Bacterial CagA protein compromises tumor suppressor mechanisms in gastric epithelial cells
Manikandan Palrasu, Elena Zaika, Wael El-Rifai, Monica Garcia-Buitrago, Maria Blanca Piazuelo, Keith T. Wilson, Richard M. Peek Jr., Alexander I. Zaika
Manikandan Palrasu, Elena Zaika, Wael El-Rifai, Monica Garcia-Buitrago, Maria Blanca Piazuelo, Keith T. Wilson, Richard M. Peek Jr., Alexander I. Zaika
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Research Article Gastroenterology

Bacterial CagA protein compromises tumor suppressor mechanisms in gastric epithelial cells

Abstract

Approximately half of the world’s population is infected with the stomach pathogen Helicobacter pylori. Infection with H. pylori is the main risk factor for distal gastric cancer. Bacterial virulence factors, such as the oncoprotein CagA, augment cancer risk. Yet despite high infection rates, only a fraction of H. pylori–infected individuals develop gastric cancer. This raises the question of defining the specific host and bacterial factors responsible for gastric tumorigenesis. To investigate the tumorigenic determinants, we analyzed gastric tissues from human subjects and animals infected with H. pylori bacteria harboring different CagA status. For laboratory studies, well-defined H. pylori strain B128 and its cancerogenic derivative strain 7.13, as well as various bacterial isogenic mutants were employed. We found that H. pylori compromises key tumor suppressor mechanisms: the host stress and apoptotic responses. Our studies showed that CagA induces phosphorylation of XIAP E3 ubiquitin ligase, which enhances ubiquitination and proteasomal degradation of the host proapoptotic factor Siva1. This process is mediated by the PI3K/Akt pathway. Inhibition of Siva1 by H. pylori increases survival of human cells with damaged DNA. It occurs in a strain-specific manner and is associated with the ability to induce gastric tumor.

Authors

Manikandan Palrasu, Elena Zaika, Wael El-Rifai, Monica Garcia-Buitrago, Maria Blanca Piazuelo, Keith T. Wilson, Richard M. Peek Jr., Alexander I. Zaika

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Figure 5

XIAP ubiquitinates Siva1 protein in H. pylori–infected cells.

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XIAP ubiquitinates Siva1 protein in H. pylori–infected cells. (A) Weste...
(A) Western blot analysis of Siva1, XIAP, pXIAP(S87), and Cbl-b proteins in AGS cells transfected with the indicated siRNA or scrambled control siRNA and treated as shown at the top of the panel. Low and high exposures are shown. (B) Western blot analysis of Siva1 protein ubiquitination in AGS cells treated as indicated at the top of the panel. Ubiquitination of Siva1 protein was analyzed after its immunoprecipitation with Siva1 antibody. Immunoprecipitation with mouse IgG was used as a control (lane 7). (C) Western blot analysis of XIAP protein phosphorylation at serine 87 after coculture of AGS cells with the indicated H. pylori strains for 4 hours. Each experiment was repeated 3 times, representative data are shown. Brackets indicate low and high exposures of Western blot images.