0 GeneChip (Affymetrix) as described by the manufacturer Washing

0 GeneChip (Affymetrix) as described by the manufacturer. Washing and staining steps were performed in a Fluidics Station 400 (Affymetrix) according to the technical manual. Microarrays were scanned with the Affymetrix GeneChip Scanner 3000. Signals, detection calls and corresponding p-values of microarrays were calculated with MAS5.0/GCOS algorithms (default mode). Global normalization was used by scaling

the microarrays to a target intensity value of 100. Signal detection of probe sets and scaling factor for the individual microarrays, also correlation coefficients of signal intensities between duplicate microarrays permitted a comparison of the different data sets obtained for FDC networks (primary, early and late secondary FDC n=6), B cells (naïve, early and late GC B cells n=6) and BP3hi reticular cells (n=2) (Supporting Information Table 1) 44. To determine those genes which are specifically expressed in FDC PD 332991 an in silico subtraction approach was used. Recently, a similar approach was used to analyze the gene expression of the thymic stromal microenvironments https://www.selleckchem.com/products/LBH-589.html 45. Data sets obtained from dissected FDC networks were compared with those of sorted B cells. Parameters (signal log ratios, change calls and change p-values) provided by the algorithm for pair wise array comparison in the GCOS software

were obtained and group comparisons performed between the two groups of arrays using the High Performance Chip Data Analysis 24. In brief, the different parameters derived from signal calculation by the GCOS software were used to calculate mean, median and standard deviation of signal values and the percentage of “present” calls for each group. The mean of the Signal Log Ratio values and the percentage of change calls were used for pair wise comparison information of all possible comparisons. Finally, different Welch t-tests were performed and only p-values<0.05 were considered to be significant. Microarrays of BP3hi Interleukin-2 receptor reticular cells were analyzed as described above for FDC-specific genes (Fig. 1A, subtraction of B-cell transcriptome) and gene expression

compared with that of primary FDC using a modification of the High-Performance Chip Data Analysis. Hereby, duplicate microarrays of primary FDC and BP3hi reticular cells were compared (altogether four comparisons). On average, the signal intensities on FDC microarrays were 2.6-fold lower than on BP3hi microarrays. Only for those genes with >1.5- or<-1.5-fold differences from the mean value of 2.6 (Fig. 3) in at least three of the four comparisons were considered as significantly different. Gene expression profiles of macrophages (GSM106426, GSM106427, GSM106428, GSM117560, GSM117561), T cells (GSM44979, GSM44980, GSM44981, GSM44982), fibroblasts (GSM106139, GSM106141) and myoblasts (GSM126586, GSM126587) were obtained from the NCBI GEO data base.

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