Fig. 1.
Fig. 1. Development and expression specificity of β-globin transgenic mice. / (A) Diagram of construct used to make the transgenic line. HS indicates DNAse-1 hypersensitive sites within the β-globin LCR; pβ, β-globin promoter. (B) Peripheral blood from a β-globin transgenic (Tg) mouse (line no. 3) and a wild-type (WT) control, viewed under brightfield or fluorescence microscopy. Original magnification, × 20. The second panel showing fluorescent transgenic erythrocytes represents a higher magnification (× 5 of the original). (C) FACS analysis of the peripheral blood from β-globin ECFP transgenic mice (line nos. 1, 2, 3) and a wild-type (WT) control. (D) FACS profiles of hematopoietic progenitors showing ECFP expression. HSCs were sorted as IL-7Rα−Lin−Sca-1+c-Kit+; CMPs as IL-7Rα−Lin−Sca-1−c-Kit+, CD34+, FCgRl0; GMPs as IL-7Rα−Lin−Sca-1−c-Kit+, CD34+FCgRhi ; MEPs as IL-7Rα−Lin−Sca-1−c-Kit+, CD34−FCgRl0; CLPs as IL-7Rα+Lin−Sca-1loc-Kit+; pro–T cells as CD4loCD8loCD25+c-Kit+, and pro–B cells as B220+IgM−CD43+ populations. Numbers indicate percentages of ECFP-positive cells detected within a given quadrant.

Development and expression specificity of β-globin transgenic mice.

(A) Diagram of construct used to make the transgenic line. HS indicates DNAse-1 hypersensitive sites within the β-globin LCR; pβ, β-globin promoter. (B) Peripheral blood from a β-globin transgenic (Tg) mouse (line no. 3) and a wild-type (WT) control, viewed under brightfield or fluorescence microscopy. Original magnification, × 20. The second panel showing fluorescent transgenic erythrocytes represents a higher magnification (× 5 of the original). (C) FACS analysis of the peripheral blood from β-globin ECFP transgenic mice (line nos. 1, 2, 3) and a wild-type (WT) control. (D) FACS profiles of hematopoietic progenitors showing ECFP expression. HSCs were sorted as IL-7RαLinSca-1+c-Kit+; CMPs as IL-7RαLinSca-1c-Kit+, CD34+, FCgRl0; GMPs as IL-7RαLinSca-1c-Kit+, CD34+FCgRhi ; MEPs as IL-7RαLinSca-1c-Kit+, CD34FCgRl0; CLPs as IL-7Rα+LinSca-1loc-Kit+; pro–T cells as CD4loCD8loCD25+c-Kit+, and pro–B cells as B220+IgMCD43+ populations. Numbers indicate percentages of ECFP-positive cells detected within a given quadrant.

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