![In vivo exposure to ruxolitinib differentially influences T-cell functions.Prf1−∕− mice were infected with LCMV and treated with ruxolitinib as described. On day 9, splenocytes from these animals were restimulated ex vivo with MHC class I (gp33-41)- or class II (gp61-80)-restricted LCMV peptides. Percentages of CD8+CD44+ (A-B [left]) and CD4+CD44+ (C-D [left]) T cells producing both TNFα and IFNγ, or CD8+CD44+ T cells expressing LAMP1 (CD107a; E-F [left]) were determined by intracellular and surface staining and flow cytometry. Absolute number of CD8+CD44+ and CD4+CD44+ T cells producing both TNFα and IFNγ, and CD8+CD44+CD107+ are shown in panels B, D, and F, respectively (right panels). In panels B, D, and F, data are presented as mean ± SD. (G) Viral titer was determined in the liver samples of Prf1−∕− mice in each group. (H) EL4 cells were pulsed with 20 μM gp33-41 peptide or left untreated and used as targets in an in vitro cytotoxicity assay. Cytolysis of gp33-loaded (filled symbols) or unloaded (open symbols) EL4 cells by splenic CD8+CD44+ cells of LCMV-infected or LCMV + ruxolitinib–treated (L+R) B6 mice. Specific lysis was determined by 51Cr release and plotted as the mean ± SD. Statistical significance in percent-specific lysis was determined by 2-way ANOVA. (I) Viral titers in the livers of B6 mice on day 8 (week 1) and day 15 (week 2) postinfection. Data in panels A through G and H and I are representative of 4 and 2 independent experiments, respectively. *P < .05.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/127/13/10.1182_blood-2015-12-684399/5/1666f6.jpeg?Expires=1720440294&Signature=b-WkMFKZQgf-8ECpD4sO5aMS-S9utzg5zZfYqmRHRfoimaNPbq~ku3P4DK78jLlCqTUh~gbkB4KIHOhJjiofBkRZxv4H0qdslm0OKmXQWSyjo-4xzj50gVAxfJsh1ksEl7TsB-kctli5S1F~18DchDRDN70KruelW6bCotj2gcpqKmLNSojTSO7TdDQ731j2uMJqy1CjzY7I-HWbmwNrq0Cmbgn1JXhagiOtwOwKMHaDJYLVuWN9AN0rF1CAHUJI~gmgvFB0dz7wixskokkdiCSTYss4n9kEcBA7RKJYn9z9fqNNk5~LyE4rmjv~d3MMsDoI9DCGWYVAfuorlqabyQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
In vivo exposure to ruxolitinib differentially influences T-cell functions.Prf1−∕− mice were infected with LCMV and treated with ruxolitinib as described. On day 9, splenocytes from these animals were restimulated ex vivo with MHC class I (gp33-41)- or class II (gp61-80)-restricted LCMV peptides. Percentages of CD8+CD44+ (A-B [left]) and CD4+CD44+ (C-D [left]) T cells producing both TNFα and IFNγ, or CD8+CD44+ T cells expressing LAMP1 (CD107a; E-F [left]) were determined by intracellular and surface staining and flow cytometry. Absolute number of CD8+CD44+ and CD4+CD44+ T cells producing both TNFα and IFNγ, and CD8+CD44+CD107+ are shown in panels B, D, and F, respectively (right panels). In panels B, D, and F, data are presented as mean ± SD. (G) Viral titer was determined in the liver samples of Prf1−∕− mice in each group. (H) EL4 cells were pulsed with 20 μM gp33-41 peptide or left untreated and used as targets in an in vitro cytotoxicity assay. Cytolysis of gp33-loaded (filled symbols) or unloaded (open symbols) EL4 cells by splenic CD8+CD44+ cells of LCMV-infected or LCMV + ruxolitinib–treated (L+R) B6 mice. Specific lysis was determined by 51Cr release and plotted as the mean ± SD. Statistical significance in percent-specific lysis was determined by 2-way ANOVA. (I) Viral titers in the livers of B6 mice on day 8 (week 1) and day 15 (week 2) postinfection. Data in panels A through G and H and I are representative of 4 and 2 independent experiments, respectively. *P < .05.
