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Polymorphonuclear Oxidative Burst after Helicobacter pylori Water Extract Stimulation Is not Influenced by the Cytotoxic Genotype but Indicates Infection and Gastritis Grade

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Abstract H. pylori-associated gastric mucosal inflammation is characterized by the presence of polymorphonuclear (PMN) leukocyte infiltrate, which is more severe when the infecting strain is cagA positive. After appropriate stimuli, such as bacterial products, PMN release large amounts of oxygen derived free radicals and proteases, to kill the bacterium. H. pylori seems to be particularly resistant to the oxidative machinery of PMN, which can in turn damage the host gastric mucosa. We evaluated peripheral PMN oxidative burst response after stimulation with water extracts from cagA positive (WEcagA+) or negative (WEcagA−) H. pylori strains in infected (n=31) and non-infected patients (n=32) in comparison with healthy controls (n=16); the influence of gastric mucosal inflammatory infiltrate and activity grade on PMN oxidative burst were also assessed. PMN oxidative burst was measured by FACS analysis. H. pylori water extracts were obtained from bacterial culture. H. pylori genotype was determined by means of the polymerase chain reaction. The PMN oxidative burst in H. pylori infected patients was significantly higher than that in H. pylori negative or healthy controls, no differences being found when the results following WEcagA+ and WEcagA-stimulation were compared. The difference in PMN oxidative burst obtained after WEcagA− and E. coli (standard stimulus for PMN oxidative burst) stimulation discriminated H. pylori infected from non-infected patients with a sensitivity of 90 % and a specificity of 97 %. The grade of PMN oxidative burst correlated with PMN infiltration grade of the gastric mucosa. Our findings allow to conclude that PMN oxidative burst activation by H. pylori WE is species-but not strain-correlated. PMN priming, probably consequent to the action of soluble mediators released by mononuclear cells, makes PMN hyper-responsive to H. pylori products, thus favoring the release in the gastric mucosa of infected patients of large amounts of oxygen-derived free radicals, which are not enough to eliminate the infection, but may contribute to damaging the gastric mucosa itself. Peripheral PMN oxidative burst response to H. pylori WE might furthermore be of help in diagnosing H. pylori infection.
Title: Polymorphonuclear Oxidative Burst after Helicobacter pylori Water Extract Stimulation Is not Influenced by the Cytotoxic Genotype but Indicates Infection and Gastritis Grade
Description:
Abstract H.
pylori-associated gastric mucosal inflammation is characterized by the presence of polymorphonuclear (PMN) leukocyte infiltrate, which is more severe when the infecting strain is cagA positive.
After appropriate stimuli, such as bacterial products, PMN release large amounts of oxygen derived free radicals and proteases, to kill the bacterium.
H.
pylori seems to be particularly resistant to the oxidative machinery of PMN, which can in turn damage the host gastric mucosa.
We evaluated peripheral PMN oxidative burst response after stimulation with water extracts from cagA positive (WEcagA+) or negative (WEcagA−) H.
pylori strains in infected (n=31) and non-infected patients (n=32) in comparison with healthy controls (n=16); the influence of gastric mucosal inflammatory infiltrate and activity grade on PMN oxidative burst were also assessed.
PMN oxidative burst was measured by FACS analysis.
H.
pylori water extracts were obtained from bacterial culture.
H.
pylori genotype was determined by means of the polymerase chain reaction.
The PMN oxidative burst in H.
pylori infected patients was significantly higher than that in H.
pylori negative or healthy controls, no differences being found when the results following WEcagA+ and WEcagA-stimulation were compared.
The difference in PMN oxidative burst obtained after WEcagA− and E.
coli (standard stimulus for PMN oxidative burst) stimulation discriminated H.
pylori infected from non-infected patients with a sensitivity of 90 % and a specificity of 97 %.
The grade of PMN oxidative burst correlated with PMN infiltration grade of the gastric mucosa.
Our findings allow to conclude that PMN oxidative burst activation by H.
pylori WE is species-but not strain-correlated.
PMN priming, probably consequent to the action of soluble mediators released by mononuclear cells, makes PMN hyper-responsive to H.
pylori products, thus favoring the release in the gastric mucosa of infected patients of large amounts of oxygen-derived free radicals, which are not enough to eliminate the infection, but may contribute to damaging the gastric mucosa itself.
Peripheral PMN oxidative burst response to H.
pylori WE might furthermore be of help in diagnosing H.
pylori infection.

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