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On. We found that CD4+CD252Nrp1+ T cells 1516647 suppress anti-donor T cell responses in vitro. In combination with short-term immunosuppression (non-therapeutic dose of Rapamycin), CD4+CD252Nrp1+ T cells significantly prolonged the survival of heart grafts in a fully MHC-mismatched model. Nrp1 was initially described as semaphorin-3A and VEGF receptor, being essential for axonal guidance and vascularization,respectively [11,12]. In the immune system, Nrp1 has been shown to be involved in the priming of T cells by DC [23] and in the regulation of the immunological synapse and response [24,25]. According to the study from Bruder and colleagues [13], Nrp1 represents a surface marker for the identification of Treg cells. Because it is highly expressed on CD4+CD25+ cells, and significantly down-regulated in activated CD4+CD25?T cells. Moreover, CD4+Nrp1high T cells suppress proliferation of naive CD4+CD25?T cells, whereas CD4+Nrp1low cells lack this capacity. However, as reported by Milpied et al., Nrp1 might only represent a novel activation marker of human T cells but not a specific marker of human Tregs, because human Foxp3+ Tregs do not specifically express Nrp1 and Nrp1 expression is induced on peripheral blood T lymphocytes upon in vitro activation as well [26]. Inconsistently, another study has found a population of Nrp1+ Treg in human lymph nodes with Foxp3 expression that exerted contact-dependent suppression of T cell proliferation [27]. Recently, Nrp1 has been reported to be expressed at high levels by most natural Tregs, but at low levels by mucosa-generated and other noninflammatory inducible Tregs, which therefore makes Nrp1 a good surface marker to distinguish natural and inducible Tregs in vivo [28,29]. While these contradictory results remain to be explained by further investigation, Battaglia’s finding that Nrp1 was also expressed on some CD4+CD25int and CD4+CD252 T cells correlates well with our previous findings in mouse [15,27].CD4+CD252Nrp1+ T Cells Prevent Cardiac RejectionFigure 4. CD4+CD252Nrp1+ T cells augment CD4+Foxp3+ Treg accumulation in transplant recipients. (A) Anti-CD4 and anti-Foxp3 intracellular staining were performed on spleen cells harvested from untreated mice on 7d or from Rapamycin and/or CD4+CD252Nrp1+ T cells on 21d, 42d and 70d. (B) The percentages of CD4+Foxp3+ T cells were pooled from 4? mice from each group. (C) CD4+CD25+ T cells were purified from each group and used for suppression assays. 26104 CD4+CD252 T cells (C57BL/6) were stimulated by the same amount of irradiated BALB/c splenocytes together with various doses of CD4+CD25+T cells purified from the indicated group. Cell proliferation was determined by 3H thymidine incorporation. Results are presented as mean 6 SD values of triplicate wells, and are representative of 3 independent experiments. *P,0.05, **P,0.01, ***P,0.001. Rapa = Rapamycin, Nrp1 = neuropilin-1, 3H-TdR = metabolic incorporation of PHCCC chemical information tritiated thymidine, cpm = cells per million, Treg = T regulatory cells doi:10.1371/journal.pone.0061151.gIt has been reported that Nrp1 expressed on Tregs prolongs the interaction between Tregs and immature DCs, allowing Tregs more time to recognize MHC class II-peptide complexes presented by iDCs, which results in higher sensitivity when limiting BTZ043 amounts of antigen are present[30]. Moreover, Nrp1 is a receptor for TGF-b1 and activates its latent form, which is also relevant to the Tregs’ activity [31]. These findings suggest thatbesides being a surf.On. We found that CD4+CD252Nrp1+ T cells 1516647 suppress anti-donor T cell responses in vitro. In combination with short-term immunosuppression (non-therapeutic dose of Rapamycin), CD4+CD252Nrp1+ T cells significantly prolonged the survival of heart grafts in a fully MHC-mismatched model. Nrp1 was initially described as semaphorin-3A and VEGF receptor, being essential for axonal guidance and vascularization,respectively [11,12]. In the immune system, Nrp1 has been shown to be involved in the priming of T cells by DC [23] and in the regulation of the immunological synapse and response [24,25]. According to the study from Bruder and colleagues [13], Nrp1 represents a surface marker for the identification of Treg cells. Because it is highly expressed on CD4+CD25+ cells, and significantly down-regulated in activated CD4+CD25?T cells. Moreover, CD4+Nrp1high T cells suppress proliferation of naive CD4+CD25?T cells, whereas CD4+Nrp1low cells lack this capacity. However, as reported by Milpied et al., Nrp1 might only represent a novel activation marker of human T cells but not a specific marker of human Tregs, because human Foxp3+ Tregs do not specifically express Nrp1 and Nrp1 expression is induced on peripheral blood T lymphocytes upon in vitro activation as well [26]. Inconsistently, another study has found a population of Nrp1+ Treg in human lymph nodes with Foxp3 expression that exerted contact-dependent suppression of T cell proliferation [27]. Recently, Nrp1 has been reported to be expressed at high levels by most natural Tregs, but at low levels by mucosa-generated and other noninflammatory inducible Tregs, which therefore makes Nrp1 a good surface marker to distinguish natural and inducible Tregs in vivo [28,29]. While these contradictory results remain to be explained by further investigation, Battaglia’s finding that Nrp1 was also expressed on some CD4+CD25int and CD4+CD252 T cells correlates well with our previous findings in mouse [15,27].CD4+CD252Nrp1+ T Cells Prevent Cardiac RejectionFigure 4. CD4+CD252Nrp1+ T cells augment CD4+Foxp3+ Treg accumulation in transplant recipients. (A) Anti-CD4 and anti-Foxp3 intracellular staining were performed on spleen cells harvested from untreated mice on 7d or from Rapamycin and/or CD4+CD252Nrp1+ T cells on 21d, 42d and 70d. (B) The percentages of CD4+Foxp3+ T cells were pooled from 4? mice from each group. (C) CD4+CD25+ T cells were purified from each group and used for suppression assays. 26104 CD4+CD252 T cells (C57BL/6) were stimulated by the same amount of irradiated BALB/c splenocytes together with various doses of CD4+CD25+T cells purified from the indicated group. Cell proliferation was determined by 3H thymidine incorporation. Results are presented as mean 6 SD values of triplicate wells, and are representative of 3 independent experiments. *P,0.05, **P,0.01, ***P,0.001. Rapa = Rapamycin, Nrp1 = neuropilin-1, 3H-TdR = metabolic incorporation of tritiated thymidine, cpm = cells per million, Treg = T regulatory cells doi:10.1371/journal.pone.0061151.gIt has been reported that Nrp1 expressed on Tregs prolongs the interaction between Tregs and immature DCs, allowing Tregs more time to recognize MHC class II-peptide complexes presented by iDCs, which results in higher sensitivity when limiting amounts of antigen are present[30]. Moreover, Nrp1 is a receptor for TGF-b1 and activates its latent form, which is also relevant to the Tregs’ activity [31]. These findings suggest thatbesides being a surf.

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Author: Potassium channel