• Nuclease-free water
• Stem-loop reverse transcription primers
• qPCR primers
• (Optional) Synthetic RNA oligonucleotide corresponding to miRNA of interest
• Low molecular weight DNA markers (25bp DNA Step Ladder; Promega, cat. no. G4511, or similar)
• Ethidium bromide (Biorad, cat. no. 161-0433) ! Caution: suspected mutagen and carcinogen, handle with suitable gloves at all times.
• Nuclease free low gelling temperature agarose (Cambrex, cat. no. #50180 or similar)
• TAE (Sigma, cat. no. T6025, or similar. Alternatively, reconstitute from basic reagents)
• Reverse Transcriptase kit (ImProm-II; Promega, cat. no. A3802 or similar.) ! Critical: Other reverse transcription enzymes can be used, but the permissible lysis conditions should be empirically optimized.
• dNTPs (Bioline, cat. no. BIO-39027 or similar)
• 25 mM MgCl2 solution (Sigma-Aldrich, cat. no. M8266)
• RNase-Free DNase (RQ1; Promega, cat. no. M6101 or similar.)
• Triton X-100 (Biorad cat. no. 161-0407 or similar)
• Nonidet P40 (Roche cat. no. 11754599001 or similar) ! Critical: Other detergents such as Tween 20 may also be used. However, do NOT use sodium deoxycholate or sodium dodecyl sulfate as in our experience they will inhibit the RT.
• Phosphate-buffered saline (PBS)
• SsoFast EvaGreen Supermix (Biorad, cat. no. 172-5202 or other SYBR Green I-based qPCR mix) ! Critical: We recommend that hotstart polymerase mixes be used to minimize primer-dimer formation.