Team:TU Darmstadt/Protocols/Antibody staining

(Difference between revisions)

Latest revision as of 21:19, 26 September 2012

centrifuge 750 µL of cell suspension for 2 min in order to gain pellet
wash the pellet two times with 200 µL PBS buffer (after every wash centrifuge for 2 min)
add 30 µL of 1. antibody 1:10 concentration in PBS buffer
incubate suspension including antibody for 10 min. on ice
centrifuge for 2 min.
wash pellet three times with 200 µL PBS buffer (after every wash centrifuge for 2 min)
add 10 µL of 2. antibody 1:10 concentration in PBS buffer
incubate suspension including antibody for at least 30 min on ice
centrifuge for 2 min
wash pellet three times with 200 µL PBS buffer (after every wash centrifuge for 2 min)
add 10 µL of SAPE 1:10 concentration in PBS buffer
incubate on ice for 10 min.
wash two times with 200 µL PBS buffer

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 # incubate on ice for 10 min.
 # wash two times with 200 µL PBS buffer
-* now your cells are ready to be detected with FACS or fluorescent microscopy
+* now your cells are ready to be detected via flow cytometry