Figure 5
Figure 5. Human T-cell development in NSγ mice. (A-E) The development of human T cells was characterized in NSγ thymuses. In some thymuses, the human CD45+ CD3+ T cells included CD4+ CD8+ “double-positive” T-cell progenitors (A), whereas other thymuses contained phenotypically mature “single-positive” T cells (B). High percentages of CD4+ CD8+ T-cell progenitors were observed in thymuses across a range of transplant cell doses (C). Similarly, high copy numbers of human TRECs could be detected in thymus cell preparations across a range of transplant cell doses (D). In 8 of 9 mice that expressed TRECs, at least 25% of the CD3+ cells were CD4+ CD8+ T-cell progenitors (E). (F-M) Human CD3+ T cells isolated from NSγ spleens were tested for their responsiveness to mitogens. In spleen cell preparations, the human CD3+ cells had matured into CD4+ or CD8+ “single-positive” T cells, which expressed CD28 (F-G). The T cells were costimulated using immobilized antibodies directed against CD3 and CD28 and cultured with (n = 6) or without irradiated HUVEC cells (20 Gy; n = 4). After 7 days, human CD45+ CD3+ T cells were present in the cultures, and expressed the CD25 (IL-2Rα) activation antigen (H-I). Both CD4+ and CD8+ were detected; however, most frequently, there was a net loss of T cells in the cultures (J,L). Cultures established CD3+ CB T cells contained similar CD4+ and CD8+ cells, but the numbers of cells increased dramatically in 7 days (K,M).

Human T-cell development in NSγ mice. (A-E) The development of human T cells was characterized in NSγ thymuses. In some thymuses, the human CD45+ CD3+ T cells included CD4+ CD8+ “double-positive” T-cell progenitors (A), whereas other thymuses contained phenotypically mature “single-positive” T cells (B). High percentages of CD4+ CD8+ T-cell progenitors were observed in thymuses across a range of transplant cell doses (C). Similarly, high copy numbers of human TRECs could be detected in thymus cell preparations across a range of transplant cell doses (D). In 8 of 9 mice that expressed TRECs, at least 25% of the CD3+ cells were CD4+ CD8+ T-cell progenitors (E). (F-M) Human CD3+ T cells isolated from NSγ spleens were tested for their responsiveness to mitogens. In spleen cell preparations, the human CD3+ cells had matured into CD4+ or CD8+ “single-positive” T cells, which expressed CD28 (F-G). The T cells were costimulated using immobilized antibodies directed against CD3 and CD28 and cultured with (n = 6) or without irradiated HUVEC cells (20 Gy; n = 4). After 7 days, human CD45+ CD3+ T cells were present in the cultures, and expressed the CD25 (IL-2Rα) activation antigen (H-I). Both CD4+ and CD8+ were detected; however, most frequently, there was a net loss of T cells in the cultures (J,L). Cultures established CD3+ CB T cells contained similar CD4+ and CD8+ cells, but the numbers of cells increased dramatically in 7 days (K,M).

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