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Quantitating Fluorescence Intensity from Fluorophore: The Definition of MESF Assignment
Authors:Abe Schwartz  Lili Wang  Edward Early  Adolfas Gaigalas  Yu-zhong Zhang  Gerald E Marti  Robert F Vogt
Affiliation:Center for Quantitative Cytometry, PO Box 194344, San Juan, Puerto Rico, 00919;National Institute of Standards and Technology, Gaithersburg, MD 20899-8312;Molecular Probes, Inc., PO Box 22010, Eugene, OR 97402-0469;Center for Biologics Evaluation and Research, U.S. Food and Drug Administration, NIH Building 29B, Room 2NN08, Bethesda, MD 20892;Division of Laboratory Sciences, CDC, Mailstop F19, 4770 Buford Highway, Atlanta, GA 30341
Abstract:The quantitation of fluorescence radiance may at first suggest the need to obtain the number of fluorophore that are responsible for the measured fluorescence radiance. This goal is beset by many difficulties since the fluorescence radiance depends on three parameters 1) the probability of absorbing a photon (molar extinction), 2) the number of fluorophores, and 3) the probability of radiative decay of the excited state (quantum yield). If we use the same fluorophore in the reference solution and the analyte then, to a good approximation, the molar extinction drops out from the comparison of fluorescence radiance and we are left with the comparison of fluorescence yield which is defined as the product of fluorophore concentration and the molecular quantum yield. The equality of fluorescence yields from two solutions leads to the notion of equivalent number of fluorophores in the two solutions that is the basis for assignment of MESF (Molecules of Equivalent Soluble Fluorophore) values. We discuss how MESF values are assigned to labeled microbeads and by extension to labeled antibodies, and how these assignments can lead to the estimate of the number of bound antibodies in flow cytometer measurements.
Keywords:flow cytometer  fluorescein  fluorescence  MESF  microbeads  quantitation  SRM 1932
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