Team:Toronto/Protocols

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Contents

Protocols

Tolerance Assay

A 0.5 M (10x) stock solution of catechol was made in a 5 ml volume of autoclaved, distilled water. This solution was added to 25 ml of sterile MM2 media to make up a volume of 30 ml. This was added to 20 ml of MM2 innoculated with E.coli DH5a (approximate density 1x10e8 cells per ml) for a final volume of 50 ml (catechol concentration 50mM). Control samples were created as above minus catechol. Treated and untreated samples were placed in a 37C shaker incubator and aliquots were removed every two hours. 0.5 ml aliquots were serially diluted in 4.5 ml of MM2 media and four dilutions representing 1 x 10-3, 1 x 10-4, 1 x 10-5 and 1x10-6 were plated by spreading 200 ul of the diluted sample on LB agar plates. After drying, plates were incubated in an inverted position in a 37C incubator overnight. Plates with between 30 and 300 colonies were counted to determine the number of colony forming units using the method described by Imperial College (iGEM 2009 OpenWetWare).

Making Chemically Competent Cells

Day 1

1. Start a 5 mL LB overnight culture in the 37C incubator from either a colony streaked plate or with one of the last frozen competent stocks of the strains you want to make competent.

Day 2

1. Inoculate the 5 mL overnight culture into a new flask with 200 mL of fresh LB.

2. Grow until O.D. 600 = 0.4.

a. To check O.D., take 1 mL of the bacterial culture and put it in a plastic cuvette.

b. Take another plastic cuvette and add in 1 mL of LB.

c. Change the wavelength of the spectrophotometer to 600 nm.

d. Blank using the LB cuvette.

e. Measure and record the absorbance of the cuvette containing the culture.

f. If the O.D. is below 0.4, place the flask back in the 37°C incubator and repeat ‘e’ at a later time point. Dispose of the cuvette with the culture but keep the cuvette with the LB as a blank.

3. Transfer 50 mL of the culture into a pre-chilled Falcon tube. Repeat for each of the remaining 3 Falcon tubes.

4. Place the Falcon tubes in ice for 15 minutes to cool the cultures.

5. Pellet the cells using a Beckman centrifuge at 4000 rpm for 10 minutes at 4°C.

6. Pour out the media in the sink and stand the Falcon tubes in an inverted position on paper towels for 1 min to drain away traces of liquid.

7. Re-suspend the pellets in each tube with 10 mL of ice cold 0.1M CaCl2 by lightly pipetteing with a P1000.

8. Store on ice for 10 min.

9. Pellet the cells using a Beckman centrifuge at 4000 rpm for 10 minutes at 4°C.

10. Pour out the media in the sink and stand the Falcon tubes in an inverted position on paper towels for 1 min to drain away traces of liquid.

11. Re-suspend the pellets in each tube with 2 mL of ice cold 0.1M CaCl2 by lightly pipetteing with a P1000.

12. Pool the aliquots and keep on ice for 1 hour.

13. Make a dry ice/ethanol bath.

a. Dry ice is on the 14th floor in the corresponding room where the incubators are at on our floor.

b. Ethanol is under the fumehood in a cabinet labelled “Flammables” beside the imaging room.

14. Add in 4.8 mL of ice cold 40% glycerol and very gently invert the tube to mix well.

15. Divide the mixture into the pre-chilled microfuge tubes in 400 µL aliquots.

16. Flash freeze the aliquots in the dry ice bath.

17. Store in the -80°C freezer.

Transforming Chemically Competent Cells

1. Thaw a stock of competent cells that you want to transform into on ice for 10 minutes. DO NOT REMOVE IT FROM THE ICE DURING THIS TIME.

2. If you are doing more than 1 transformation, take 100 µL of cells from the freezer stock and add it to prechilled microfuge tubes. If not, take 100 µL of cells to use as transformation controls.

3. Add 1 µL of DNA to the cells you want transformed. Stir gently with the pipette as any serious agitation will decrease transformation by a lot.

4. Leave mixtures on ice for 30 minutes.

5. Heat shock cells for 30s at 42°C. Different times and temperatures will decrease transformation efficiency.

6. Place mixtures on ice for 5 min.

7. Add LB to each tube until the total volume is 1 mL. (i.e. If there is 100 µL of cells, add 900 µL of fresh LB)

8. Place the tubes in the 37°C shaker for 1 hour.

9. Pre-warm and label (date, initials, what DNA is transformed with what cells, amount plated) selection plates in the 37°C incubator with the sign “BACTERIA ONLY”.

10. Spread plate 2 amounts of transformants (10 µL and 50 µL) onto the corresponding selection plates.

11. Place overnight in the 37°C incubator with the sign “BACTERIA ONLY”.