CD101 Surface Expression Discriminates Potency Among Murine FoxP3 super(+) Regulatory T Cells
CD4 super(+)CD25 super(+)FoxP3 super(+) regulatory T cells (Treg) have been shown to be protective in animal models of autoimmunity and acute graft-vs-host disease. However, owing to the functional heterogeneity among CD4 super(+)CD25 super(+) T cells, surface markers expressed selectively on functi...
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Veröffentlicht in: | Journal of Immunology 2007-09, Vol.179 (5), p.2808-2814 |
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description | CD4 super(+)CD25 super(+)FoxP3 super(+) regulatory T cells (Treg) have been shown to be protective in animal models of autoimmunity and acute graft-vs-host disease. However, owing to the functional heterogeneity among CD4 super(+)CD25 super(+) T cells, surface markers expressed selectively on functionally active Treg would be useful for purposes of identifying and isolating such cells. We generated a rabbit mAb against murine CD101, a transmembrane glycoprotein involved in T cell activation. Among freshly isolated T cells, CD101 was detected on 25-30% of CD4 super(+)CD25 super(+) Treg and similar to 20% of conventional memory T cells. CD101 super(high) Treg displayed greater in vitro suppression of alloantigen-driven T cell proliferation as compared with CD101 super(low) Treg. In a model of graft-vs-host disease induced by allogeneic bone marrow transplantation in vivo bioluminescence imaging demonstrated reduced expansion of donor-derived luciferase-labeled conventional T cells in mice treated with CD101 super(high) Treg, compared with CD101 super(low) Treg. Moreover, treatment with CD101 super(high) Treg resulted in improved survival, reduced proinflammatory cytokine levels and reduced end organ damage. Among the CD101 super(high) Treg all of the in vivo suppressor activity was contained within the CD62L super(high) subpopulation. We conclude that CD101 expression distinguishes murine Treg with potent suppressor activity. |
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However, owing to the functional heterogeneity among CD4 super(+)CD25 super(+) T cells, surface markers expressed selectively on functionally active Treg would be useful for purposes of identifying and isolating such cells. We generated a rabbit mAb against murine CD101, a transmembrane glycoprotein involved in T cell activation. Among freshly isolated T cells, CD101 was detected on 25-30% of CD4 super(+)CD25 super(+) Treg and similar to 20% of conventional memory T cells. CD101 super(high) Treg displayed greater in vitro suppression of alloantigen-driven T cell proliferation as compared with CD101 super(low) Treg. In a model of graft-vs-host disease induced by allogeneic bone marrow transplantation in vivo bioluminescence imaging demonstrated reduced expansion of donor-derived luciferase-labeled conventional T cells in mice treated with CD101 super(high) Treg, compared with CD101 super(low) Treg. Moreover, treatment with CD101 super(high) Treg resulted in improved survival, reduced proinflammatory cytokine levels and reduced end organ damage. Among the CD101 super(high) Treg all of the in vivo suppressor activity was contained within the CD62L super(high) subpopulation. 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However, owing to the functional heterogeneity among CD4 super(+)CD25 super(+) T cells, surface markers expressed selectively on functionally active Treg would be useful for purposes of identifying and isolating such cells. We generated a rabbit mAb against murine CD101, a transmembrane glycoprotein involved in T cell activation. Among freshly isolated T cells, CD101 was detected on 25-30% of CD4 super(+)CD25 super(+) Treg and similar to 20% of conventional memory T cells. CD101 super(high) Treg displayed greater in vitro suppression of alloantigen-driven T cell proliferation as compared with CD101 super(low) Treg. In a model of graft-vs-host disease induced by allogeneic bone marrow transplantation in vivo bioluminescence imaging demonstrated reduced expansion of donor-derived luciferase-labeled conventional T cells in mice treated with CD101 super(high) Treg, compared with CD101 super(low) Treg. Moreover, treatment with CD101 super(high) Treg resulted in improved survival, reduced proinflammatory cytokine levels and reduced end organ damage. Among the CD101 super(high) Treg all of the in vivo suppressor activity was contained within the CD62L super(high) subpopulation. 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However, owing to the functional heterogeneity among CD4 super(+)CD25 super(+) T cells, surface markers expressed selectively on functionally active Treg would be useful for purposes of identifying and isolating such cells. We generated a rabbit mAb against murine CD101, a transmembrane glycoprotein involved in T cell activation. Among freshly isolated T cells, CD101 was detected on 25-30% of CD4 super(+)CD25 super(+) Treg and similar to 20% of conventional memory T cells. CD101 super(high) Treg displayed greater in vitro suppression of alloantigen-driven T cell proliferation as compared with CD101 super(low) Treg. In a model of graft-vs-host disease induced by allogeneic bone marrow transplantation in vivo bioluminescence imaging demonstrated reduced expansion of donor-derived luciferase-labeled conventional T cells in mice treated with CD101 super(high) Treg, compared with CD101 super(low) Treg. Moreover, treatment with CD101 super(high) Treg resulted in improved survival, reduced proinflammatory cytokine levels and reduced end organ damage. Among the CD101 super(high) Treg all of the in vivo suppressor activity was contained within the CD62L super(high) subpopulation. We conclude that CD101 expression distinguishes murine Treg with potent suppressor activity.</abstract></addata></record> |
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title | CD101 Surface Expression Discriminates Potency Among Murine FoxP3 super(+) Regulatory T Cells |
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