Fig. 1.
Fig. 1. Expression of RAG1/GFP signal in the peripheral lymphoid organs. / (A) Flow cytometric analysis of the GFP expression in B220+cells of the spleen, Peyer patch, axillary LN, and mesenteric LN of heterozygous rag1/gfp knockin mouse (left). Five percent of splenic B cells expressing the highest level of GFP are shown in the gated area on the left of panel A. Next, splenic B220+ B cells were separated into GFP−, GFPlow, and GFPhigh populations by cell sorter using gates shown in the left panel. The RNA isolated from each cell population was used for reverse transcriptase–PCR (RT-PCR) with gene specific primers for RAG1, GFP, and HPRT, respectively (right). Only the GFPhighB cells showed rag1 mRNA. (B) Flow cytometric analysis of the splenic B cells. GFP signal was compared in B220+ cell fractions further separated by staining with sIgM (G1, G2, G3, and G4), CD43 (G5 and G6), and HSA+ (G7 and G8). GFP signals in splenic B cells were also analyzed in different fractions stained with sIgM+ and sIgD+ (T1, T2, and M). For regions G1 to G8, the vertical bars to the right of each histogram show the percentage of B220+ cells represented by each gate that were GFP+. (C) Fluorescence microscopy analysis of GFP signal. The upper panels show GFP signals of purified splenic cells sorted with B220+ from WT or RAG1/GFP knockin mice. The middle panels show tissue sections from thymus and spleen of WT or RAG1/GFP mice analyzed for GFP expression. The bottom panels show the same sections stained with H&E (middle panels). Original magnification, 100 ×.

Expression of RAG1/GFP signal in the peripheral lymphoid organs.

(A) Flow cytometric analysis of the GFP expression in B220+cells of the spleen, Peyer patch, axillary LN, and mesenteric LN of heterozygous rag1/gfp knockin mouse (left). Five percent of splenic B cells expressing the highest level of GFP are shown in the gated area on the left of panel A. Next, splenic B220+ B cells were separated into GFP, GFPlow, and GFPhigh populations by cell sorter using gates shown in the left panel. The RNA isolated from each cell population was used for reverse transcriptase–PCR (RT-PCR) with gene specific primers for RAG1, GFP, and HPRT, respectively (right). Only the GFPhighB cells showed rag1 mRNA. (B) Flow cytometric analysis of the splenic B cells. GFP signal was compared in B220+ cell fractions further separated by staining with sIgM (G1, G2, G3, and G4), CD43 (G5 and G6), and HSA+ (G7 and G8). GFP signals in splenic B cells were also analyzed in different fractions stained with sIgM+ and sIgD+ (T1, T2, and M). For regions G1 to G8, the vertical bars to the right of each histogram show the percentage of B220+ cells represented by each gate that were GFP+. (C) Fluorescence microscopy analysis of GFP signal. The upper panels show GFP signals of purified splenic cells sorted with B220+ from WT or RAG1/GFP knockin mice. The middle panels show tissue sections from thymus and spleen of WT or RAG1/GFP mice analyzed for GFP expression. The bottom panels show the same sections stained with H&E (middle panels). Original magnification, 100 ×.

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