Figure 7
Crosstalk between BMSCs and MCs in mouse models. (A) Confocal microscopy analysis for IgD (green), IgM (red), and CD169 (blue) of the spleen of p53+/+ and p53−/− mice shows the expansion of IgMhighIgDlow MZ B cell in p53−/− mice compared with their wild-type counterpart. In p53+/+ mice, MZ B cells are not expanded and confined within the MZ (arrows). Upper panel original magnification ×100; lower panel, original magnification ×200. (B) Representative flow cytometry analysis showing the increased accumulation of CD21/35highIgMhigh in the spleen of p53−/− mice. The complete gating strategy is shown in supplemental Figure 6. (C) Cumulative data showing the increased percentage of MZ B cells in the spleens from p53−/− mice if compared with p53+/+ mice. (D) Confocal microscopy analysis for tryptase (green), IgM (red), and CD29 (blue) performed in the spleen of p53+/+ and p53−/− mice. Representative pictures are shown. In the spleen of p53−/− mice, tryptase+ MCs make contact with CD29+ mesenchymal cells. This interaction does not occur within the spleens of wild-type mice. Original magnification ×400. (E) Confocal microscopy analysis showing the expression of CD40 in the spleen of p53+/+ and p53−/− mice. In wild-type mice, CD40 (green) expression is restricted to the follicular area. In the spleen of p53−/− mice, CD40 is also expressed by mesenchymal CD29+ (red) cells outside the follicular area, which take contact with tryptase+ MCs (blue). Original magnification ×200. (F) TNF production was measured by ELISA in supernatants obtained from BM-MSC and MC cocultures. In this experiment, wild-type or CD40L−/− MCs were treated with 100 ng/mL LPS for 4 hours, washed, and than added to a monolayer of BM mesenchymal SCs for 24 hours. Each bar, untreated (black bars) or stimulated (white bars), represents the mean ± standard deviation of 2 independent cocultures.

Crosstalk between BMSCs and MCs in mouse models. (A) Confocal microscopy analysis for IgD (green), IgM (red), and CD169 (blue) of the spleen of p53+/+ and p53−/− mice shows the expansion of IgMhighIgDlow MZ B cell in p53−/− mice compared with their wild-type counterpart. In p53+/+ mice, MZ B cells are not expanded and confined within the MZ (arrows). Upper panel original magnification ×100; lower panel, original magnification ×200. (B) Representative flow cytometry analysis showing the increased accumulation of CD21/35highIgMhigh in the spleen of p53−/− mice. The complete gating strategy is shown in supplemental Figure 6. (C) Cumulative data showing the increased percentage of MZ B cells in the spleens from p53−/− mice if compared with p53+/+ mice. (D) Confocal microscopy analysis for tryptase (green), IgM (red), and CD29 (blue) performed in the spleen of p53+/+ and p53−/− mice. Representative pictures are shown. In the spleen of p53−/− mice, tryptase+ MCs make contact with CD29+ mesenchymal cells. This interaction does not occur within the spleens of wild-type mice. Original magnification ×400. (E) Confocal microscopy analysis showing the expression of CD40 in the spleen of p53+/+ and p53−/− mice. In wild-type mice, CD40 (green) expression is restricted to the follicular area. In the spleen of p53−/− mice, CD40 is also expressed by mesenchymal CD29+ (red) cells outside the follicular area, which take contact with tryptase+ MCs (blue). Original magnification ×200. (F) TNF production was measured by ELISA in supernatants obtained from BM-MSC and MC cocultures. In this experiment, wild-type or CD40L−/− MCs were treated with 100 ng/mL LPS for 4 hours, washed, and than added to a monolayer of BM mesenchymal SCs for 24 hours. Each bar, untreated (black bars) or stimulated (white bars), represents the mean ± standard deviation of 2 independent cocultures.

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