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PU.1/Spi-B Regulation of c-rel Is Essential for Mature B Cell Survival

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Presentation on theme: "PU.1/Spi-B Regulation of c-rel Is Essential for Mature B Cell Survival"— Presentation transcript:

1 PU.1/Spi-B Regulation of c-rel Is Essential for Mature B Cell Survival
Cheng-Jun Hu, Sridhar Rao, Diana L. Ramirez-Bergeron, Lee Ann Garrett-Sinha, Steve Gerondakis, Marcus R. Clark, M.Celeste Simon  Immunity  Volume 15, Issue 4, Pages (October 2001) DOI: /S (01)

2 Figure 1 Northern Blot Analysis of 3H12 in Splenic B Cells and Hematopoietic Cell Lines (A) Northern blot analysis of 3H12 expression in purified splenic B cells (more than 90% B220+ based on flow cytometry) from PU.1+/+ Spi-B+/+, PU.1+/−Spi-B+/+, PU.1+/+Spi-B−/−, and PU.1+/−Spi-B−/− mice. The same blot was then stripped and reprobed with an actin probe for RNA loading control. The 3H12 expression level is shown as a percentage of wild-type cells after normalization for RNA loading. Similar results were obtained from multiple mice. (B) Expression of 3H12 in murine hematopoietic cell lines using Northern blot analysis of total RNA prepared from pro-B (NFS 70 c/10), pre-B (70 z/3 and 38 B9), immature B (WeHi 231), mature B (A20), mature T (RMA), immature T (EL-4), macrophage (J774.1), erythroid (MEL), and fibroblast (3T3) cells. 28S rRNA is shown as a loading control Immunity  , DOI: ( /S (01) )

3 Figure 2 The Murine c-rel Promoter Contains at Least Three PU.1/Spi-B Binding Sites (A) Sequences of five potential PU.1/Spi-B binding sites in the murine c-rel promoter are shown with GGAA core sequences boxed. PU.1 and Spi-B consensus binding sites are also shown. (B) EMSAs of three PU.1/Spi-B binding sites in the c-rel promoter using PU.1 or Spi-B IVT proteins are shown. (C) An EMSA of the −474 PU.1/Spi-B binding site using nuclear extracts prepared from A20 mature B cells is shown. PI stands for preimmune serum Immunity  , DOI: ( /S (01) )

4 Figure 3 Three PU.1/Spi-B Binding Sites in the c-rel Promoter Are Important for c-rel Promoter Activity (A) A schematic diagram of the c-rel promoter reporter is shown with three PU.1/Spi-B binding sites indicated. In tmRelGH, three PU.1/Spi-B binding sites were mutated. The arrow indicates the transcription start site. (B) A functional examination of PU.1/Spi-B binding sites for c-rel promoter activity using transient transfection of the wild-type c-rel promoter (pRelGH) or the promoter with PU.1/Spi-B sites mutated (tmRelGH) in several cell lines. The data represent results obtained from four independent experiments. (C) PU.1 and Spi-B transactivate the c-rel promoter reporter in 3T3 cells. PU.1 or Spi-B expression vectors (or mutants lacking transactivation or Ets DNA binding domains) were tranfected into 3T3 cells with the wild-type c-rel promoter reporter. The data represent mean fold induction in comparison to the empty pcDNA3 vector from four independent experiments Immunity  , DOI: ( /S (01) )

5 Figure 4 Reintroduction of Rel Protein Restores Bone Marrow B Cell Numbers in Mice Reconstituted with PU.1+/−Spi-B−/− Bone Marrow Cells (A) A diagram of the Rel retrovirus construct. 5′ LTR-mediated transcription generates a bicistronic mRNA, with the GFP reading frame accessed by an internal ribosomal entry site (IRES). (B) Representative data from a single mouse are shown. The source of bone marrow and the type of retrovirus with which they were infected specified four categories of reconstituted mice; PU.1+/−Spi-B−/−/GFP-reconstituted mice are boxed. The percentages of GFP+ (column I) and B220+/IgM+ (column II) cells from total bone marrow were determined by immunostaining and flow cytometry. GFP+ (column III) or GFP− (column IV) populations were then analyzed for numbers of B220+/IgM+ cells Immunity  , DOI: ( /S (01) )

6 Figure 5 Reintroduction of Rel Protein Restores Splenic B Cell Numbers to Mice Reconstituted with PU.1+/−Spi-B−/− Bone Marrow Cells The arrangement of data is identical to that of Figure 4; besides the B220+/IgM+ immature B cells, IgM+/IgD+ mature B cells are also shown Immunity  , DOI: ( /S (01) )

7 Figure 6 Overexpression of Bcl-2 Gene Increased the B Cell Numbers in PU.1+/−Spi-B−/− Bone Marrow and Spleen PU.1+/−Spi-B−/−/Bcl-2 mice were generated by crossing PU.1+/−Spi-B−/− mice with Bcl-2 transgenic mice. Two- to three-month-old animals were sacrificed, and single-cell suspensions were prepared from the bone marrow and spleen for flow cytometry analysis of IgM+/B220+ or IgM+/IgD+ B cells Immunity  , DOI: ( /S (01) )

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