The identification was further confirmed by comparing mass spectra of all compounds with those contained in available databases (NIST version 2005 and Wiley version 1996) and in literature [41]. Quantitative data of the identified compounds were obtained by interpolation of the C188-9 purchase relative areas versus the internal standard area, in calibration curves built with pure reference compounds. The concentration Belinostat of volatile compounds, for which there were no pure references, was obtained by using the same calibration graphs of the compounds with the most similar chemical structure. Statistical analyses For each subject, variations of the DGGE profiles related to the
time points T0 and T1 were analyzed by Pearson correlation. Significant differences in the intensity of each DGGE band among all fecal samples were searched by using Mann-Whitney U-test. Mann-Whitney U-test was also used to analyze differences in total rrn operons of target genera and species and to determine metabolites significantly affected by the synbiotic food intake. A P value
below 0.05 was considered statistically significant. Metabolites with a P value below 0.05 were then used in further multivariate analysis. These selected learn more metabolites formed a matrix containing two kinds of information: the effects of the synbiotic food intake (within-individual variability) and the natural differences between individuals (between-individuals variability). These two kinds of information were separated following the method of Jansen et al. [59]. A CAP analysis was then performed on the within-individual variability Prostatic acid phosphatase matrix [60]. The CAP constrained ordination procedure can be summarized as follows: the data were reduced by performing
a principal coordinate analysis (PCO) on the parameters using a dissimilarity measure based on Euclidean distances; an appropriate number of PCOs were chosen non-arbitrarily, which maximize the number of observations correctly classified [61, 60]. The robustness of the model obtained was established by a 4-fold cross validation method, repeatedly leaving out a fourth of the samples and predicting them back into the model [62]. Finally a traditional canonical analysis on the first three PCOs was performed. The hypothesis of no significant difference in multivariate location among the groups was tested by using a permutation test based on 9999 permutations. Statistical analyses were performed using the software SigmaStat (Systat Sofware Inc., San Jose, CA) and the package Canoco for Windows 4.5 (Microcomputer Power, Ithaca, NY). Electronic supplementary material Additional file 1: Metabolites detected by GC-MS/SPME analysis. Metabolites were identified and quantified (mg/kg) in stool samples collected from 20 volunteers before (T0) and after (T1) the synbiotic food intake. (DOC 281 KB) Additional file 2: Confusion matrix.