CADO Zymo DNA/RNA Extractions of Large Juvenile Oyster Samples
Zymo DNA/RNA Extractions of Juvenile Oyster (> 4 mm) Samples
Extracting DNA and RNA from juvenile oyster samples from a multi-stressor exposure experiment.
Juveniles were collected individually in 1.5 mL tubes, preserved with liquid nitrogen, and held in a -80 freezer until processing.
This is the general protocol followed for DNA/RNA Extractions. I typically processed 12 samples at a time.
Time to Completion: 6-8 hours (includes QC)
Homogenization
- Turn on thermomixer and set to 55 degrees C, speed 1000 rpm
- Pull Proteinase K out of -20 freezer to warm to room temperature
- In 1.5 mL tubes, add 300 μL of DNA/RNA Shield
- Pull samples out of -80 freezer and put on ice
- Sterilize forceps with 100% EtOH, Type II DI Water, RNAse Zap, and RNAse-free Water
- Sterilize forceps between each sample
- Using forceps, transfer juvenile to 1.5 mL tube with DNA/RNA Shield
- Sterilize cone-shaped dremmel bit with 100% EtOH, Type II DI Water, RNAse Zap, and RNAse-free Water
- Sterilize the dremmel bit between each sample
- Insert dremmel bit into 1.5 mL tube with juvenile and grind up juvenile for ~10 seconds at speed 5
- Add 30 μL PK Digestion Buffer to each tube
- Add 15 μL Proteinase K
- Vortex and spin down
- Incubate in thermomixer at 55 degrees C and 1000 rpm for 30 minutes
- Halfway through incubation, spin down tubes in tabletop centrifuge for 1 minute at 13000 rpm
- During incubation period
- Prep and label all tubes for extraction protocol (for each tube type, multiply by number of samples being processed)
- 1.5 mL tubes for intermediate DNA
- 1.5 mL tubes for intermediate RNA
- Yellow spin-column and collection tubes for DNA purification
- Green or white spin-column and collection tubes for RNA purification (spin-column color will depend on kit)
- 1.5 mL tubes for final DNA sample
- 1.5 mL tubes for final RNA sample
- Prep 10 mM Tris HCl pH 8.0 and RNAse-free Water for thermomixer
- For each, 50 μL x # of samples (plus error) in 1.5 mL tubes
- Put in thermomixer set to 70 degrees C
- Make DNAse reaction mix:
- DNA Digestion Buffer: 75 μL x # of samples
- DNAse I: 5 μL x # of samples
- Prep and label all tubes for extraction protocol (for each tube type, multiply by number of samples being processed)
- After incubation, spin down tubes at max speed for 2 minutes in tabletop centrifuge
- Without disturbing the debris pellet, gently transfer all supernatant (~350 μL) to new 1.5 mL tube for DNA
- Save debris pellet and store in -20 freezer (can check for incomplete digestion later on if necessary)
- Add equal volume (300 μL) of DNA/RNA Lysis Buffer to each tube
- Finger flick to mix
- Transfer all supernatant (~600 μL) to yellow spin-column
- Centrigue at 16000 rpm for 30 seconds
- Transfer flow-through to new 1.5 mL tube for RNA
DNA Purification
- Add 400 μL of DNA/RNA Prep Buffer to yellow spin-column
- Centrifuge at 16000 rpm for 30 seconds
- discard flow-through
- Add 700 μL of DNA/RNA Wash Buffer
- Centrifuge at 16000 rpm for 30 seconds
- discard flow-through
- Add 400 μL of DNA/RNA Wash Buffer
- Centrifuge at 16000 rpm for 2 minutes
- discard flow-through
- Transfer spin-column to final 1.5 mL tube
- Carefully drip 50 μL of warmed 10 mM Tris HCl pH 8.0 directly onto filter
- Incubate at room temperature for 5 minutes
- Centrifuge at 16000 rpm for 30 seconds
- Pipette the 50 μL out of the 1.5 mL tube and drip directly onto the filter again
- Incubate at room temperature for 5 minutes
- Centrifuge at 16000 rpm for 30 seconds
- Should have 50 μL of DNA
RNA Purification
- Add equal volume (600 μL) 100% EtOH to each 1.5 mL tube for RNA
- Transfer 600 μL of supernatant to white spin-column
- Centrifuge at 16000 rpm for 30 seconds
- Discard flow-through
- Repeat until all supernatant is filtered (2 times total)
- Add 400 μL of DNA/RNA Wash Buffer to white spin-column
- Centrifuge at 16000 rpm for 30 seconds
- discard flow-through
- Add 80 μL of DNAse reaction mix to each column (I add directly onto filter)
- Incubate at room temperature for 30 minutes
- Add 400 μL of DNA/RNA Prep Buffer to white spin-column
- Centrifuge at 16000 rpm for 30 seconds
- discard flow-through
- Add 700 μL of DNA/RNA Wash Buffer
- Centrifuge at 16000 rpm for 30 seconds
- discard flow-through
- Add 400 μL of DNA/RNA Wash Buffer
- Centrifuge at 16000 rpm for 2 minutes
- discard flow-through
- Transfer spin-column to final 1.5 mL tube
- Carefully drip 50 μL of warmed RNAse-free Water directly onto filter
- Incubate at room temperature for 5 minutes
- Centrifuge at 16000 rpm for 30 seconds
- Pipette the 50 μL out of the 1.5 mL tube and drip directly onto the filter again
- Incubate at room temperature for 5 minutes
- Centrifuge at 16000 rpm for 30 seconds
- Should have 50 μL of RNA
Quality Control Check
Qubit
- DNA and RNA concentrations are checked using the Biotium dsDNA Broad Range and RNA Broad Range quantitation kits
- Final DNA and RNA concentrations (ng/μL) can be accessed here
Agarose Gel
- DNA quality is checked using an Agarose Gel, following the protocol for a Small 1% gel run
- Sample gel can be accessed here
TapeStation
- RNA quality is checked using the RNA ScreenTape Assay
- Sample TapeStation report can be accessed here
Written on February 1, 2024