Fig. 3.
Fig. 3. Flow cytometric analysis and immunoglobulin gene rearrangement studies of tumor cells from transgenic animals. (A) Flow cytometric analysis of involved tissues from from affected mice. I-line mice and N-line mice with lymphoma phenotype (I-836) show a large population of early B cells (B220+, CD3−, CD43+, BP-1+, CD117+, IgM−) in lymph node tumors (shown), as well as in bone marrow, spleen, and peripheral blood (data not shown). N-line animals with leukemic phenotype (N-2051) do not have adenopathy, but show a similar immunophenotype in the spleen (shown), marrow and blood (not shown). Normal cells can also be seen in these samples. Cells from an N-line animal with mediastinal tumor phenotype (N-2288) show tumor cells that are CD3+, B220−, CD2+, aβTCR+, and both CD4+/CD8+, as well as CD4+/CD8− and CD4−/CD8+. (B-D) Immunoglobulin and T-cell receptor gene rearrangements in tumors from transgenic animals. (B)EcoRI digests, μVJ probe; faint low–molecular-weight bands in transgenic samples are due to nonspecific probe binding. (C)EcoRI + BamHI digests, kC probe; (D) HindIII digests, βTCR probe. Southern blot analyses of genomic DNA from tumor samples show clonal rearrangements of the immunoglobulin heavy-chain locus in I-line mice. The N-line founder shows a clonal rearrangement of the βTCR locus. Conversely, tumors from I-line mice do not show rearrangements of the kappa light-chain locus or βTCR locus. Genomic tail DNA from an unaffected littermate is used as a control and the germline bands are indicated by an arrow.

Flow cytometric analysis and immunoglobulin gene rearrangement studies of tumor cells from transgenic animals. (A) Flow cytometric analysis of involved tissues from from affected mice. I-line mice and N-line mice with lymphoma phenotype (I-836) show a large population of early B cells (B220+, CD3, CD43+, BP-1+, CD117+, IgM) in lymph node tumors (shown), as well as in bone marrow, spleen, and peripheral blood (data not shown). N-line animals with leukemic phenotype (N-2051) do not have adenopathy, but show a similar immunophenotype in the spleen (shown), marrow and blood (not shown). Normal cells can also be seen in these samples. Cells from an N-line animal with mediastinal tumor phenotype (N-2288) show tumor cells that are CD3+, B220, CD2+, aβTCR+, and both CD4+/CD8+, as well as CD4+/CD8 and CD4/CD8+. (B-D) Immunoglobulin and T-cell receptor gene rearrangements in tumors from transgenic animals. (B)EcoRI digests, μVJ probe; faint low–molecular-weight bands in transgenic samples are due to nonspecific probe binding. (C)EcoRI + BamHI digests, kC probe; (D) HindIII digests, βTCR probe. Southern blot analyses of genomic DNA from tumor samples show clonal rearrangements of the immunoglobulin heavy-chain locus in I-line mice. The N-line founder shows a clonal rearrangement of the βTCR locus. Conversely, tumors from I-line mice do not show rearrangements of the kappa light-chain locus or βTCR locus. Genomic tail DNA from an unaffected littermate is used as a control and the germline bands are indicated by an arrow.

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