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< | Isolation of Total RNA |
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> | Isolation of Total RNA |
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< | Materials and Reagents |
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> | Materials and Reagents |
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Use filter tips. Keep all solutions, reagents and plastics to be used for RNA work separate from general supplies. Solutions need to be certified RNase free.
Equipment:
- Set a heat block to 95°C.
- A bench top centrifuge is required.
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- ZYMO RNA Clean & Concentrator™- 25 kit Cat # R1017 - add ethanol to buffers prior to use.
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- ZYMO RNA Clean & Concentrator™- 25 kit Cat # R1017 - add ethanol to buffers prior to use.
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- Tapestation access/training
- Qubit
Solutions: |
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- RNA extraction solution (needs to be made fresh before each use).
- 18mM EDTA
- 0.025% SDS
- 1% 2-mercaptoethanol
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- RNA extraction solution (needs to be made fresh before each use).
- 18mM EDTA
- 0.025% SDS
- 1% 2-mercaptoethanol
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- 95% formamide (RNA grade)
- RNase free water
- DNase 1 solution for on-column digestion (from Zymo, cat #E1010)
- Ethanol, 95-100% (from Biosci store is fine)
- Ethanol, 80% (diluted from above with RNase free water)
For quality check:
- Tapestation RNA screentape (Agilent cat #5067-5576)
- Tapestation RNA screentape sample buffer (Agilent cat #5067-5577)
- Qubit RNA broadrange assay kit (Thermofiosher cat# Q10210)
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- Ensure DNase 1 is thawed.
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- Pellet cells and prepare immediately OR flash freeze on liquid nitrogen and store at -80. When removing cells from -80 for prep, store on dry ice until ready for extraction.
- Critical Rapidly resuspend cell pellet in 500ul of RNA extraction solution. Use pipette tip to dislodge a frozen pellet, break apart and triturate until homogeneous. Work quickly to avoid RNase degradation.
- Incubate sample at 95°C for 7min to lyse cells. Place a weight on top of tubes (or use tube locks) to prevent pressure from opening tubes.
- Pellet the warm sample by centrifuging at 16 000 x g for 5min at room temperature.
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- Pellet cells and prepare immediately OR flash freeze on liquid nitrogen and store at -80. When removing cells from -80 for prep, store on dry ice until ready for extraction.
- Critical Rapidly resuspend cell pellet in 500ul of RNA extraction solution. Use pipette tip to dislodge a frozen pellet, break apart and triturate until homogeneous. Work quickly to avoid RNase degradation.
- Incubate sample at 95°C for 7min to lyse cells. Place a weight on top of tubes (or use tube locks) to prevent pressure from opening tubes.
- Pellet the warm sample by centrifuging at 16 000 x g for 5min at room temperature.
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- Transfer 200ul of supernatant containing RNA to a fresh tube and continue with below RNA clean up. Store the remaining ~300ul at -80°C, as a back up.
The following uses the Zymo clean and concentrator kit:
- Add 2 volumes (400ul) of RNA Binding Buffer to each volume of RNA sample and mix well.
- Add 1 volume (600ul) ETOH (95-100%) to the mixture and mix well.
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- Transfer the mixture to the Zymo-Spin IIC column in a collection tube and centrifuge at >12,000 x g for 1 min. Discard the flow through.
- During this spin, prepare the DNase 1 cocktail for use. Per reaction:
- 5ul RNase-Free DNase I
- 75ul Reaction Buffer
- Add 400ul of 80% ethanol to the Zymo-Spin IIC column in a collection tube and centrifuge at >12,000 x g for 30 secs. Discard the flow through.
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- Transfer the mixture to the Zymo-Spin IIC column in a collection tube and centrifuge at >12,000 x g for 1 min. Discard the flow through.
- During this spin, prepare the DNase 1 cocktail for use. Per reaction:
- 5ul RNase-Free DNase I
- 75ul Reaction Buffer
- Add 400ul of 80% ethanol to the Zymo-Spin IIC column in a collection tube and centrifuge at >12,000 x g for 30 secs. Discard the flow through.
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- Add 80ul DNase I cocktail directly to the matrix of the Zymo-Spin IIC column.
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- Incubate the column at 25-370C for > 15 mins (optimal temp for DNase I is 370C).
- Centrifuge > 12,000 x g for 30 seconds. Discard the flow through.
- Add 400ul RNA Prep Buffer to the column and centrifuge at 12,000 x g for 1 minute. Discard the flow trough.
- Add 800ul RNA Wash Buffer to the column and centrifuge at > 12,000 x g for 30 seconds. Discard the flow through. Repeat this wash step with 400ul RNA Wash Buffer.
- Centrifuge the Zymo-Spin IIC Column in an emptied collection tube at >12,000 x g for 2 minutes. Remove the column carefully from the collection tube and transfer to new RNase-free tube.
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- Incubate the column at 25-370C for > 15 mins (optimal temp for DNase I is 370C).
- Centrifuge > 12,000 x g for 30 seconds. Discard the flow through.
- Add 400ul RNA Prep Buffer to the column and centrifuge at 12,000 x g for 1 minute. Discard the flow trough.
- Add 800ul RNA Wash Buffer to the column and centrifuge at > 12,000 x g for 30 seconds. Discard the flow through.
- Add 400ul RNA Wash Buffer to the column and centrifuge at > 12,000 x g for 2 minutes. Discard the flow through. Remove the column carefully from the collection tube and transfer to new RNase-free tube.
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- Add 30 ul of DNase/RNase-Free water directly to the column matrix and let stand for 1 minute at room temperature.
- Centrifuge at 10,000 x g for 1 min.
- Use the eluted RNA immediately or store at -80C.
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< | Assess the RIN and quantity of RNA eluted using the Tapestation (load ~100ng) and Qubit (a dilution of 1/10 will be required to reach linear range), respectively. |
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> | Assess the RIN and quantity of RNA eluted using the Tapestation (load ~100ng) and Qubit (a dilution of 1/10 will be required to reach linear range), respectively. |
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-- Main.SimonDAlton - 23 Jan 2017 |
