2´-O-Methylation of Capped RNA (M0366)

Introduction

1. Combine capped RNA and nuclease-free water in a final volume of 16 μl. (Refer to step 1 in the notes on use).
   
   
2. Heat at 65°C for 5 minutes (Refer to step 2 in the notes on use).
   
   
3. Place tube on ice for 5 minutes.
   
   
4. Add the following components in the order specified:

   Denatured capped RNA (from above)	16.0 μl
   10X Capping Buffer	2.0 μl
   SAM (4 mM, dilute 32 mM stock to 4 mM)	1.0 μl
   mRNA Cap 2´-O-Methyltransferase (50 U/μl)	1.0 μl
   	20.0 μl

   
   Note: Use of RNase Inhibitor is recommended to enhance stability of RNA in the reaction. Add 0.5 μl of RNase Inhibitor (e.g., Murine RNase Inhibitor NEB #M0314 ) during reaction set up. Subtract the additional volume from the amount of H₂O used in the reaction.
   
   
5. Incubate at 37°C for 60 minutes (For RNA less than 200 nt long increase incubation time to 2 hours).
   
   
6. Proceed with purification of the RNA (if required) for downstream applications.