ELISA (aka Enzyme-Linked Immunosorbent Assay) Professor C. Roth 125:315: BME Measurements and Analysis Laboratory Spring 2003
Welcome message from author
This document is posted to help you gain knowledge. Please leave a comment to let me know what you think about it! Share it to your friends and learn new things together.
Transcript
ELISA(aka Enzyme-Linked
Immunosorbent Assay)
Professor C. Roth125:315: BME Measurements and
Analysis LaboratorySpring 2003
What is an ELISA?
• Enzyme-linked immunosorbent assay• Name suggests three components
– Antibody• Allows for specific detection of analyte of interest
– Solid phase (sorbent)• Allows one to wash away all the material that is not
specifically captured– Enzymatic amplification
• Allows you to turn a little capture into a visible color change that can be quantified using an absorbance plate reader
What is it used for?
• Measure antibody levels (allergies, vaccines)
• Detect viruses (hepatitis, HIV, venereal diseases)
• Detect hormonal changes (pregnancy)• Detect circulatory inflammatory markers
(cytokines)
Advantages
• Sensitivity• Quantitative• Reproducible• Kit format
Relative sensitivities of tests (approx)
Usual operating range [Ab] or [Ag]
precipitationimmunoelectrophoresisdouble/radial diffusion
10 g/ml - 1 mg/ml
immunofluorescence 0.1 - 10 g/ml
ELISA (colour) 0.1 - 10 ng/ml (chemiluminescence) 0.01 - 10 ng/ml
radioimmunoassay 0.01 - 10 ng/ml
Enzymes with Chromogenic Substrates
• High molar extinction coefficient (i.e., strong color change)
• Strong binding between enzyme and substrate (low KM)
• Linear relationship between color intensity and [enzyme]
Antibodies• Specificity• Diversity – hypervariable region (2020 ~
1026 combinations; human make ~ 108)• Affinity – range 105 < K < 109 M-1
Capture and Detection Antibodies
Sandwich ELISA
Competitive ELISA
• Less is more. More antigen in your sample will mean more antibody competed away, which will lead to less signal
Today’s Lab
• Our antigen = human albumin• Our antibody = rabbit anti-human• Our enzyme = horseradish peroxidase
• You will develop (i.e. perform enzymatic reaction) using o-phenylene diamine (OPD). It is hazardous. Please wear gloves and treat with respect.
Antibody Steps
• Antigen (purified albumin) is already coated onto microwell plates
• You will add standards and samples in triplicate• You will incubate for 60 minutes at 37 degrees C
to allow for Ab-Ag binding50 50 50
25 25 25
10 10 10
5 5 5
2.5 2.5 2.5
1 1 1
0.5 0.5 0.5
0 0 0
= standardU = unknown
U1 U1 U1
U2 U2 U2
U3 U3 U3
U4 U4 U4
= blank
Data Analysis
• Standard Curve in Excel– Insert chart– Insert trendline (logarithmic)
• T-test– Ttest(array1, array2, tails, type)
Sample Standard Curve
y = -0.0583Ln(x) + 0.3858R2 = 0.9919
0
0.05
0.1
0.15
0.2
0.25
0.3
0.35
0.4
0.45
0.5
0.1 1 10 100
Concentration (ug/mL)Ab
orba
nce
(490
nm
)
absorbance
Log. (absorbance)
Related Documents
