Microarray & NGS: RNA QA Guidelines

RNA must be prepared and examined using the following assays.
 

1. Isolate total RNA using Trizol (GIBCO,BRL) and clean using RNeasy Kit (Qiagen). When using mRNA it must be isolated from total RNA using Oligotex columns (Qiagen) or oligo DT cellulose columns (GIBCO,BRL).
    
2. Measure the optical density (OD) of total RNA and mRNA samples including OD₂₆₀, OD₂₈₀, OD₂₆₀ /OD₂₈₀, and calculate the concentration (µg/µL) of your samples. Submit your samples with all the values above and the dilution factor that you used to take these readings.
   
   For each mRNA sample, please send at least 5 µg at a concentration of 0.5 - 2 µg/µL.
   
   For each total RNA sample, send 12 µg at a concentration 1 µg/µL.
   
   Users outside of UAlbany East Campus must send RNA samples in ethanol on dry ice or as a dry pellet.
    
3. Visualize each total RNA sample by running on an agarose gel containing 1.1% formaldehyde and photograph. Please attach a photo of the results (please remember to clearly label each lane with the sample label).
   
   Please label each tube of RNA sample prepared in DEPC-H2O carefully and complete all the details on the RNA submission form with the volume and concentration or µg amount for a dry pellet. This form must be faxed to 518-591-7211 or hand delivered to CRC building, Room 328, East Campus, Rensselaer, NY 12144.