Team:Washington/Protocols/MMAssay
From 2010.igem.org
(Difference between revisions)
Line 58: | Line 58: | ||
*Make one row of blank (1.1x diH2O Master Mix without enzyme) | *Make one row of blank (1.1x diH2O Master Mix without enzyme) | ||
- | ''Prepare Spectramax plate reader with desired settings'' | + | '''Prepare Spectramax plate reader with desired settings''' |
*Pipette 10uL of Substrate into each well. (Column 1 from well 1 of strip tube, Column 2 from well 2 of strip tube, etc.) | *Pipette 10uL of Substrate into each well. (Column 1 from well 1 of strip tube, Column 2 from well 2 of strip tube, etc.) | ||
*Immediately place into Spectramax plate reader and begin reading | *Immediately place into Spectramax plate reader and begin reading | ||
- | Final Concentrations | + | '''Final Concentrations''' |
*Enzyme (CapD) - 5nM (0.00025mg/mL) | *Enzyme (CapD) - 5nM (0.00025mg/mL) | ||
*Amino Acid (L-Glutamate) - 0mM or 5mM | *Amino Acid (L-Glutamate) - 0mM or 5mM |
Revision as of 20:19, 25 October 2010
Michaelis-Menten Assay
Prepare a 10x Master Mix with these concentrations (10uL/rxn)
Make one for each enzyme
- HEPES 7.4 pH (250mM)
- 1% Tween
- Purified Enzyme (50nM)
- Dilute enzyme in 1x HEPES/Tween buffer
Note: Make one without enzyme for blank
Prepare Substrate
- Prepare 10x substrate (10uM) in one well of a 12-well strip tube
- Do half concentration serial dilutions (equal parts diH2O and substrate) until 11th well.
- Leave the 12th well with no substrate
Final Concentrations of Substrate (Left to Right in uM):
10, 5, 2.5, 1.25, 0.625, 0.3125, 0.15625, 0.078125, 0.0390625, 0.01953125, 0.009765625
1.1x Master Mix
- Put equal parts 10x Master Mix and 10x L-Glu eppendorf tube (Referred to as L-Glu Master Mix)
- Put equal parts 10x Master Mix and diH2O in an eppendorf tube (Referred to as diH2O Master Mix)
- Fill each tube with diH2O (70uL/rxn)
Prepare a 96-well plate for transpeptidation
- Pipette 90uL of 1.1x L-Glu Master Mix for one each enzyme across a row for the transpeptidation reaction
- Repeat for each enzyme
- Make one row of blank (1.1x L-Glu Master Mix without enzyme)
Prepare a 96-well plate for hydrolysis
- Pipette 90uL of 1.1 diH2O Master Mix for each different enzyme in each new row
- Repeat for each enzyme
- Make one row of blank (1.1x diH2O Master Mix without enzyme)
Prepare Spectramax plate reader with desired settings
- Pipette 10uL of Substrate into each well. (Column 1 from well 1 of strip tube, Column 2 from well 2 of strip tube, etc.)
- Immediately place into Spectramax plate reader and begin reading
Final Concentrations
- Enzyme (CapD) - 5nM (0.00025mg/mL)
- Amino Acid (L-Glutamate) - 0mM or 5mM
- Substrate - Variable Concentration
- HEPES (7.4pH) - 25mM
- 0.1% Tween
Final Reaction Volume 100uL