Haynes:ELISA: Difference between revisions
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'''Cell lysis''' | '''Cell lysis''' | ||
# | # Standard protein prep procedure | ||
'''Bradford assay''' | '''Bradford assay''' | ||
# | # See the [Haynes:Bradford Bradford Assay Protocol] | ||
'''Protein-well binding''' | '''Protein-well binding''' |
Revision as of 19:23, 1 July 2013
ELISA Assay
Enzyme-linked immunosorbent assay
by Karmella Haynes, 2013
Principle: Proteins are captured on the bottom of a micro well plate, either by direct binding or by a conjugated antibody "trap". A second antibody is added to detect one specific type of protein. A counter-stain antibody (usually HRP-conjugated) is used to generate visible signal, which is proportional to the number of proteins. Normalization (e.g., using the number of cells per lysate sample, and a purified protein with known concentration if you're fortunate to have one available) can be used to calculate proteins per cell.
DIRECT ELISA
This key feature of this approach is the attachment of proteins directly to the bottom surfaces of the micro wells. A specific protein is detected with a primary and secondary-HRP. The advantage over "sandwich" ELISA is that fewer antibodies are needed, but this method is known to be less sensitive/ accurate. Because of this I recommend this method for artificially over-expressed or abundant naturally expressed proteins.
MATERIALS
- Well-Coated Amine Binding, 8 well strip plate, clear (G Bioscience #786-753)
- FemtoELISA-HRP kit (G Biosciences #786-110)
PROCEDURE
Cell lysis
- Standard protein prep procedure
Bradford assay
- See the [Haynes:Bradford Bradford Assay Protocol]
Protein-well binding
Primary antibody
Secondary antibody-HRP
What to do with your data: calculate unknown protein concentration(s) per cell