Labelling of aRNA Fourty micrograms of aRNA were labelled with Alexa Fluor dyes 647 or 555 (Invitrogen) respectively for control samples and for experimental samples, following the manufacturer’s protocol. Purification of coupled aRNA was performed by RNeasy purification system (Qiagen) and incorporation of dye was evaluated using Nanodrop. Before hybridization, coupled aRNA was fragmented using RNA fragmentation reagents (Ambion) following manufacturer’s protocol. Microarray hybridizations Microarray
slides were purchased from Biodiscovery LLC (Ann Arbor, MI, USA). MAP K10 expression microarray contains one probe per gene for a total of 4337 probes covering 99.7% of all genes with 4 probe replicates per array in a 3 Akt inhibitor arrays format per slides for a total of 7-Cl-O-Nec1 solubility dmso Depsipeptide 3x20K per slide. Each hybridization has been prepared following the Recommended Sample Preparation and Hybridization Protocols for Use with MYcroarrays (Biodiscovery LLC) with some modifications. Briefly, an hybridization solution of 220 μl (66 μl of 20X SSPE (3 M NaCl, 20 mM EDTA, 118.2 mM NaH2PO4, 81.8 mM Na2HPO4), formamide (10%), BSA (0.01 mg/ml), Tween-20 (0.01%), DTT (1 mM), manufacturer control oligos
1%, 10 μg of each target coupled-aRNA, RNAse free water until final volume) was prepared and pre-warmed Quinapyramine at 56°C before hybridization. All hybridizations were carried out in a water bath at 55°C for 18 h in OneArray
Sealed Hybridization Chambers (PhalanxBio Inc., Palo Alto, CA, USA) applicated to array slides following manufacturer’s protocol. After incubation, microarrays were washed at RT with two rounds of SSPE 1X with Dithiothreitol (DTT) (0.1 mM) for 2 min, a 30 s final wash of SSPE 0.25 X with DTT (0.1 mM) and dried with spray air before been immediately scanned. All scans were carried out with an Axon 4200A scanner (Molecular Devices) at 5 μm resolution with full dynamic range of signal intensities at 1–65,000 in two-color mode (635 nm and 532 nm filters). Microarrays data analysis Scanned images were obtained using the GenePix 6.0 software (Molecular devices). The signal intensity of each gene in both colors was calculated by the mean of median intensity of each replicate spot for each gene in the array giving an average for each gene extrapolated from 4 single spot signals. Median intensity values were corrected by background subtraction and negative corrected intensities were set to 10. Data were further normalized using the ratio-based setting for GenePix and gpr files belonging to hybridization signals analyzed by GenePix software were then loaded into the Multi Experiment viewer (MeV) from TM4 software suite for subsequent expression analysis.