaty, and D. G. Evans. 1991. Seroepidemiology of Helicobacter pylori in India: comparison of developing and developed countries. Dig. Dis. Sci. 36:1084-1088[Medline].
10.	Graham, D. Y., H. M. Malaty, D. G. Evans, D. J. Evans, Jr., P. D. Klein, and E. Adam. 1991. Epidemiology of Helicobacter pylori in an asymptomatic population in the United States: effect of age, race and socioeconomic status. Gastroenterology 100:1495-1501[Medline].
11.	Graham, D. Y. 1991. Helicobacter pylori: its epidemiology and its role in duodenal ulcer disease. J. Gastroenterol. Hepatol. 6:105-113[Medline].
12.	Greenberg, B. 1965. Flies and disease. Sci. Am. 213:92-99[Medline].
13.	Greenberg, B. 1971. Flies and diseases. Princeton University Press, Princeton, N.J.
14.	Grubel, P., and D. R. Cave. 1997. Flies $---$ reservoirs and vectors of Helicobacter pylori. Fortschr. Med. 115:35-36[Medline].
15.	Grubel, J. P., S. Hoffman, F. K. Chong, N. A. Burstein, C. Mepani, and D. R. Cave. 1997. Vector potential of houseflies (Musca domestica) for Helicobacter pylori. J. Clin. Microbiol. 35:1300-1303[Abstract].
16.	Hachem, C. Y., J. E. Clarridge, D. G. Evans, and D. Y. Graham. 1995. Comparison of agar based media for primary isolation of Helicobacter pylori. J. Clin. Pathol. 48:714-716[Abstract/Free Full Text].
17.	Hazell, S. L., H. M. Mitchell, M. Hedges, X. Shi, P. J. Hu, Y. Y. Li, A. Lee, and E. Reiss-Levy. 1994. Hepatitis A and evidence against the community dissemination of Helicobacter pylori via feces. J. Infect. Dis. 170:686-689[Medline].
18.	Hopkins, R. J., P. A. Vial, C. Ferreccio, J. Ovalle, P. Prado, V. Sotomayor, R. G. Russell, S. S. Wasserman, and J. Morris, Jr. 1993. Seroprevalence of Helicobacter pylori in Chile: vegetables may serve as one route of transmission. J. Infect. Dis. 163:222-226.
19.	Hulten, K., S. W. Han, H. Enroth, P. D. Klien, A. R. Opekun, R. H. Gilman, D. G. Evans, L. Engstrand, D. Y. Graham, and F. A. K. El-Zaatari. 1996. Helicobacter pylori in the drinking water in Peru. Gastroenterology 110:1031-1035[Medline].
20.	Isaacson, P. G., and J. Spencer. 1993. Is gastric lymphoma an infectious disease? Hum. Pathol. 24:569-570[Medline].
21.	Kelly, S. M., M. C. L. Pitcher, S. M. Farmery, and G. B. Gibson. 1994. Isolation of Helicobacter pylori from feces of patients with dyspepsia in the United Kingdom. Gastroenterology 107:1671-1674[Medline].
22.	Klein, P. D., D. Y. Graham, A. Gaillour, A. R. Opekun, and E. O. Smith. 1991. Water source as risk factor for Helicobacter pylori infection in Peruvian children. Gastrointestinal Physiology Working Group. Lancet 337:1503-1506[Medline].
23.	Langenberg, W., E. A. Rauws, J. H. Qudbier, and G. N. Tytgat. 1990. Patient-to-patient transmission of Campylobacter pylori infection by fiberoptic gastroduodenoscopy and biopsy. J. Infect. Dis. 161:507-511[Medline].
24.	Malaty, H. M., D. G. Evans, D. J. Evans, Jr., and D. Y. Graham. 1992. Helicobacter pylori infection in Hispanics: comparison with Blacks and Whites of similar age and socioeconomic class. Gastroenterology 103:813-816[Medline].
25.	Malaty, H. M., D. Y. Graham, P. D. Klein, D. G. Evans, E. Adam, and D. J. Evans, Jr. 1991. Transmission of Helicobacter pylori infection: studies in families of healthy individuals. Scand. J. Gastroenterol. 9:927-932.
26.	Megraud, F., M. P. Brassens-Rabbë, F. Denis, A. Belbouri, and D. Q. Hoa. 1989. Seroepidemiology of Campylobacter pylori infection in various populations. J. Clin. Microbiol. 27:1870-1973[Abstract/Free Full Text].
27.	Mendall, M. A., P. M. Goggin, N. Molineaux, J. Levy, T. Toosy, D. Strachan, and T. C. Northfield. 1992. Childhood living conditions and Helicobacter pylori seropositivity in adult life. Lancet 339:896-897[Medline].
28.	Nowotty, U., and K. Heilmann. 1990. Epidemiology of Helicobacter pylori infection. Leber Magen Darm 20:183-186.
29.	Perez-Perez, G. I., D. N. Taylor, L. Bodhidatta, J. Wongsrichanalai, W. B. Baze, B. E. Dunn, P. D. Echeverria, and M. J. Blaser. 1990. Seroprevalence of Helicobacter pylori infections in Thailand. J. Infect. Dis. 161:1237-1241[Medline].
30.	Radhakrishnan, S., B. al Nakib, M. Kalaoui, and J. Patric. 1993. Helicobacter pylori-associated gastritis in Kuwait: endoscopy-based study in symptomatic and asymptomatic children. J. Pediatr. Gastroenterol. Nutr. 16:126-129[Medline].
31.	Sitas, F., D. Forman, J. W. Yarnell, M. L. Burr, P. C. Elwood, S. Pedley, and K. J. Marks. 1991. Helicobacter pylori infection rates in relation to age and social class in a population of Welsh men. Gut 32:25-28[Abstract/Free Full Text].
32.	Teh, B. H., J. T. Lin, W. H. Pan, S. H. Lin, L. Y. Wang, T. K. Lee, and C. J. Chen. 1994. Seroprevalence and associated risk factors of Helicobacter pylori infection in Taiwan. Anticancer Res. 14:1389-1392[Medline].
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