Try using NEBNext RNA fragmentation buffer. We do a 3 min incubation and get a pretty good size distribution for 100 PE runs

Thank you! We have been quite succesful with NEB RNA fragmetation for pair end sequencing too.

It's just this time we are using Ambion kits and we need to use RNaseIII.

(1) I think you already under stand this, but you can't swap out RNAseIII digestion of RNA for heat/chemical fragmentation without altering your protocol! RNAseIII produces 5'-phosphate, 3'-hydroxyl ends -- exactly what RNA ligases need. heat/chemical fragmentation and most RNAses produce 3'-phosphate, 5'-hydroxyl ends.

(2) What is the average length of your RNA prior to RNAseIII digestion?

You might want to try an RNAseIII minus control reaction. That is, add all the reaction components, except RNAseIII (replace with water). Then do the normal incubation. If your RNA is still fragmenting, then it is contaminating RNAses in your RNA prep that are the problem, not the RNAseIII reaction.

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Phillip

Thanks for your help. Pls see replies below.