My question is related to interpreting results by Flow Cytometry.
Let’s say I have a background level of staining of Isotype-FITC at 100 MFI units. Then, let’s say I have protein A-FITC, which stains at 20,000 MFI units, and Protein B-FITC which stains at 10,000 MFI units. Assume that the staining for A and B are of equivalent affinity and kinetics.
To find the relative levels, do I divide numbers, like this:
A/bkgd = 20,000/100 = 200; B/bkgd = 10,000/100 = 100; A-B = 200-100 = 100 unit difference, and A/B = 2.00 fold difference
Or do I subtract numbers to quantify changes in protein levels, like this:
A- bkgd: 20,000-100 = 19,900; B-bkgd = 10,000-100 = 9,900; A-B = 19,900 - 9,900 = 10,000 unit difference, and A/B = 2.01 fold difference.
Also, is there a reference for this?
in order to standardize your different samples within the same experiment or from different experiments, it is better to use the Ration of Fluorescence Intensity (RFI) instead of MFI.
for each sample is calculated from the MFI of your staining divided by the MFI of your neg or isotope control.
From your example your prof A would have a RFI of 200 and prot B of 100.
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