Carolyn, My experiences from my previous job: 1) We successfully sorted pre-enriched populations (using the Miltenyi MACS system) with no interference evident. 2) We did not notice a significant diminution of signal when following the purity of MACS enriched populations. We did, however, see a variation in purity depending on the source of cells and the type of purification (positive versus negative selection). By counterstaining the populations, we were able to account for most of the contaminating cells. 3) We did sort rare populations from mouse spleen using a FACStar plus, but I cannot remember the rate. It did take a long time to get a significant number of cells, but we were looking at about a 1% maximum population. Randy Fischer TherImmune Research Corporation 9700 Great Seneca Hwy Rockville, MD 20850 (240) 453-6256 RFischer@therimmune.com > ---------- > From: Carolyn Jefferiss > Sent: Tuesday, August 8, 2000 1:35 AM > To: Cytometry Mailing List > Subject: magnetic beads and/or sorting > > > Dear Everyone, > Three things:- > 1) Magnetic beads and Flow Sorting: > I have presumed that the beds (Miltenyi) would interfere with sorting > by flow cytometry, even though they are absolutely titchy. Please say > if you have sorted cells from a population containing > magnetically-labelled cells, to good effect. > > 2) Magnetically labelled cells: > When checking magnetically labelled and isolated cells for purity by > flow cytometry, has anyone looked at loss of label? I was wondering > whether or not there is a significant loss of label somewhere from > the positive fraction in coming off the column or later. - I do > everything at 4degrees and despite using the usual concentrations of > conjugated second abs see a significant proportion of totally > unlabelled cells in the fraction which was positively bound to the > magnetic column. > > 3)Sorting time: > Finally, When sorting a rare population from whole bone marrow, what > kind of sort rate should be used? How stable could I expect "my" > Vantage to be over the number of hours I'd need to use it? I am > extremely impressed by the indication that other users seem to have a > stable settup for many hours. I have never sorted for more than four > hours. I'd need to run at least 100 million cells to get enough of my > chosen population. > > > Thank you for your attention. > Carolyn Jefferiss > Carolyn Jefferiss Ph. D. > Pharmacy and Pharmacology > University of Bath > Claverton Down > Bath BA2 7HY > >
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