Figure 3
Figure 3. Decreased functional NK cells in CXCR4 conditionally deficient mice. (A) In vitro cytotoxicity of NK cells in the bone marrow (left and middle) or spleen (right) from pIpC-treated MxCre/CXCR4f/wt or MxCre/CXCR4f/null mice. LDH release assay was used to measure NK lytic activity against the NK cell-sensitive YAC-1 target cells. DX5+ cells purified by magnetic-activated cell sorting (left) and sorted CD3−NK1.1+ NK cells (middle and right) were used as effector cells and were incubated with YAC-1 target cells at the indicated effector-to-target cell ratios (E/T) for 4 hours. Data are representative of 3 experiments; n = 3. *P < .05. (B) Flow cytometric analysis of in vitro IFN-γ production by NK cells in the spleen from pIpC-treated MxCre/CXCR4f/wt or MxCre/CXCR4f/null mice. Splenocytes were stimulated with IL-12 and IL-18 for 6 hours. IFN-γ production was measured in CD3−NK1.1+ NK cells by intracellular staining.

Decreased functional NK cells in CXCR4 conditionally deficient mice. (A) In vitro cytotoxicity of NK cells in the bone marrow (left and middle) or spleen (right) from pIpC-treated MxCre/CXCR4f/wt or MxCre/CXCR4f/null mice. LDH release assay was used to measure NK lytic activity against the NK cell-sensitive YAC-1 target cells. DX5+ cells purified by magnetic-activated cell sorting (left) and sorted CD3NK1.1+ NK cells (middle and right) were used as effector cells and were incubated with YAC-1 target cells at the indicated effector-to-target cell ratios (E/T) for 4 hours. Data are representative of 3 experiments; n = 3. *P < .05. (B) Flow cytometric analysis of in vitro IFN-γ production by NK cells in the spleen from pIpC-treated MxCre/CXCR4f/wt or MxCre/CXCR4f/null mice. Splenocytes were stimulated with IL-12 and IL-18 for 6 hours. IFN-γ production was measured in CD3NK1.1+ NK cells by intracellular staining.

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