Figure 2.
Figure 2. Mouse Gr-1+ granulocytes do not express gzmA or gzmB intracellularly. All indicated cell populations were stained, intracellularly, with either rabbit αmgzmAIS followed by FITC-labeled αrabbit IgG (1:500) or with APC-labeled αhugzmB mAb; rabbit IgG and mouse IgG were used as isotype control, as described in “Flow cytometry.” Analysis was performed using FACSCalibur. (A) 1.3E6SN, EL4.F15:αmgzmA IS (1:1000), αhugzmB mAb (1:100). (Bi) Ex vivo-derived LCMV-immune (day 8 after infection) spleen cells from B6, gzmA-/-, and gzmB-/- mice were stained with αCD8 mAb (1:100) and, subsequently, with either αmgzmA IS (1:100), or αhugzmB (1:1000) mAb for intracellular expression of gzms and analyzed as described in “Flow cytometry.” (Bii) In vitro-propagated alloreactive (H-2b anti-H-2d; third stimulation) T cells from B6, gzmA-/-, and gzmB-/- mice were treated as in panel Bi. (Ci) In vitro-generated granulocytes (BM cells, day 9, G-CSF) from either B6, gzmA-/-, or gzmB-/- mice were stained with the αGr-1 mAb and, subsequently, with either αmgzmA IS (1:100) or αhugzmB (1:10) mAb for intracellular expression of gzms, as described in “Flow cytometry.” (Cii) Alternatively, in vitro-enriched B6 granulocytes were sensitized to either LPS (1 μg/mL) or Lip-OspA (10 μg/mL) for 8 hours, prior to phenotypic analysis, using αGr-1 mAb and either αmgzmA IS (1:100) or αhugzmb (1:10) mAb for intracellular expression of gzms as described above. Numbers in graphs indicate the percentages of gated cells.

Mouse Gr-1+ granulocytes do not express gzmA or gzmB intracellularly. All indicated cell populations were stained, intracellularly, with either rabbit αmgzmAIS followed by FITC-labeled αrabbit IgG (1:500) or with APC-labeled αhugzmB mAb; rabbit IgG and mouse IgG were used as isotype control, as described in “Flow cytometry.” Analysis was performed using FACSCalibur. (A) 1.3E6SN, EL4.F15:αmgzmA IS (1:1000), αhugzmB mAb (1:100). (Bi) Ex vivo-derived LCMV-immune (day 8 after infection) spleen cells from B6, gzmA-/-, and gzmB-/- mice were stained with αCD8 mAb (1:100) and, subsequently, with either αmgzmA IS (1:100), or αhugzmB (1:1000) mAb for intracellular expression of gzms and analyzed as described in “Flow cytometry.” (Bii) In vitro-propagated alloreactive (H-2b anti-H-2d; third stimulation) T cells from B6, gzmA-/-, and gzmB-/- mice were treated as in panel Bi. (Ci) In vitro-generated granulocytes (BM cells, day 9, G-CSF) from either B6, gzmA-/-, or gzmB-/- mice were stained with the αGr-1 mAb and, subsequently, with either αmgzmA IS (1:100) or αhugzmB (1:10) mAb for intracellular expression of gzms, as described in “Flow cytometry.” (Cii) Alternatively, in vitro-enriched B6 granulocytes were sensitized to either LPS (1 μg/mL) or Lip-OspA (10 μg/mL) for 8 hours, prior to phenotypic analysis, using αGr-1 mAb and either αmgzmA IS (1:100) or αhugzmb (1:10) mAb for intracellular expression of gzms as described above. Numbers in graphs indicate the percentages of gated cells.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal