Effects were observed on the composition of the microbiota after 4 weeks as well as after 14 weeks. In the long-term feeding study the changes could be identified by PCA of the gel patterns produced by DGGE of PCR amplified 16S rRNA genes. In the short-term study, PCA did not reveal any
major changes, however a statistically significant decrease in the Bacteroides group was observed by qPCR. This indicates that even though short-term consumption introduced click here minor changes in the intestinal microbiota, long-term consumption was required for these changes to be substantial enough to be detected by the PCA. The observation that long-term consumption of whole apples influenced the rat intestinal microbiota (Figure 1) is consistent with previous studies showing effects of extraction juices, rich in dietary QNZ chemical structure fibers from apples, on gut microbes in
rats [5, 14]. In contrast to the extraction juices investigated by Sembries and coworkers, the clear and cloudy apple juices applied in the present study contained only very low amounts of dietary fibers and had no effect on the gut microbiota detectable by the methods applied. Addition of either 0.3, 3.3 or 7.0% of dry apple pectin to the diet caused overall changes in DGGE profiles of the cecal microbiota, which for the 7% pectin group was shown to include an increase in species belonging to the Gram-negative genus of Anaeroplasma, and the Gram-positive genera Anaerostipes and Roseburia, and a decrease in Gram-negative Alistipes and Bacteroides spp (Figure 2 and Figure 3). Previous studies have demonstrated the ability of some Bacteroides species to ferment pectin [15, 16] and shown an increase in the Bacteroides population after feeding rats with pectin related products [17]. In Florfenicol vitro fermentation studies have showed an increase in Bacteroides when low methylated pectin was used [18], but other fermentation studies failed to show any effect on this group [18, 19]. The discrepancies between the studies may be due to differences in pectin used and/or the fact that different Bacteroides populations were studied. Quantitative real-time
PCR (Figure 4a) using a primer set constructed based on the sequenced bands from the DGGE analysis (Figure 3) specified that three-fold less Bacteroides spp were present in samples from pectin-fed rats than in the control. Additionally, a more than four-fold increase in Clostridium coccoides, (corresponding to the Clostridium cluster XIVa) in the pectin-fed animals was showed (Figure 4d). Furthermore, samples from the pectin-fed animals contained four times as many genes https://www.selleckchem.com/products/Dasatinib.html encoding the butyryl-coenzyme A CoA transferase as the control samples (Figure 4e). This enzyme is known to be present in bacteria from the Clostridium Cluster XIVa, in strains in the Roseburia-Eubacterium rectale cluster, and in Faecalibacterium prausnitzii, which are known to be numerically important butyrate-producers in the human gut [20, 21].