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Found 3 matching solutions for this experiment
Upstream tips |
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. Each cell type was single cell suspended and, incubated in FACS buffer containing pre-conjugated antibodies (see supplementary Table 2) for 20 min on ice. Following incubation, cells were washed twice with FACS buffer. |
All the flow cytometry performed using a Cell Lab Quanta SCMPL. The data were analyzed using Kaluza®1.2 software (Beckman Coulter, Denmark) and the expression of each CD markers on the cells was calculated based on the percentage and mean fluorescence intensity (MFI). |
Protocol tips |
. Each cell type was single cell suspended and, incubated in FACS buffer containing pre-conjugated antibodies (see supplementary Table 2) for 20 min on ice. Following incubation, cells were washed twice with FACS buffer. |
Downstream tips |
All the flow cytometry performed using a Cell Lab Quanta SCMPL. The data were analyzed using Kaluza®1.2 software (Beckman Coulter, Denmark) and the expression of each CD markers on the cells was calculated based on the percentage and mean fluorescence intensity (MFI). |
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Transfer 10 μl of the cell suspension to a 5-ml FACS tube containing 190 μl WM and leave on ice. This is the unstained control sample. |
Add 190 μl WM into each tube and 10 μl of the cell suspension. Add PI so that the final concentration is 0.3 μg/ml, add 0.25 μl Ab |
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Upstream tips |
Transfer 10 μl of the cell suspension to a 5-ml FACS tube containing 190 μl WM and leave on ice. This is the unstained control sample. |
Protocol tips |
Add 190 μl WM into each tube and 10 μl of the cell suspension. Add PI so that the final concentration is 0.3 μg/ml, add 0.25 μl Ab |
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Add the following volumes of primary antibodies to together the original 2 ml sort samples: 10 μl biotin Ly-6A/E-Sca1 |
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Protocol tips |
Add the following volumes of primary antibodies to together the original 2 ml sort samples: 10 μl biotin Ly-6A/E-Sca1 |
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