Methods/DNA barcoding: Difference between revisions
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# Incubate the sample at 65°C for 18 mins + 98°C for 2 mins in a PCR machine | # Incubate the sample at 65°C for 18 mins + 98°C for 2 mins in a PCR machine | ||
# Add the same amount of neutralizing buffer as you used of the alkaline buffer (so 10 μl alkaline + 10 μl neutralizing or 15 μl alkaline + 15 μl neutralizing) | # Add the same amount of neutralizing buffer as you used of the alkaline buffer (so 10 μl alkaline + 10 μl neutralizing or 15 μl alkaline + 15 μl neutralizing) | ||
== Our extraction protocol == | |||
'''BEFORE starting''', check if we have: | |||
* enough buffers (alkaline and neutralizing) – if not, mix new one | |||
* enough sterile stripes – if not, autoclave more | |||
=== Prepare the Extraction Plate Map (MS Excel) === | |||
* select the samples you will extract | |||
* make a plate map, '''keep at least 2 positions empty''' | |||
* save the plate map, and print it out | |||
* mark positions with BIG animals (they have "yes" in the sample sorting file) | |||
* upload the plate map into the Lab Cloud | |||
=== Prepare the place for work === | |||
* 2× 48-well plastic tray, fill each well with a bit of purified water | |||
* burner with enough alcohol | |||
* lighter | |||
* sterile Petri dish with a bit of purified water | |||
* paper tissues | |||
* one soft and two hard forceps (sterilize properly in the beginning) | |||
=== Prepare stripes === | |||
# Prepare 12 sterile strips. | |||
# Pipette '''15 μl of alkaline buffer into each microvial''' (use tips with filter) | |||
# Close all strips. | |||
# '''Number the strips''' – numbers 1–12 on the lid of the first microvial in the strip | |||
# Mark the empty positions. | |||
=== Put specimens into the alkaline buffer === | |||
* Take one '''specimen from each sample''', put in 48-well plate in purified water | |||
* In '''large specimens''', take 1–3 legs (ideally each from one side) using hard forceps. Return the specimen to the original vial, and mark the vial label in red | |||
* After some time (5–15 mins) move the specimen from the water to the strip microvial with buffer using sterile forceps. | |||
=== DNA extraction === | |||
# '''Put into PCR machine''' – the program is called '''HOTSHOT''' (65°C for 18 mins + 98°C for 2 mins) | |||
# Add '''15 μl of neutralizing buffer into each microvial'''. | |||
=== After DNA extraction === | |||
* '''Pipette out the liquid''' into new marked strips. This will be your '''DNA extract''' | |||
* '''Add 75% or 95% alcohol''' to the strips with specimens | |||
* '''Add Sample ID labels to each sample.''' | |||
=== Storing the extraction === | |||
* Double-check that the plate is properly marked (e.g., '''Extraction: Eric001''') | |||
* You can use it immediately for PCR | |||
* '''If you will use it''' soon (in 1–2 days), keep it in the '''-20°C freezer''' | |||
* '''If you will not use it''' soon or it is finalized, keep it in the '''-70°C freezer''' | |||
Revision as of 03:03, 6 May 2026
DNA extraction using HotShot
Mixing the buffers
Alkaline Buffer (= 25 mM NaOH + 0.2 mM disodium EDTA)
- Premix 10M NaOH:
- 70 ml H₂O + 40g NaOH and adjust to 100 ml
- or
- 17.5 ml H₂O + 10g NaOH and adjust to 25 ml
- To 25 ml of H₂O add:
- 62.5 μl of 10M NaOH
- 10 μl of 0.5 M disodium EDTA
Neutralizing Buffer (40 mM trisHCl)
Mix the following:
- 24 ml of H₂O
- 1 ml of 1M trisHCl
How to use the buffers to extract DNA
- Place the specimen into 10–15 μl of alkaline buffer in a microvial
- Incubate the sample at 65°C for 18 mins + 98°C for 2 mins in a PCR machine
- Add the same amount of neutralizing buffer as you used of the alkaline buffer (so 10 μl alkaline + 10 μl neutralizing or 15 μl alkaline + 15 μl neutralizing)
Our extraction protocol
BEFORE starting, check if we have:
- enough buffers (alkaline and neutralizing) – if not, mix new one
- enough sterile stripes – if not, autoclave more
Prepare the Extraction Plate Map (MS Excel)
- select the samples you will extract
- make a plate map, keep at least 2 positions empty
- save the plate map, and print it out
- mark positions with BIG animals (they have "yes" in the sample sorting file)
- upload the plate map into the Lab Cloud
Prepare the place for work
- 2× 48-well plastic tray, fill each well with a bit of purified water
- burner with enough alcohol
- lighter
- sterile Petri dish with a bit of purified water
- paper tissues
- one soft and two hard forceps (sterilize properly in the beginning)
Prepare stripes
- Prepare 12 sterile strips.
- Pipette 15 μl of alkaline buffer into each microvial (use tips with filter)
- Close all strips.
- Number the strips – numbers 1–12 on the lid of the first microvial in the strip
- Mark the empty positions.
Put specimens into the alkaline buffer
- Take one specimen from each sample, put in 48-well plate in purified water
- In large specimens, take 1–3 legs (ideally each from one side) using hard forceps. Return the specimen to the original vial, and mark the vial label in red
- After some time (5–15 mins) move the specimen from the water to the strip microvial with buffer using sterile forceps.
DNA extraction
- Put into PCR machine – the program is called HOTSHOT (65°C for 18 mins + 98°C for 2 mins)
- Add 15 μl of neutralizing buffer into each microvial.
After DNA extraction
- Pipette out the liquid into new marked strips. This will be your DNA extract
- Add 75% or 95% alcohol to the strips with specimens
- Add Sample ID labels to each sample.
Storing the extraction
- Double-check that the plate is properly marked (e.g., Extraction: Eric001)
- You can use it immediately for PCR
- If you will use it soon (in 1–2 days), keep it in the -20°C freezer
- If you will not use it soon or it is finalized, keep it in the -70°C freezer
