Team:Washington/Notebook
From 2009.igem.org
(Difference between revisions)
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# Allow beads to bind to flourophore, then spin beads down, remove supernatent and replace with 1 ml water. | # Allow beads to bind to flourophore, then spin beads down, remove supernatent and replace with 1 ml water. | ||
# Next place the cells and the beads under the microscope | # Next place the cells and the beads under the microscope | ||
+ | |||
+ | ==== Procedure ==== | ||
+ | # Set up overnights of parts 48-51. Let grow overnight. | ||
+ | # Dilute 1 ul overnight into 1ml | ||
+ | # Add 1 mm IPTG and let grow for four hours | ||
+ | # After cells have grown up, place in flourophore (1 um) and allow time to bind (1 hour) | ||
+ | # Also place 1 ul beads in 1 ml along with 1 ul flourophore. | ||
+ | # Allow beads to bind to flourophore, then spin beads down, remove supernatent and replace with 1 ml water. | ||
+ | # Read the samples through the flow cytometer | ||
Revision as of 21:28, 12 October 2009
A DETAILED DESCRIPTION OF THE PROTCOLS WE USED
- Gene Synthesis
- Colony PCR
- Assembly
- Cloning
- Expression
- Purification
Procedure
- Set up overnights of parts 48-51
- Dilute 1 ul overnight into 1ml
- Add 1 mm IPTG and let grow for four hours
- After cells have all grown up uniformly start boiling water for the boil step
- Add 100uL of overnight to a 1.5mL tube
- Pellet by spinning at max speed for 30 secs in the microcentrifuge
- discard supernatent
- Pull an aliquot of 5x sample loading buffer out of the freezer and thaw
- Add 20uL BME to aliquot
- Resuspend samples in 50uL sample loading buffer (pipette up/down)
- Boil samples for 10 minutes
- While boiling, prepare 500mL 1x SDS buffer:
- 50mL 10x buffer to 450mL water
- Take a gel out of the fridge and and put it in the gel box (keep the gel container for staining!!!)
- Pour the mixed buffer solution into the half of the gel box that the gel is in
- Remove the gel comb
- Fill the little container on the top of the gel until it's about 0.5 cm from the top with buffer
- Remove any bubbles in the wells
- Spin down samples for a few seconds
- Vortex samples
- Load 3uL into each well
- Load 10uL of ladder in appropriate wells
- Run at 180V until the dye is about to fall off the gel
Procedure
- Set up overnights of parts 48-51. Let grow overnight.
- Dilute 1 ul overnight into 1ml
- Add 1 mm IPTG and let grow for four hours
- After cells have grown up, place in flourophore (1 um) and allow time to bind (1 hour)
- Also place 1 ul beads in 1 ml along with 1 ul flourophore.
- Allow beads to bind to flourophore, then spin beads down, remove supernatent and replace with 1 ml water.
- Next place the cells and the beads under the microscope
Procedure
- Set up overnights of parts 48-51. Let grow overnight.
- Dilute 1 ul overnight into 1ml
- Add 1 mm IPTG and let grow for four hours
- After cells have grown up, place in flourophore (1 um) and allow time to bind (1 hour)
- Also place 1 ul beads in 1 ml along with 1 ul flourophore.
- Allow beads to bind to flourophore, then spin beads down, remove supernatent and replace with 1 ml water.
- Read the samples through the flow cytometer
A ROUGH TIMELINE OF THE PROJECT!