RNA Detection

3. Second strand synthesis oligo 5^0 - GTTCAGAGTTCTACA
   GTCCGACGATCNNNNNN-3^0.
   The underlined portion corresponds to Illumina 5^0 adapter
   sequence vital for PCR amplification.


4. 10Klenow Buffer: 500 mM Tris–HCl pH 7.5, 100 mM
   MgCl 2 , 10 mM DTT, and 0.5 mg/mL BSA. Store buffer at
    20 C.


5. S3 master mix (per sample):12μL nuclease-free water, 10μL
   10 Klenow Buffer 5μL 10 mM dNTPs, and 10μL10μM
   second strand synthesis oligo.

2.7 PCR
Amplification and
Size-Selection of
Libraries

1. GoTaq Green 2PCR Master Mix (Promega).


2. 10μM5^0 PCR primer
   50 - AATGATACGGCGACCACCGAGATCTACACGTTCA
   GAGTTCTACAGTCCGA-3^0


3. 10μM3^0 Barcoded PCR Primer
   5-CAAGCAGAAGACGGCATACGAGATNNNNNNGTG
   ACTGGAGTTCCTTGGCACCCGAGAATTCCA- 30. The
   NNNNNNrepresents the unique barcode. Use a unique bar-
   code for each sample.


4. 80% ethanol (seeNote 3).

3 Methods

This protocol requires that the relevant RBP–PUP fusion proteins

already be engineered and introduced into cells. Upon request, we

provide a kit that includes plasmids that encode the PUP-2 open-

reading frame, free of charge to any academic lab.

3.1 Isolate Total RNA
fromS. cerevisiae

Isolate total RNA from yeast in completely denaturing conditions

(seeNote 4).

Timing:steps 3– 21 : 1.5–2 h;steps 22– 31 : 3–4 h.

1. Place 25 mL ofA 660 ~ 0.5–0.8 cultures on ice for 5 min.


2. Harvest cultures by centrifugation at 1900 rcf for 5 min at
   4 C.


3. Wash yeast pellets once with 40 mL of ice-cold water.


4. Resuspend yeast in 500μL RNA ISO buffer.


5. Add ~200μL of acid-washed beads.


6. Add 500μL of phenol–chloroform–isoamyl alcohol.


7. Vortex for 20 s at room temp., then incubate for 20 s on ice.
   Repeat for a total of ten cycles.


8. Split into two tubes. Each sample is now in two tubes.

RNA Tagging Library Preparation 459