Fig. 1.
Fig. 1. Higher levels of human cell engraftment in NOD/SCID/B2mnull mice. / (A) Summary of engraftment levels in mice transplanted with enriched cord blood CD34+ cells. Similar percentage of human engraftment was detected by either Southern blot with human-specific α satellite probe (open circles) or by flow cytometry using human-specific anti CD45 mAb (filled circles). NOD/SCID mice were transplanted with 8 × 104 cells per mouse and NOD/SCID/B2mnull mice with 4 × 104 cells per mouse, in 5 independent experiments. (B) Bone marrow cells of mice presented in A were assayed for colony formation in semisolid culture selective for the growth of human colonies. Data shown are mean ± SE of 5 experiments. (C) Human DNA in the bone marrow of primary NOD/SCID/B2mnullmice transplanted with 103 CD34+ cells (lanes 1-3) and NOD/SCID mice transplanted with 104CD34+ cells (lanes 4-6). Secondary NOD/SCID/B2mnull recipients were transplanted with 2 to 5 × 103 human CD34+ cells that were recovered from engrafted primary NOD/SCID mice (lanes 7, 8). (D) NOD/SCID mice were transplanted with 12.5 × 104cord blood MNC per mouse (DI) and NOD/SCID/B2mnull mice with 8 × 104or 5 × 104 cord blood MNC per mouse (DII and DVI, respectively). Bone marrow cells from transplanted mice were analyzed 1 month later for the presence of human CD45+cells (R2). Human lineage-specific mAb were used to detect lymphoid CD45+CD19+ (DII, DVI, R1), myeloid CD45+CD33+ (DIII), and immature CD34+CD38−/low (DIV) progenitor cells in the marrow of engrafted NOD/SCID/B2mnull mice. Lymphoid CD45+CD56+ NK cell differentiation was induced in vitro before analysis (DV). A representative mouse out of 9 in 3 different experiments is shown.

Higher levels of human cell engraftment in NOD/SCID/B2mnull mice.

(A) Summary of engraftment levels in mice transplanted with enriched cord blood CD34+ cells. Similar percentage of human engraftment was detected by either Southern blot with human-specific α satellite probe (open circles) or by flow cytometry using human-specific anti CD45 mAb (filled circles). NOD/SCID mice were transplanted with 8 × 104 cells per mouse and NOD/SCID/B2mnull mice with 4 × 104 cells per mouse, in 5 independent experiments. (B) Bone marrow cells of mice presented in A were assayed for colony formation in semisolid culture selective for the growth of human colonies. Data shown are mean ± SE of 5 experiments. (C) Human DNA in the bone marrow of primary NOD/SCID/B2mnullmice transplanted with 103 CD34+ cells (lanes 1-3) and NOD/SCID mice transplanted with 104CD34+ cells (lanes 4-6). Secondary NOD/SCID/B2mnull recipients were transplanted with 2 to 5 × 103 human CD34+ cells that were recovered from engrafted primary NOD/SCID mice (lanes 7, 8). (D) NOD/SCID mice were transplanted with 12.5 × 104cord blood MNC per mouse (DI) and NOD/SCID/B2mnull mice with 8 × 104or 5 × 104 cord blood MNC per mouse (DII and DVI, respectively). Bone marrow cells from transplanted mice were analyzed 1 month later for the presence of human CD45+cells (R2). Human lineage-specific mAb were used to detect lymphoid CD45+CD19+ (DII, DVI, R1), myeloid CD45+CD33+ (DIII), and immature CD34+CD38−/low (DIV) progenitor cells in the marrow of engrafted NOD/SCID/B2mnull mice. Lymphoid CD45+CD56+ NK cell differentiation was induced in vitro before analysis (DV). A representative mouse out of 9 in 3 different experiments is shown.

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