Figure 2
Figure 2. Recent thymic emigrants CD4+ do not proliferate more than peripheral CD4+ T cells during IL-7 therapy. (A) Schematic of the experimental design where CD45.2+CD4+PERIGFP+, CD45.2+CD4+PERIGFP−, and thymic CD45.2+CD8−CD4+SPTGFP+ cells were sorted from LNs or thymuses of CD45.2+Rag−/−GFP mice and stained with CFSE prior to their transfer into CD45.1+C57BL/6 mice. Recipient mice were then treated with PBS (vehicle) or rhIL-7 (10 μg/day) for 6 days. (B) Representative flow cytometric analysis of CFSE (CTV)–labeled CD4+PERIGFP+ and CD4+PERIGFP− and CD4+SPTGFP+ found in the LN of PBS- and IL-7–treated animals 7 days post transfer. (C) Graphic summary of the percentage of proliferating cells ± standard error of CD4+PERIGFP+, CD4+PERIGFP−, and CD4+SPTGFP+ based on the dilution of CFSE staining after 6 days of IL-7 therapy. (D) Phenotypic analysis of CD4+PERIGFP+, CD4+PERIGFP−, and CD4+SPTGFP+. Data show 2 animals per group from 2 experiments.

Recent thymic emigrants CD4+ do not proliferate more than peripheral CD4+ T cells during IL-7 therapy. (A) Schematic of the experimental design where CD45.2+CD4+PERIGFP+, CD45.2+CD4+PERIGFP, and thymic CD45.2+CD8CD4+SPTGFP+ cells were sorted from LNs or thymuses of CD45.2+Rag−/−GFP mice and stained with CFSE prior to their transfer into CD45.1+C57BL/6 mice. Recipient mice were then treated with PBS (vehicle) or rhIL-7 (10 μg/day) for 6 days. (B) Representative flow cytometric analysis of CFSE (CTV)–labeled CD4+PERIGFP+ and CD4+PERIGFP and CD4+SPTGFP+ found in the LN of PBS- and IL-7–treated animals 7 days post transfer. (C) Graphic summary of the percentage of proliferating cells ± standard error of CD4+PERIGFP+, CD4+PERIGFP, and CD4+SPTGFP+ based on the dilution of CFSE staining after 6 days of IL-7 therapy. (D) Phenotypic analysis of CD4+PERIGFP+, CD4+PERIGFP, and CD4+SPTGFP+. Data show 2 animals per group from 2 experiments.

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