To provide insight in the molecular basis for intestinal host-microbe interactions, we determined the genome-wide transcriptional response of human intestinal epithelial cells following exposure to cells of Bifidobacterium breve. To select an appropriate test system reflecting inflammatory conditions, the responsiveness to TNF-α was compared in T84, Caco-2 and HT-29 cells. The highest TNF-α response was observed in HT-29 cells and this cell line was selected for exposure to the B. breve strains M-16V, NR246 and UCC2003. After one hour of bacterial pre-incubation followed by two hours of additional TNF-α stimulation, B. breve M-16V (86%), but to a much lesser extent strains NR246 (50%) or UCC2003 (32%), showed a strain-specific reduction of the HT-29 transcriptional response to the inflammatory treatment. The most important functional groups of genes that were transcriptionally suppressed by the presence of B. breve M-16V, were found to be involved in immune regulation and apoptotic processes. About 54% of the TNF-α induced genes were solely suppressed by the presence of B. breve M-16V. These included apoptosis-related cysteine protease caspase 7 (CASP7), interferon regulatory factor 3 (IRF3), amyloid beta (A4) precursor proteinbinding family A member 1 (APBA1), NADPH oxidase (NOX5), and leukemia inhibitory factor receptor (LIFR). The extracellular IL-8 concentration was determined by an immunological assay but did not change significantly, indicating that B. breve M-16V only partially modulates the TNF-α pathway. In conclusion, this study shows that B. breve strains modulate gene expression in HT-29 cells under inflammatory conditions in a strain-specific way.
Bifidobacterium breve – HT-29 cell line interaction: modulation of TNF-α induced gene expression
R. Boesten Related information
1 Microbiology Department, TNO Quality of Life, Utrechtseweg 48, 3704 HE, Zeist, the Netherlands
2 Laboratory of Microbiology, Wageningen University, Dreijenplein 10, 6703 HB, Wageningen, the Netherlands
, F. Schuren Related information2 Laboratory of Microbiology, Wageningen University, Dreijenplein 10, 6703 HB, Wageningen, the Netherlands
1 Microbiology Department, TNO Quality of Life, Utrechtseweg 48, 3704 HE, Zeist, the Netherlands
, L. Willemsen Related information3 Utrecht Institute of Pharmaceutical Sciences, Division of Pharmacology, Utrecht University, Universiteitsweg 99, 3584 CG Utrecht, the Netherlands
, A. Vriesema Related information4 Danone Research, Centre for Specialised Nutrition, Bosrandweg 20, 6704 PH, Wageningen, the Netherlands
, J. Knol Related information4 Danone Research, Centre for Specialised Nutrition, Bosrandweg 20, 6704 PH, Wageningen, the Netherlands
, W. De Vos Related information2 Laboratory of Microbiology, Wageningen University, Dreijenplein 10, 6703 HB, Wageningen, the Netherlands
5 Department of Veterinary Biosciences, Helsinki University, Sjöberginkatu 2, 00014 Helsinki, Finland
5 Department of Veterinary Biosciences, Helsinki University, Sjöberginkatu 2, 00014 Helsinki, Finland
Beneficial Microbes: 2
(2)- Pages: 115 - 128
Published Online: June 22, 2011
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