Difference between revisions of "Bradford Assay"
From Bridges Lab Protocols
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Protein Lysate Bradford Assay | Protein Lysate Bradford Assay | ||
#Dilute reagent 5X in water, stable for 2-3 weeks | #Dilute reagent 5X in water, stable for 2-3 weeks | ||
− | #In a 96 well plate, dilute sample 20X (190ul | + | #In a 96 well plate, dilute sample 20X (190ul H2O, 10ul Sample) |
#Add 5ul of sample to 100ul of reagent in well | #Add 5ul of sample to 100ul of reagent in well | ||
#Run "Bradford Assay Protocol" on Plate Reader | #Run "Bradford Assay Protocol" on Plate Reader |
Revision as of 15:51, 8 August 2017
Materials
- BioRad Protein Assay Dye Reagent Concentrate cat#500-0006
- Disposable Plastic Cuvette
- 0.1mg/mL BSA in H20 as standard
Protocol
Cuvette Bradford Assay
- Dilute reagent 5X in water, stable for 2-3 weeks
- Pipet 1 mL into disposable plastic cuvette
- Add 1-10 uL of protein sample, cover with parafilm and mix
- Let sit 5-10 min to react
- Set spectrophotometer as follows:
- Go to protein assay then Bradford assay
- Set formula, then select more
- Set b=0.045 (or determine slope)
- Set dilution to be 1/vol (ie 0.1 for 10 uL)
- Blank then measure samples, absorbance must be less than 0.9
- Print (hit Recall, then enter, then print) and attach to experiment
Protein Lysate Bradford Assay
- Dilute reagent 5X in water, stable for 2-3 weeks
- In a 96 well plate, dilute sample 20X (190ul H2O, 10ul Sample)
- Add 5ul of sample to 100ul of reagent in well
- Run "Bradford Assay Protocol" on Plate Reader
Reference
- Wikipedia: Bradford Protein Assay
- PMID 942051