Meta-Analysis of Fecal Microbiota and Metabolites in Experimental Colitic Mice during the Inflammatory and Healing Phases.

The imbalance of gut microbiota is known to be associated with inflammatory bowel disease, but it remains unknown whether dysbiosis is a cause or consequence of chronic gut inflammation. In order to investigate the effects of gut inflammation on microbiota and metabolome, the sequential changes in gut microbiota and metabolites from the onset of colitis to the recovery in dextran sulfate sodium-induced colitic mice were characterized by using meta 16S rRNA sequencing and proton nuclear magnetic resonance (¹H-NMR) analysis. Mice in the colitis progression phase showed the transient expansions of two bacterial families including Bacteroidaceae and Enterobacteriaceae and the depletion of major gut commensal bacteria belonging to the uncultured Bacteroidales family S24-7, Rikenellaceae, Lachnospiraceae, and Ruminococcaceae. After the initiation of the recovery, commensal Lactobacillus members promptly predominated in gut while other normally abundant bacteria excluding the Erysipelotrichaceae remained diminished. Furthermore, ¹H-NMR analysis revealed characteristic fluctuations in fecal levels of organic acids (lactate and succinate) associated with the disease states. In conclusion, acute intestinal inflammation is a perturbation factor of gut microbiota but alters the intestinal environments suitable for Lactobacillus members.

Strengthening of the intestinal epithelial tight junction by Bifidobacterium bifidum.

Epithelial barrier dysfunction has been implicated as one of the major contributors to the pathogenesis of inflammatory bowel disease. The increase in intestinal permeability allows the translocation of luminal antigens across the intestinal epithelium, leading to the exacerbation of colitis. Thus, therapies targeted at specifically restoring tight junction barrier function are thought to have great potential as an alternative or supplement to immunology-based therapies. In this study, we screened Bifidobacterium, Enterococcus, and Lactobacillus species for beneficial microbes to strengthen the intestinal epithelial barrier, using the human intestinal epithelial cell line (Caco-2) in an in vitro assay. Some Bifidobacterium and Lactobacillus species prevented epithelial barrier disruption induced by TNF-α, as assessed by measuring the transepithelial electrical resistance (TER). Furthermore, live Bifidobacterium species promoted wound repair in Caco-2 cell monolayers treated with TNF-α for 48 h. Time course (1)H-NMR-based metabonomics of the culture supernatant revealed markedly enhanced production of acetate after 12 hours of coincubation of B. bifidum and Caco-2. An increase in TER was observed by the administration of acetate to TNF-α-treated Caco-2 monolayers. Interestingly, acetate-induced TER-enhancing effect in the coculture of B. bifidum and Caco-2 cells depends on the differentiation stage of the intestinal epithelial cells. These results suggest that Bifidobacterium species enhance intestinal epithelial barrier function via metabolites such as acetate.

Micelle formation of N-(1,1-dihydroperfluorooctyl)- and N-(1,1-dihydroperfluorononyl)-N,N,N-trimethylammonium chlorides.

Micelle formation of N-(1,1-dihydroperfluorooctyl)-N,N,N- and N-(1,1-dihydroperfluorononyl)-N,N,N-trimethylammonium chloride was investigated by analyzing the concentration dependence of the electric conductivity and of the activity of the counterion (Cl(-)) of the solution. The three micellization parameters for ionic surfactants, the micellization constant K(n), the micelle aggregation number n, and the number of counterions per micelle m, were determined by combination of electric conductivity and counterion concentration. The present analysis employed two slopes of the plots of specific conductivity against surfactant concentration below and above the critical micelle concentration and the mass action model of micelle formation. The aggregation numbers thus obtained were relatively small, while the degrees of counterion binding to the micelle (m/n) were found to be quite large, much larger than expected from the small aggregation numbers. Thermodynamical parameters of the micellization were evaluated from the temperature dependence of the three parameters, and the micellization of the fluorinated surfactant was found to be enthalpy-driven. A CF(2) group in the perfluorocarbon chain was found to be 1.44 times larger in hydrophobicity for micellization than a CH(2) group in the hydrocarbon chain.