Raw Experimental Notes June 2016
6/22/2016 Magi, Patrik, Kristen, Johan
Completed the following steps (as per plan!)
- Prepare define medium plates and broth
- For the plates: we mixed SD-URA+ glucose+Agar
- For the broth: we mixed SD-URA+ glucose
- Pour plates
- Save broth is fridge (to be used later)
- Culture yeast in medium
- Culture control yeast in defined medium overnight (12-72 hrs)
- Culture mutant yeast BY4741 in YPD overnight (12-72 hrs)
- Culture mutant yeast BY4742 in YPD overnight (12-72 hrs)
Small plates were used (because we are out of large size plates). The small plates have a total volume of 14mL. We poured approximately 5mL per plate
Note: Need to purchase Agar and large plates
- Step 1B. Pour plates
6/20/2016 Magi, Patrik, Kristen
Planning for Next Steps: Verification of Yeast (Streaking) and Transformation Objective: Verify the phenotype of two yeasts by growing them on various media
Streaking:
Day 1 Wednesday (starting at 6): 3-4 hrs
- Step 0. Make & Autoclave define (SD-URA) medium broth (2 hrs) (x2 for plates and broth)
- Step 1A. Culture control yeast in defined medium overnight (12-72 hrs)
- Step 1B. Pour plates
Day 2 Friday 5 pm
- Step 3. Measure optical density & normalize amount that we grow on each plate (1/2 hr): Need to get someone to help with that
- Step 4. Streak on different plates (1/2 hr)
- Step 5. Freeze remainder (1/2 hr)
Day 3 (Sun/Mon) after 1-2 days to take pictures of plates to double-check that yeast and plates work correctly
- Take pictures of all plates
Transformation: goal is to do this by Monday 6/27
- Figuring Out Protocol & Confirming Reagents
Day 1 (some Monday when Patrik can come in in the morning) Step 0. 5 Hour Growth in Specific Medium (may require autoclaving)
06/15/16 Patrik & Magi
Several of the standard URA- yeast strains grow poorly in defined medium, because the have a leucine uptake defect. So we decided to pour some plates with defined medium and double the normal amount of leucine. Standard leucine concentration in SD is 120mg/L.
See:
- Commonly used Saccharomyces cerevisiae strains (e.g. BY4741, W303) are growth sensitive on synthetic complete medium due to poor leucine uptake
- http://onlinelibrary.wiley.com/enhanced/doi/10.1111/j.1574-6968.2007.00798.x/
Ingredients:
- 7.47g/L SD-URA-Glucose
- 20g/L glucose
- 20g/L agar
- 120mg/L leucine
Adding leucine at 120mg/L in a 160mL mix which equates to 19.2mg of Leucine- used 23.4mg (accuracy achieved on scale)
In 160mL we added: 23.4mg of Leucine, 3.2g of Agar, 1.15g of SD-Ura-Glucose and 3.2g of Glucose
Added to autoclave until it reaches 121C then removed by Patrik.
Next steps:
- Get ready for Electroporation:
- Figure out the ideal timing to perform electroporation- ideally during the log phase of the yeast growth phase
6/13/2016 - Magi, Kristen, Patrik, Sean
Experiment: Yeast Revival & Confirmation of Correct Yeast
Tasks:
- 0. Revive yeast cultures (Patrik did this previously, and confirmed that the baker's yeast (control) was able to produce its own Uracil; however, the revived cell did not appear to exhibit much growth, so additional 500l of yeast strain was added to the tube, and another tube was also made) - Complete
- 1. Prepare agar mixes (done) - Complete
- 2. Pour Plates - Complete
- 3. Streak plates & then check for colony growth - Pending
ToDo(s):
- Immediate: Confirm that the yeast cultures exhibit the correct behavior (ability to grow in 5-FOA and not in SD-URA)
- Next Steps: Make new glycerol stock
- Later (Next Week): transformation (assuming everything goes well)
- Found previous prepared plates (large & labeled RVC)
- Check for contamination: 4 -URA + Glucose (colorless), 5 (mixture of YPD + YPD + FOA):> decided not to use these and to repaired
- Pouring medias: YPD, SD (-Ura -Glu), 5-FOA; decided to pour whole pack (25), so 8 plates of each
- Volume of plate: 700 ml per plate; decide to make 20 ml of working media (so 20 x 8 plates = 160 ml)
- YPD = 50 g/L; SD- = 7.47 g/L; (need to add 20 g/L of glucose); 5-FOA: 0.5% see prep calculations here: https://docs.google.com/spreadsheets/d/1SRrFP4an20c3uaTYZRlUEeXM6md2O3ES7In1e4Jjqnk/edit#gid=0
- Last night Patrik started some cultures: 1) control 2) revived culture (from the glycerol stock): should be able to grow in presence of 5-FOA but not in SD-URA
- Autoclave settings: 121 C (setting at 21)
- agar (non-LB) is added at 20 g/ml
Practices:
- Plates should be stored upside to avoid collecting contamination on lids)
- Contaminated plate submerged in bleach water
- Preparing bleach: 1:10 bleach to tapwater (grab from restroom; not hand-washing water)