Figure 3
Figure 3. NKp80+ effector CD8 T cells possess an inflammatory NK-like phenotype. (A) NKp80+ and NKp80− cells within the effector memory CD8 subset (CCR7− CD8+ αβ TCR+) in freshly isolated PBMCs (pooled from 6 donors and depleted of CD4+ and CD14+ cells) were sorted by FACS for transcriptional profiling by microarray analysis. (B) Signal intensities of mRNA microarrays for FACS-sorted NKp80+ versus NKp80− cells. One dot represents expression of one gene. Differentially expressed genes are listed in Table 1. (C-F) Flow cytometric analysis of effector memory CD8 T cells (CCR7− CD8+ αβ TCR+) for coexpression of NKp80 and various cell surface receptors selected on the basis of differential mRNA expression in NKp80+ versus NKp80− subsets of CCR7− CD8+ T cells (see Table 1). (C) Results for a representative donor. For analysis of most surface molecules, respective histograms for NKp80+ (dark gray) and NKp80− cells (light gray) are overlaid. Coexpression of 4-1BBL and CD161, respectively, with NKp80 is shown in dot plots. (D,E) Data compiled from 3 donors and depicted either as fold change in MFI in NKp80+ versus NKp80− cells (D) or percentage of marker-positive cells (E) among NKp80+ cells (■) and NKp80− cells (). Mean values of data are shown with error bars indicating standard deviation. For analysis of NKR-P1A/CD161 in (D), only MFI of the CD161+ subpopulation were considered. (F) Coexpression of PD-1 and KLRG1, respectively, with NKp80 on effector memory CD8 T cells (CCR7− CD8+ αβ TCR+) of 2 representative donors.

NKp80+ effector CD8 T cells possess an inflammatory NK-like phenotype. (A) NKp80+ and NKp80 cells within the effector memory CD8 subset (CCR7 CD8+ αβ TCR+) in freshly isolated PBMCs (pooled from 6 donors and depleted of CD4+ and CD14+ cells) were sorted by FACS for transcriptional profiling by microarray analysis. (B) Signal intensities of mRNA microarrays for FACS-sorted NKp80+ versus NKp80 cells. One dot represents expression of one gene. Differentially expressed genes are listed in Table 1. (C-F) Flow cytometric analysis of effector memory CD8 T cells (CCR7 CD8+ αβ TCR+) for coexpression of NKp80 and various cell surface receptors selected on the basis of differential mRNA expression in NKp80+ versus NKp80 subsets of CCR7 CD8+ T cells (see Table 1). (C) Results for a representative donor. For analysis of most surface molecules, respective histograms for NKp80+ (dark gray) and NKp80 cells (light gray) are overlaid. Coexpression of 4-1BBL and CD161, respectively, with NKp80 is shown in dot plots. (D,E) Data compiled from 3 donors and depicted either as fold change in MFI in NKp80+ versus NKp80 cells (D) or percentage of marker-positive cells (E) among NKp80+ cells (■) and NKp80 cells (). Mean values of data are shown with error bars indicating standard deviation. For analysis of NKR-P1A/CD161 in (D), only MFI of the CD161+ subpopulation were considered. (F) Coexpression of PD-1 and KLRG1, respectively, with NKp80 on effector memory CD8 T cells (CCR7 CD8+ αβ TCR+) of 2 representative donors.

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