To all, We only run the unstained COMP bead as our negative controls, autofluorescense has little or NO effect on compensation. You can empirically test this by setting up COMPS both ways. Cell autofluorescense is different for different lasers the beads do not, except in the near UV range. To properly set compensation, you must ensure that: (1) Your compensation control is at least as bright as your stained sample (2) When, for any given fluorochrome compensation control, you are comparing a positive to a negative (or dim) population, both populations have the same autofluorescence (e.g., both + and - are macrophages, or both are lymphocytes, or both are beads) (3) You do not change any instrument settings such as PMT voltages of the fluorescence channels between collecting the compensation control and collecting your sample. The standard COMP beads (kappa-antibody labelled) do have limitations where cells will be required, such as the use of interculating viability dyes or CFSE. In addition, they can not capture lambda antibodies. SP ======================================================= Stephen P. Perfetto, MS.,MT. (ASCP) Manager, Core Flow Cytometry Facility Vaccine Research Center, NIH Building 40 40 Convent Dr., Room 5507 Bethesda, MD 20892-3015 email: sperfetto@nih.gov Phone: (301) 594-8659 Disclaimer: The information in this e-mail and any of its attachments is confidential and may contain sensitive information. It should not be used by anyone who is not the original intended recipient. If you have received this e-mail in error please inform the sender and delete it from your mailbox or any other storage devices. The National Institute of Allergy and Infectious Diseases (NIAID) shall not accept liability for any statement made that are the sender's own and not expressly made on behalf of the NIAID by one of its representatives. > ---------- > From: Rick Dunham > Sent: Tuesday, November 29, 2005 6:10 PM > To: Cytometry Mailing List > Subject: Comp beads and negative populations > > Hello list, > > We recently started using Ig capture beads for compensation and are > in a debate over whether to use unstained cells or unstained beads as > the negative population in automatic compensation with DiVa or > FlowJo. One 'school of thought' is that the positive and negative > populations should have the same autofluorescent properties, thus > dictating that one should use unstained beads as the universal > negative population. The other 'school of thought' is that the > negative population should have the same autofluorescent properties > as the sample, dictating that one should use unstained cells as the > universal negative population. Both arguments seem to have merit, > though looking at previous discussions of autofluorescence and > compensation on this list and in BD and FlowJo literature, > autofluorescense is thought to have little effect on compensation. > > However, one can imagine a scenario from the 'old days' of manual > compensation when for many, the goal was equalization of the median > of the positive and negative populations for a given stained channel > vs the other unstained channels, in which different autofluorescent > properties of the experimental sample vs the compensation sample > would generate over or under compensation, if the mean > autofluorescence of one channel of the negative events were > significantly different with respect to another channel. > > This is where we are in this discussion. Does anyone out there in > the ether have a solution or any comments? What do you do when using > beads? > > Rick Dunham > Graduate Student > Emory Vaccine Center > Emory University > Atlanta, GA USA > > rdunham@emory.edu > >Received on Thu Dec 1 14:58:00 2005
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