Physiological concentrations of butyrate favorably modulate genes of oxidative and metabolic stress in primary human colon cells |
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| Authors: | Sauer Julia Richter Konrad Klaus Pool-Zobel Beatrice Louise |
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| Institution: | 1. Division of Applied Life Sciences, Graduate School of Life and Environmental Sciences, Kyoto Prefectural University, Shimogamo-Hangi, Sakyo, Kyoto 606-8522, Japan;2. Horticultural Division, Kyoto Prefectural Agriculture, Forestry and Fisheries Technology Center, Amarube, Kameoka, Kyoto 621-0806, Japan;3. Department of Microbiology, Faculty of Pharmacy, Mahidol University, 447 Sri Ayuthaya Rd., Bangkok 10400, Thailand;4. Division of Postharvest Technology, School of Bioresources and Technology, King Mongkut''s University of Technology Thonburi, 49 Soi Thian Thale 25, Bang Khun Thain-Chai Thale Rd., Tha Kham, Bang Khun Thain, Bangkok 10150, Thailand;5. Department of Agricultural Science, Kagoshima University, Korimoto 1-21, Kagoshima 890-0065, Japan;6. Department of Biochemical Science and Technology, Kagoshima University, Korimoto 1-21, Kagoshima 890-0065, Japan;1. Department of Ambulatory Care and Community Medicine, University of Lausanne, Lausanne, Switzerland;2. Department of General Internal Medicine, Bern University Hospital, Bern, Switzerland;3. Clinical Trials Unit Bern, Department of Clinical Research, Institute of Social and Preventive Medicine, University of Bern, Bern, Switzerland;4. Department of Internal Medicine, University Hospital, Lausanne, Switzerland |
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| Abstract: | Butyrate, a metabolite of gut flora-mediated fermentation of dietary fibre, was analysed for effects on expression of genes related to oxidative stress in primary human colon cells. An induction of detoxifying, antioxidative genes is expected to contribute to dietary chemoprevention. Cells were treated with butyrate (3.125-50 mM; 0.5-8 h), and kinetics of uptake and survival were measured. Gene expression was determined with a pathway-specific cDNA array after treating colon epithelium stripes with nontoxic doses of butyrate (10 mM, 12 h). Changes of hCOX-2, hSOD2 and hCAT expression were confirmed with real-time polymerase chain reaction (PCR) and by measuring catalase-enzyme activity. Primary colon cells consumed 1.5 and 0.5 mM butyrate after 4- and 12-h treatment, respectively. Cell viability was not changed by butyrate during 0.5-2-h treatment, whereas cell yields decreased after 1 h. Metabolic activity of remaining cells was either increased (4 h, 50 mM) or retained at 97% (8 h, 50 mM). Expression of hCAT was enhanced, whereas hCOX-2 and hSOD2 were lowered according to both array and real-time PCR analysis. An enhanced catalase-enzyme activity was detected after 2 h butyrate treatment. Healthy nontransformed colon cells well tolerated butyrate (50 mM, 2 h), and lower concentrations (10 mM, 12 h) modulated cyclooxygenase 2 (COX-2) and catalase genes. This points to a dual role of chemoprotection, since less COX-2 could reduce inflammatory processes, whereas more catalase improves detoxification of hydrogen peroxide (H(2)O(2)), a compound of oxidative stress. Changes of this type could reduce damaging effects by oxidants and protect cells from initiation. |
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