Figure 5
Figure 5. D6active B1 cells in omentum, blood, spleen, mesenteric lymph node, and Peyer patches. (A) Overlaid CCL2AF647 uptake profiles for WT (black) and D6-deficient (KO, gray) omental CD19+ B-cell subsets (identified using Abs against CD5, CD11b, and CD23 as in the analysis of peritoneal cavity lavage cells). Numbers above plots show proportion of retrieved CD19+ cells in each subset in WT mice (means ± SEM). B1d cells (CD19+CD11b−CD5−CD23−D6active) are indicated in the far right plot. (B) Contour plot showing CD11b expression on CD19+ blood cells with the proportion of CD19+ CD11b+ cells indicated. Overlaid CCL2AF647 uptake profiles are shown in the right panels (WT, black; D6-deficient (KO), gray). (C) Contour plots showing gating of CD19+ splenocytes for FO/T2 cells, MZ B cells, and B1 cells fractionated into CD21+ (B121+) and CD21− (B121−) subsets. Events in gate R1 (CD5hi) are rare T/B-cell conjugates and were excluded. The CD19+IgMhiCD23loCD5−CD21− population, containing T1 progenitors, are labeled ‘21−'. The overlaid histograms show CCL2AF647 uptake profiles for WT (black) and D6-deficient (KO; gray) subsets. (D-E) CD19+ cells in mesenteric lymph node and pooled Peyer patches fractionated into CD23lo, CD23med, and CD23hi subsets (central dot plot in each figure). Subset size, as a proportion of retrieved WT CD19+ cells, is indicated above each CCL2AF647 uptake dot plot. The mean ± SEM of CCL2AF647-positive cells (as a proportion of retrieved CD19+ cells) is indicated on each plot. All data are representative of experiments repeated 2-5 times.

D6active B1 cells in omentum, blood, spleen, mesenteric lymph node, and Peyer patches. (A) Overlaid CCL2AF647 uptake profiles for WT (black) and D6-deficient (KO, gray) omental CD19+ B-cell subsets (identified using Abs against CD5, CD11b, and CD23 as in the analysis of peritoneal cavity lavage cells). Numbers above plots show proportion of retrieved CD19+ cells in each subset in WT mice (means ± SEM). B1d cells (CD19+CD11bCD5CD23D6active) are indicated in the far right plot. (B) Contour plot showing CD11b expression on CD19+ blood cells with the proportion of CD19+ CD11b+ cells indicated. Overlaid CCL2AF647 uptake profiles are shown in the right panels (WT, black; D6-deficient (KO), gray). (C) Contour plots showing gating of CD19+ splenocytes for FO/T2 cells, MZ B cells, and B1 cells fractionated into CD21+ (B121+) and CD21 (B121−) subsets. Events in gate R1 (CD5hi) are rare T/B-cell conjugates and were excluded. The CD19+IgMhiCD23loCD5CD21 population, containing T1 progenitors, are labeled ‘21'. The overlaid histograms show CCL2AF647 uptake profiles for WT (black) and D6-deficient (KO; gray) subsets. (D-E) CD19+ cells in mesenteric lymph node and pooled Peyer patches fractionated into CD23lo, CD23med, and CD23hi subsets (central dot plot in each figure). Subset size, as a proportion of retrieved WT CD19+ cells, is indicated above each CCL2AF647 uptake dot plot. The mean ± SEM of CCL2AF647-positive cells (as a proportion of retrieved CD19+ cells) is indicated on each plot. All data are representative of experiments repeated 2-5 times.

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