BACKGROUND: Little is known about levels of expression of Helicobacter pylori genes in the human host. We therefore developed a quantitative real-time reverse-transcriptase polymerase chain reaction (qRT-PCR) assay to measure transcript profiles of H. pylori in the human stomach. METHODS: In vivo expression of 16 genes on the cag pathogenicity island and of 18 putative virulence genes was quantitated by isolation of total RNA directly from infected human gastric mucosa. The results were compared with in vitro expression determined from H. pylori cells grown in culture. RESULTS: The highest levels of expression were found for cag1 and cag25 and for genes, such as urease and catalase, that may be important for bacterial homeostasis in the relatively hostile environment of the gastric mucosa. Transcript abundance, relative to 16S rRNA, was lower in vivo than in vitro, which suggests that H. pylori cells are in stationary phase in the gastric environment. This was particularly apparent for cagA. Since CagA is arguably of unique importance, in terms of interaction with the host, tight control of its in vivo expression might be particularly important. CONCLUSIONS: qRT-PCR is a powerful tool to measure gene expression in human or animal tissue that contains minute amounts of microbial mRNA, and the results reflect on the physiology of the pathogen in its natural host.
BACKGROUND: Little is known about levels of expression of Helicobacter pylori genes in the human host. We therefore developed a quantitative real-time reverse-transcriptase polymerase chain reaction (qRT-PCR) assay to measure transcript profiles of H. pylori in the human stomach. METHODS: In vivo expression of 16 genes on the cag pathogenicity island and of 18 putative virulence genes was quantitated by isolation of total RNA directly from infected humangastric mucosa. The results were compared with in vitro expression determined from H. pylori cells grown in culture. RESULTS: The highest levels of expression were found for cag1 and cag25 and for genes, such as urease and catalase, that may be important for bacterial homeostasis in the relatively hostile environment of the gastric mucosa. Transcript abundance, relative to 16S rRNA, was lower in vivo than in vitro, which suggests that H. pylori cells are in stationary phase in the gastric environment. This was particularly apparent for cagA. Since CagA is arguably of unique importance, in terms of interaction with the host, tight control of its in vivo expression might be particularly important. CONCLUSIONS: qRT-PCR is a powerful tool to measure gene expression in human or animal tissue that contains minute amounts of microbial mRNA, and the results reflect on the physiology of the pathogen in its natural host.
Authors: Francisco Avilés-Jiménez; Adriana Reyes-Leon; Erik Nieto-Patlán; Lori M Hansen; Juan Burgueño; Irma P Ramos; Margarita Camorlinga-Ponce; Hector Bermúdez; Juan M Blancas; Lourdes Cabrera; Rosa María Ribas-Aparicio; Jay V Solnick; Javier Torres-López Journal: Infect Immun Date: 2011-11-28 Impact factor: 3.441
Authors: Andrea R Castillo; Andrew J Woodruff; Lynn E Connolly; William E Sause; Karen M Ottemann Journal: Infect Immun Date: 2008-09-15 Impact factor: 3.441
Authors: Aleksandra W Debowski; Miriam Sehnal; Tingting Liao; Keith A Stubbs; Barry J Marshall; Mohammed Benghezal Journal: Appl Environ Microbiol Date: 2015-09-11 Impact factor: 4.792
Authors: Linda H Ta; Lori M Hansen; William E Sause; Olga Shiva; Aram Millstein; Karen M Ottemann; Andrea R Castillo; Jay V Solnick Journal: Front Cell Infect Microbiol Date: 2012-04-20 Impact factor: 5.293