Maheshri:TransformationY

The TRAFO method

High Efficiency Transformation Protocol

This protocol can be used to generate sufficient transformants in a single reaction to screen multiple yeast genome equivalents for plasmids that complement a specific mutation. It can also be used to transform integrating plasmids, DNA fragments and oligonucleotides for yeast genome manipulation. Finally, it is used to optimise the conditions for transformation of a particular yeast strain, for example, the transformation of a plasmid library into a two-hybrid yeast strain transformed with a bait plasmid by the Rapid Transformation Protocol. The High Efficiency Protocol can also be employed to transform a yeast strain simultaneously with two different plasmids, such as the two-hybrid bait and prey plasmids.

Day 1

Inoculate the yeast strain into 2-5 mL of liquid medium (2x YPAD or SC selection medium) and incubate overnight on a rotary shaker at 200 rpm and 30°C. Place a bottle of 2x YPAD and a 250 ml culture flask in the incubator as well.

Day 2

1. Determine the OD of the yeast culture. Dilute the overnight YPAD or SC cultures in 50mL of 2x YPAD to an OD of ~0.1.
2. Incubate the flask on a rotary or reciprocating shaker at 30°C and 200 rpm. Note that:

i)   It is important to allow the cells to complete at least two divisions. 
ii)  This will take 3 to 5 hours. 
iii) This culture will give sufficient cells for 10 transformations.
iv)  Transformation efficiency (remains constant for 3 to 4 cell divisions.   

1. When the OD becomes ~1, which should take about 5 hours, harvest the cells by centrifugation at 3000 g for 5 min, wash the cells in 25 mL of sterile water and resuspend in 1 ml of sterile water.
2. While your are harvesting the cells, boil a 1.0 mL sample of carrier DNA for 5 min and chill in an ice/water bath while harvesting the cells. Note that it is not necessary or desirable to boil the carrier DNA every time. Keep a small aliquot in your own freezer box and boil after 3-4 freeze-thaws. But keep on ice when out.
3. Transfer the cell suspension to a 1.5 mL microcentrifuge tube, centrifuge for 30 sec and discard the supernatant.
4. Add water to a final volume of 1.0 mL and resuspend the cells by pipetting. If the OD of the culture is greater than 1 (but not much greater) then increase the volume accordingly. If the OD is less than 1 then decrease volume.
5. Pipette 100 µL samples (~10^8 cells) into 1.5 mL microfuge tubes, one for each transformation, centrifuge at 3000 min for 1 min and remove the supernatant.
6. Add the following Transformation Mix to each tube, resuspend the cells by pipetting and gentle vortexing (speed 7).

PEG 3500 50% w/v           240 µL
LiAc 1.0 M                 36 µL
Boiled SS-carrier DNA      50 µL
Plasmid DNA plus Water     34 µL
Total                      360 µL

1. Incubate the tubes in a 42°C water bath for 40 min. Note that the optimum time can vary for different yeast strains. Please test this if you need high efficiency from your transformations.
2. Microcentrifuge at 3000 rpm for 1 min and remove the Transformation Mix with a micropipettor.
3. Optional - Wash (resuspend and pellet) the cells with 1.0 mL of sterile water
4. Add 200μL of sterile water to the tube, resuspend cells, and plate the cell suspension onto selection medium (e.g. a SD dropout plate).

Additional Notes

A 'sleazy' method for plasmid transformation

1) Using sterile technique, mix the following in a microcentrifuge tube:

PEG 3500 50% W/V        240μL
LiAc 1.0M               36μL
Boiled SS-carrier DNA   50μL
Plasmid DNA plus ddH2O  34μL
A toothpick full of yeast from a fresh plate (<2 days old)

2) Incubate the tubes at room temperature for overnight (>8 hours)

3) Microcentrifuge at 3000rpm for 1 min and remove the Transformation Mix

4) Optional - Wash (resuspend and pellet) the cells with 1.0 mL of sterile water

5) Add 200μL of sterile water to the tube, resuspend cells, and plate the cell suspension onto selection medium (e.g. a SD dropout plate).