Team:Calgary/Notebook/Protocols/Process1
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- | TITLE=Plasmid | + | TITLE=Plasmid Isolation| |
BODY=<html> | BODY=<html> | ||
<p> | <p> | ||
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<br> | <br> | ||
- | <h4> Reagents </h4> | + | <h4> Reagents and Materials </h4> |
<ol> | <ol> | ||
<li>LB broth, pH 7</li> | <li>LB broth, pH 7</li> | ||
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<ol> | <ol> | ||
- | <li>Inoculate a loopful of Pseudomonas sp. at | + | <li>Inoculate a loopful of Pseudomonas sp. at 25°C, in 10mL LB broth (10g tryptone; 5g yeast extract, 5g NaCl, 1000mL distilled H<sub>2</sub>O, pH 7.0), and incubate for 16-18hr.</li> |
<li>Centrifuge 1.5 ml of a 16-18hr bacterial culture for 1 min at 11,500 x g in a polypropylene centrifuge tube.</li> | <li>Centrifuge 1.5 ml of a 16-18hr bacterial culture for 1 min at 11,500 x g in a polypropylene centrifuge tube.</li> | ||
<li>Remove supernatant by aspirating, leaving the pellet as dry as possible.</li> | <li>Remove supernatant by aspirating, leaving the pellet as dry as possible.</li> | ||
- | <li>Add to each tube, 400µL of 8% sucrose, 5.0% Triton X-100, 50 mM EDTA, and 10mM Tris | + | <li>Add to each tube, 400µL of 8% sucrose, 5.0% Triton X-100, 50 mM EDTA, and 10mM Tris HCl (pH 8.0). Mix well.</li> |
- | <li>Add 50µL of freshly prepared lysozyme solution (10mg/mL in 10mM Tris HCl, | + | <li>Add 50µL of freshly prepared lysozyme solution (10mg/mL in 10mM Tris HCl, pH 8), mix by inverting 3X. Lysozyme digests bacterial cell wall.</li> |
- | <li>Immediately incubate at | + | <li>Immediately incubate at 100°C for 10, 20, 40, 80s.</li> |
<li>Spin for 10min 11,500Xg at room temp.</li> | <li>Spin for 10min 11,500Xg at room temp.</li> | ||
<li>Remove pellet with sterile forceps.</li> | <li>Remove pellet with sterile forceps.</li> | ||
- | <li>Add to supernatant, 50µL of cold 3M | + | <li>Add to supernatant, 50µL of cold 3M NaOAc and 420µL of cold isopropanol.</li> |
- | <li>Incubate 30min at - | + | <li>Incubate 30min at -20°C.</li> |
- | <li>Centrifuge 15min for 11,500Xg at | + | <li>Centrifuge 15min for 11,500Xg at 4°C.</li> |
<li>Decant supernatant, invert and drain on clean paper towel.</li> | <li>Decant supernatant, invert and drain on clean paper towel.</li> | ||
- | <li>Add 15µL of cold/ | + | <li>Add 15µL of cold/4°C TE buffer (0.05M Tris, 0.01M EDTA, pH8).</li> |
- | <li>Incubate for 1hr at | + | <li>Incubate for 1hr at 4°C in dark. </li> |
- | <li>Run a small amount of this sample on gel electrophoresis on 0.7% (w/ | + | <li>Run a small amount of this sample on gel electrophoresis on 0.7% (w/v) agarose. With the rest, submit to further purification.</li> |
</ol> | </ol> | ||
<br> | <br> | ||
- | <h4>Further purification (Plasmid from putida)</h4> | + | <h4>Further purification (Plasmid from <i>Pseudomonas putida</i>)</h4> |
<ol> | <ol> |
Latest revision as of 04:16, 29 September 2011
Plasmid Isolation
This protocol will purify plasmids from bacteria, though identification of plasmids will need to be confirmed by PCR.
Reagents and Materials
- LB broth, pH 7
- 10g tryptone
- 5g yeast extract
- 5g NaCl
- 20% sucrose (autoclaved)
- Triton X-100
- 500mM EDTA stock (pH 8.0)
- Tris-HCl 50mM
- NaCl 3M
- Isopropanol
- Autoclaved Milli-Q water
Procedure
- Inoculate a loopful of Pseudomonas sp. at 25°C, in 10mL LB broth (10g tryptone; 5g yeast extract, 5g NaCl, 1000mL distilled H2O, pH 7.0), and incubate for 16-18hr.
- Centrifuge 1.5 ml of a 16-18hr bacterial culture for 1 min at 11,500 x g in a polypropylene centrifuge tube.
- Remove supernatant by aspirating, leaving the pellet as dry as possible.
- Add to each tube, 400µL of 8% sucrose, 5.0% Triton X-100, 50 mM EDTA, and 10mM Tris HCl (pH 8.0). Mix well.
- Add 50µL of freshly prepared lysozyme solution (10mg/mL in 10mM Tris HCl, pH 8), mix by inverting 3X. Lysozyme digests bacterial cell wall.
- Immediately incubate at 100°C for 10, 20, 40, 80s.
- Spin for 10min 11,500Xg at room temp.
- Remove pellet with sterile forceps.
- Add to supernatant, 50µL of cold 3M NaOAc and 420µL of cold isopropanol.
- Incubate 30min at -20°C.
- Centrifuge 15min for 11,500Xg at 4°C.
- Decant supernatant, invert and drain on clean paper towel.
- Add 15µL of cold/4°C TE buffer (0.05M Tris, 0.01M EDTA, pH8).
- Incubate for 1hr at 4°C in dark.
- Run a small amount of this sample on gel electrophoresis on 0.7% (w/v) agarose. With the rest, submit to further purification.
Further purification (Plasmid from Pseudomonas putida)
- Layer the resuspended DNA on a 2.5mL bed of saturated CsCl in a polymer tube. Centrifuge for 14hr at 14 000 rpm in a fixed-angle 30 rotor at 2°C. After the run, ~25mL of liquid can be discarded from the top without disturbing the remainder. Mix the lower part to form the concentrated lysate.
- Slowly dissolve ~5.7g CsCl to the concentrated lysate, until the refractive index is 1.399. Mix solution with Syber-safe or gel-red. Centrifuge for 40hr in a Spinco fixed-angle rotor 50 at 105 000 x g at 12°C. After this run, 2 well-separated bands should be able to be seen. Alternatively, do only this spin where DNA mixed with CsCl is concentrated to a refractive index of 1.399 with the fluorescent DNA stain.
- Because the DNA was infused with dye, 2 well-separated bands will appear. The upper band is linear and non-circular DNA (junk). The lower band is the plasmid of interest. Remove the upper layer with a micropipette. After it is removed, pool bands from several tubes centrifuge again SW50.1 rotor for 20h at 40 000rpm. Again there will be 2 bands and the lower band is the desired intact plasmid.