First Strand cDNA Synthesis (Standard Protocol) (NEB #M0253)

If denaturation of template RNA is desired, use the following protocol.
  1. Mix RNA sample and primer d(T)23VN in a sterile RNase-free microfuge tube.
     
    COMPONENT VOLUME
    Total RNA up to 1 µg*
    d(T)23VN (50 µM) or Random Primer Mix (60 µM) 2 µl
    10 mM dNTP 1 µl
    Nuclease-free H2O To a total volume of 10 µl

     
  2. Denature sample RNA/primer for 5 minutes at 65°C. Spin briefly and put promptly on ice.
  3. Add the following components
     
  4. COMPONENT VOLUME
    10X M-MuLV buffer 2 µl
    M-MuLV RT (200 U/µl) 1 µl
    RNase Inhibitor (40 U/µl) 0.2 µl
    Nuclease-free H2O 6.8 µl

     
  5. Incubate the 20 μl cDNA synthesis reaction at 42°C** for one hour. If Random Primer Mix is used, an incubation step at 25°C for 5 minutes is recommended before the 42°C incubation.
  6. Inactivate the enzyme at 65°C for 20 minutes. The cDNA product should be stored at -20°C. In general, the volume of cDNA product should not exceed 1/10 of the PCR reaction volume.

* 1 ng-1 µg total RNA or 50 pg-100 ng poly(A)-RNA
** M-MuLV Reverse Transcriptase can be used at 37°–42°C.