RNA Detection

Important: Following the PCR, do not open PCR tubes in

same room where iCLIP library preparations (i.e., all steps

before step 8 of Subheading3.11) were carried out. All

post-PCR analysis and storage needs to be carried out in

separate room to avoid amplicon contamination.

8. Assemble the XCell III gel system according to manufacturer’s
   instructions using a 6% TBE gel and TBE running buffer.


9. Add 2μLof6loading dye to each PCR sample and 10μLof
   1:30 low molecular weight marker. Load 12μL of samples/
   ladder into gel wells.


10. Run gel for 30 min at 180 V


11. Remove gel from cassette and stain for 5 min in SYBR Safe in
    TBE buffer. Visualize using appropriate imager (Fig.4a). The
    P5/P3 primers account for 128 nt of PCR product. Appropri-
    ate PCR band sizes are therefore:

Fig. 4cDNA library PCRs. (a) Example of final library PCR (steps 13– 17 of Subheading3.11) showing low,
medium, and high bands. Both a low RNase sample and a no UV control sample are shown. (b) Example of a
cDNA library amplified with different PCR cycle numbers.Red boxesindicate secondary spurious products that
migrate at a higher molecular weight to the expected products

446 Christopher R. Sibley