Revision as of 19:05, 15 August 2013

Protocols

950 mL H₂0

10 g Tryptone

10 g NaCl

5 g Yeast Extract

1 L Total

Add 15 g Agar, if being poured into plates.

Autoclave, when cool add antibiotics if desired.

Chloramphenicol

Working Concentration 12.5 μg/ml

Stock solutions can be made at 35 mg/ml in ethanol and kept at -20º C

Kanamycin

Filter sterilize for kanamycin

Working Concentration:

25 μg/mL for low-copy plasmids

35 µg/mL for high-copy plasmids

Stock solution is 35 mg/ml in water and kept at -20º C

Spectinomycin

Filter sterilize

Working Concentration 50 μg/mL

Stock solution is 100 mg/mL in water and kept at -20º C

Preheat water bath to 42º C.
Thaw competent cells on ice for 10 minutes.
Use 50 µL competent cells, add transforming DNA [up to 25 ng per 50 µL of cells, volume not exceeding 2.5 µL (5%)]. For control add 1 µL of control DNA (PUC19 carb resistance). Swirl to mix, store on ice 5 minutes.
Heat shock in 42º C water bath for 45 seconds.
Cool cells in ice bath for a few minutes.
Add 800 µL LB to each tube, set in shaker at 37º C for 45 minutes.
Transfer 200 µL of culture per plate (containing the appropriate antibiotic).
Spread using glass beads.
Invert plates and incubate overnight (12-16 hrs) at 37º C.< /li>

@@ Line 43: / Line 43: @@
 <li>Spread using glass beads.</li>
 <li>Invert plates and incubate overnight (12-16 hrs) at 37º C.< /li>
-</ol><br></br>
+</ol>
         <h2 class="title">Making Chemically Competent Cells</h2>
         <h2 class="title">Double Restriction (Fast) Digest </h2>