"
Team:Cambridge/Protocols/Extraction of genomic DNA from squid
From 2011.igem.org
(→Practice) |
(→Practice) |
||
| Line 14: | Line 14: | ||
===Practice=== | ===Practice=== | ||
| - | 1. Prepare | + | 1. Prepare squid tissue samples and at least 100μl of PCR extraction buffer per tissue sample. |
| - | + | ||
| - | + | ||
:PCR Extraction buffer | :PCR Extraction buffer | ||
| Line 25: | Line 23: | ||
::*200 µg/ml Proteinase K | ::*200 µg/ml Proteinase K | ||
| + | :squid tissue sample | ||
| + | ::*~1 mm<sup>3</sup> cut into several pieces | ||
| + | |||
| + | |||
| + | 2. Place each tissue sample in an eppendorf tube with 100 µl PCR Extraction buffer, and incubate at 50-56°C for 2-3 hrs (longer is ok). Vortex occasionally. | ||
3. Boil samples in waterbath for 5-10 min to inactivate Proteinase K. | 3. Boil samples in waterbath for 5-10 min to inactivate Proteinase K. | ||
| - | 4. Spin in microfuge for | + | 4. Spin in microfuge at 13000 rpm for 5 minutes. The supernatant should contain the DNA while the proteins and cell fragments are in the pellet. |
| + | |||
| + | 5. Using a pipette, transfer the supernatant (containing genomic DNA) into another tube for storage. | ||
| - | + | Tip: For a 50 μl PCR reaction, use 10-15 μl of one of these DNA samples. | |
===Safety=== | ===Safety=== | ||
Revision as of 09:32, 20 July 2011
Extraction of genomic DNA from squid
A method to extract genomic DNA from squid tissue.
Large sample number, very quick and dirty, adequate for PCR
protocol adapted from http://zfin.org/zf_info/zfbook/chapt9/9.3.html
Theory
How it works
Practice
1. Prepare squid tissue samples and at least 100μl of PCR extraction buffer per tissue sample.
- PCR Extraction buffer
- 10 mM Tris pH 8
- 2 mM EDTA
- 0.2% Triton X-100
- 200 µg/ml Proteinase K
- squid tissue sample
- ~1 mm3 cut into several pieces
2. Place each tissue sample in an eppendorf tube with 100 µl PCR Extraction buffer, and incubate at 50-56°C for 2-3 hrs (longer is ok). Vortex occasionally.
3. Boil samples in waterbath for 5-10 min to inactivate Proteinase K.
4. Spin in microfuge at 13000 rpm for 5 minutes. The supernatant should contain the DNA while the proteins and cell fragments are in the pellet.
5. Using a pipette, transfer the supernatant (containing genomic DNA) into another tube for storage.
Tip: For a 50 μl PCR reaction, use 10-15 μl of one of these DNA samples.
Safety
The safety implication of the procedure.
