7 Questions 16 Answers 0 Followers
Questions related from Komal k kumar j
Can anyone tell me how to save the cells (Human Leukemic cell lines) after treating with drugs before preparing proteins for Mass spectra? i have other things to do so i have planned to save the...
17 December 2014 5,697 2 View
Hi I am defining populations of spleen and bone marrow based on surface markers, but I am confused with TCR beta, CD69. What population is positive to these markers?Thanks
04 December 2014 5,990 7 View
Hi guys. Can anyone tell me the suitable stimulation conditions to stimulate pStat1, pStat3, pStat4, p38 and pAkt. I am working with mouse spleen, bone marrow and murine cell line BaF3. I am...
25 November 2014 3,054 4 View
I performed multicolour analysis in flow cytometry. I stained for FITC, PercpCy5, PercpCy7, PE and PB on cancer cells. I compensated using Beads and used FMos for gating population, but when I run...
11 April 2014 9,137 13 View
In flow cytometry single histogram of a single phosphoprotein splitted into two peaks. Even that is a stable cancer cell line. Why is this?
28 December 2013 9,732 1 View
I added PI to the cell line that I am interested to exclude dead cells. Then run the experiment in FACS canto. But GFP is sowing the peak at 10 to the power of 5 in FITC channel for all the...
18 December 2013 10,036 4 View
I am working on phosphoflow in FACS and have stained the cells with surface markers and intercellular markers. I got the FSC and SCC results and histogram but I am confused about how to interpret...
07 November 2013 8,434 3 View
