User:Torsten Waldminghaus/flow cytometry notes: Difference between revisions

Revision as of 05:58, 14 April 2008

1x TBS with 20mM Tris used for flow cytometry in Skarstad-Lab (reduced NaCl concentration from 150mM in the usual TBS to 130mM (everything else is the same).

When started new no washing is required but before starting with samples one should press 'Prime' without any liquid (never have 'Prime' with liquid!!!' to let run air run through the system.

Start software FACSDiva
Select Instrument Configuration
- Select presettings of Gunnar F
Go to Cellbiology > Torsten > new exp. (brown icon) > rename (torsten date)>
press syringe icon
go to 'tube_001' > things will show up on right screen
make local sheet by pressing on icon on left top
Create diagrams:
- Click on DotPlot icon and than on the sheet
- Axes can be changed by clicking on the axe-title
- Make dot plot with FITC versus Hoechst
- Make 4 histograms:

Go to Instruments > Parameters > Voltage:
- SSC: 500
- Hoechst: adjust later using the standart /linear scale
- FITC: 580 /log scale
Go to Instruments > Threshhold:
- Press Add two times; delete SSCA and change Hoechst to 5000 for Standard (for samples it should be 2000)
Go to laser and set windows ext. to 2000
UV delay is 40.000 and can be changed if one gets strange results.

@@ Line 36: / Line 36: @@
 **Make 4 histograms:
 #Count/SSCA
-#Cont/Hoechst
+#Count/Hoechst
-#Cont/FITC
+#Count/FITC
-#Cont/Hoechst
+#Count/Hoechst
-*Go
+*Go to Instruments > Parameters > Voltage:
+**SSC: 500
+**Hoechst: adjust later using the standart /linear scale
+**FITC: 580 /log scale
+*Go to Instruments > Threshhold:
+**Press Add two times; delete SSCA and change Hoechst to 5000 for Standard (for samples it should be 2000)
+*Go to laser and set windows ext. to 2000
+*UV delay is 40.000 and can be changed if one gets strange results.