Ligation of 3´ and 5´ Adaptors (E6120)
Overview
Starting Material:
1–10 μg total RNA. Alternatively, previously isolated small RNA from 1–10 μg total RNA can be used as starting material.
Protocol
- Mix the following components in a sterile PCR tube:
Input RNA: 1–6 μl
3´ SR Adaptor 1: 1 μl
Nuclease-free Water: variable
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Total volume: 7 μl - Incubate in a preheated thermal cycler for 2 minutes at 70°C.
- Transfer tube to ice.
- Add the following components:
3´ Ligation Reaction Buffer (2X): 10 μl
3´ Ligation Enzyme Mix: 3 μl
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Total volume: 20 μl - Incubate for 1 hour at 25°C in a thermal cycler.
- Add the following components to the ligation mixture from step 5 and mix well:
Nuclease-free Water: 4.5 μl
SR RT Primer 1: 1 μl
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Total volume now should be: 25.5 μl - Heat samples for 5 minutes at 75°C. Transfer to 37°C for 30 minutes and then, to 25°C for 15 minutes.
- With 5 minutes remaining, resuspend the 5´ SR Adaptor 1 in Nuclease-free Water (For NEB #E6120S resuspend NEB #E6125A in 60 μl Nuclease-free Water and for NEB #E6120L resuspend NEB #E6125AA in 300 μl Nuclease-free Water).
- Heat the adaptor at 70°C for 2 minutes.
- Transfer tube to ice.
- Add the following components to the ligation mixture from step 7 and mix well:
5´ SR Adaptor 1 (from Step 10): 1 μl
5´ Ligation Reaction Buffer (10X): 1 μl
5´ Ligation Enzyme Mix: 2.5 μl
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Total volume now should be: 30 μl - Incubate for 1 hour at 25°C in a thermal cycler.
