Team:WashU/Notebook
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***Make solution of 5uL URA3, 45uL DI water | ***Make solution of 5uL URA3, 45uL DI water | ||
***Concentration: 35.9 ng/mL | ***Concentration: 35.9 ng/mL | ||
+ | |||
+ | *KanMX4 group | ||
+ | **30.5 ng/uL (from previous day) | ||
+ | |||
+ | *NatMX4 group | ||
+ | **Performed mini-prep on previous day's culture | ||
+ | **200uL eluent with concentration of 28.7 ng/mL | ||
+ | |||
+ | *Made a 1/10 dilution of last year's NatMX4 stock | ||
+ | **23.3 ng/mL |
Revision as of 17:03, 6 June 2011
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Contents |
Notebook
You should make use of the calendar feature on the wiki and start a lab notebook. This may be looked at by the judges to see how your work progressed throughout the summer. It is a very useful organizational tool as well.
May 31
- Preliminary Shopping List
- PCR buffer w/o MgCl - 5ML - $45.00
- M8787- 5ML -MgCl Reagent- $49.30
- D7295-.5ML - dNTP - $73.00
- D4184-250UN - Taq Polymerase - $150.00
- D8045-250UN - AccuTaq - $300
- E1385-5ML – Ethidium Bromide – $23.70
- T8280-1L – Tris Acetate EDTA Buffer – $45.10
- NA1020-1KT – PCR Clean-Up Kit -$102.50
- NA1111-1KT - Gel Extraction Kit - $102.00
Subtotal: $890.60
- Met with Cohen Lab grad students to finalize plan and get cassettes.
- Received Leu2 cassette in pRS305 plasmid.
- Received Ura3 cassette in pRS306 plasmid.
June 1
- Lesson from Bert Berla on how to design primers
- Codon Optimized the four genes using tool at: http://www.encorbio.com/protocols/Codon.htm
- Double checked gene and restriction sites to make sure enzyme does not cut in the middle of the gene
- Design Primers for cassettes
- Ura3, Leu2, KanMX4, and NatMX4
June 2
- Made two liters of LB solution
- 25g of LB Broth per Liter (10g Tryptone, 5g Yeast Extract, and 10g NaCl)
- Autoclaved solutions: 30 minute sterilization.
- Refrigerated after cooling.
June 3
- Made YPD
- In 800ml water in 1 L bottle dissolve 10g of BactoYeast extract
- Dissolve 20g of BactoPeptone in the above solution
- In 200ml water in 500ml bottle dissolve 20g Dextrose
- Autoclave both, combine after autoclaving. (30 minute sterilization)
- Made 1000X Ampicillin Stock
- Added 2g Ampicillin to 20ml water.
- Added NaOH until dissolved.
- Sterile filtered.
- Frozen in -20C Freezer
- Made cultures of E. coli strains with KanMx4 and Natmx4 inserts.
- In culture tubes, added 5ml LB and 5ul 1000X Ampicillin Stock.
- Transferred one colony per strain from plates to culture tubes.
- Incubate at 30 degrees Celsius shaking at 225rpm overnight.
- Made cultures of Yeast strains BC177 and BC178
- Added 5ml YPD to two culture tubes.
- Transferred one colony per strain from plates to culture tubes.
- Incubate at 30 degrees Celsius shaking at 225rpm overnight.
June 4
- Making freezer stocks of yeast cultures BC177 and BC178
- Add 1.25mL glycerol to yeast culture
- Freeze yeast culture in -80 degree freezer
- Make E.coli mini-preps for plasmids containing KanMX4 and NatMX4 (Sigma-Aldrich Mini-Prep Kit)
- Transferred 4 ml of each culture to microcentrifuge tubes.
- Centrifuge for one minute at 12000xg
- Pour out supernatant
- add 200uL of resuspension solution with RNase
- add 200uL of lysis buffer
- add 350uL of neutralization buffer
- Centrifuge for 10 minutes at 12000xg
- Insert a Miniprep Binding Column into microcentrifuge tubes and add 500uL of Column Preparation Solution to each miniprep column.
- Centrifuge at 12000xg for 1 minute. Discard the flow-through
- Take the lysis of the cultures resulting from the 10 minute centrifuge and pipet it into the binding column
- Centrifuge at 12000xg for 1 minute. Discard the flow-through
- Add 500uL of Wash Solution 1 to the column and centrifuge at 12000xg for one minute. Discard the flow-through.
- Repeat the previous step
- Add 750uL of Wash Solution 2 (with ethanol) to the column and centrifuge at 12000xg for one minute. Discard the flow-through.
- Centrifuge at 12000xg for one minute.
- Transfer the column to a fresh collection tube and add 100uL of Elution Solution to the column
- Centrifuge at 12000xg for one minute.
- Store the eluate at -20 degrees C
- This procedure was done separately for the plasmids that contain KanMX4 and NatMX4.
June 5
Read absorbances for all four solutions that contain plasmids with our cassettes: Ura3, Leu3, KanMX4, and NatMX4.
Data was obtained using a nano-drop spectrophotometer. Absorbance was observed between 250nm and 280nm.
DNA Concentrations were as follows:
- Ura3: Very high absorbance reading, must be diluted 1/10 in order to get accurate concentration reading.
- Leu2: Very high absorbance reading, must be diluted 1/10 in order to get accurate concentration reading.
- KanMX4: 30.5 ng/uL
- NatMX4: Very low absorbance reading, eluent was discarded.
- Last year's NatMX4 solution: Very high absorbance reading, must be diluted 1/10 in order to get accurate concentration reading.
Next step: Make diluted stock solutions of the Ura3 and Leu2 plasmids and take new absorbance readings.
For NatMX4, we will begin a new culture with a new colony and redo the mini-prep. If unsuccessful, we will use last year's stock.
- Made new culture of NatMX4
- 5ml of TB + 5uL of 1000x Ampicillin
- Incubated overnight at 31 degrees Celsius.
June 6
- LEU2 group
- Make dilution for nanodrop
- Make solution of 5uL LEU2, 45uL DI water
- Concentration: 42.0 ng/mL
- Make dilution for nanodrop
- URA3 group
- Make dilution for nanodrop
- Make solution of 5uL URA3, 45uL DI water
- Concentration: 35.9 ng/mL
- Make dilution for nanodrop
- KanMX4 group
- 30.5 ng/uL (from previous day)
- NatMX4 group
- Performed mini-prep on previous day's culture
- 200uL eluent with concentration of 28.7 ng/mL
- Made a 1/10 dilution of last year's NatMX4 stock
- 23.3 ng/mL