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Fig.2.C showing Flow cytometry/Cell sorting in a Mus musculus (House mouse) sample from the publication: A Myb enhancer-guided analysis of basophil and mast cell differentiation.
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Macrophage-to-endothelial cell crosstalk by the cholesterol metabolite 27HC promotes atherosclerosis in male mice.

In Nature Communications on 25 July 2023 by Yu, L., Xu, L., et al.

Hypercholesterolemia and vascular inflammation are key interconnected contributors to the pathogenesis of atherosclerosis. How hypercholesterolemia initiates vascular inflammation is poorly understood. Here we show in male mice that hypercholesterolemia-driven endothelial activation, monocyte recruitment and atherosclerotic lesion formation are promoted by a crosstalk between macrophages and endothelial cells mediated by the cholesterol metabolite 27-hydroxycholesterol (27HC). The pro-atherogenic actions of macrophage-derived 27HC require endothelial estrogen receptor alpha (ERα) and disassociation of the cytoplasmic scaffolding protein septin 11 from ERα, leading to extranuclear ERα- and septin 11-dependent activation of NF-κB. Furthermore, pharmacologic inhibition of cyp27a1, which generates 27HC, affords atheroprotection by reducing endothelial activation and monocyte recruitment. These findings demonstrate cell-to-cell communication by 27HC, and identify a major causal linkage between the hypercholesterolemia and vascular inflammation that partner to promote atherosclerosis. Interventions interrupting this linkage may provide the means to blunt vascular inflammation without impairing host defense to combat the risk of atherosclerotic cardiovascular disease that remains despite lipid-lowering therapies.
© 2023. The Author(s).

  • FC/FACS
  • Cell Biology
  • Immunology and Microbiology
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A Myb enhancer-guided analysis of basophil and mast cell differentiation.

In Nature Communications on 18 November 2022 by Matsumura, T., Totani, H., et al.

The transcription factor MYB is a crucial regulator of hematopoietic stem and progenitor cells. However, the nature of lineage-specific enhancer usage of the Myb gene is largely unknown. We identify the Myb -68 enhancer, a regulatory element which marks basophils and mast cells. Using the Myb -68 enhancer activity, we show a population of granulocyte-macrophage progenitors with higher potential to differentiate into basophils and mast cells. Single cell RNA-seq demonstrates the differentiation trajectory is continuous from progenitors to mature basophils in vivo, characterizes bone marrow cells with a gene signature of mast cells, and identifies LILRB4 as a surface marker of basophil maturation. Together, our study leads to a better understanding of how MYB expression is regulated in a lineage-associated manner, and also shows how a combination of lineage-related reporter mice and single-cell transcriptomics can overcome the rarity of target cells and enhance our understanding of gene expression programs that control cell differentiation in vivo.
© 2022. The Author(s).

  • FC/FACS
  • Mus musculus (House mouse)
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A Myb enhancer-guided analysis of basophil and mast cell differentiation.

In Nat Commun on 18 November 2022 by Matsumura, T., Totani, H., et al.

Fig.2.C
Fig.2.C showing Flow cytometry/Cell sorting in a Mus musculus (House mouse) sample from the publication: A Myb enhancer-guided analysis of basophil and mast cell differentiation.
  • FC/FACS
  • Mus musculus (House mouse)
The Myb -68 enhancer is active in Ly6C- GMPs in Myb -68 GFP transgenic mice. GFP activity in whole bone marrow (a), LS-K cells (b), and GMPs (c) of Myb -68 GFP mice. FACS gating strategies are shown in Supplementary Fig. 12. Representative FACS plots of indicated cells from control (grey) and Myb... more
The Myb -68 enhancer is active in Ly6C- GMPs in Myb -68 GFP transgenic mice. GFP activity in whole bone marrow (a), LS-K cells (b), and GMPs (c) of Myb -68 GFP mice. FACS gating strategies are shown in Supplementary Fig. 12. Representative FACS plots of indicated cells from control (grey) and Myb -74 GFP mice (green) are shown. Numbers shown are mean percentages±SD of GFP+ cells in Myb -68 GFP mice. The percentages of GFP+ cells are also shown in the right graphs. an = 10 mice for LSK cells and LS-K cells, and n = 4 mice for others. p = 4.1 × 10−4 by one-way Welch’s ANOVA. ***p < 0.001 by the Games-Howell post hoc test. p = 4.1 × 10−4 between LSK and LS-K, p = 3.7 x 10−4 between CD11b+Gr1+ and LS-K, p = 3.5 x 10−4 between B220+ and LS-K, p = 3.5 x 10−4 between CD4+ and LS-K, p = 3.5 x 10−4 between CD8+ and LS-K, and p = 3.9 × 10−4 between Ter119+- and LS-K. (b) n = 6 mice. p = 5.8 × 10−7 by one-way Welch’s ANOVA. **p < 0.01 by the Games-Howell post hoc test. p = 0.0014 between PreGM and GMP, p = 0.0008 between PreMegE and GMP, p = 0.0007 between PreCFU-E and GMP, p = 0.0006 between CFU-E/ProEry and GMP, and p = 0.0006 between MkP and GMP. cn = 10 mice for Ly6C- GMPs and n = 7 mice for others. p = 8.5 × 10−6 by one-way Welch’s ANOVA. ***p < 0.001 by the Games-Howell post hoc test. p = 1.1 × 10−5 between Ly6C- GMPs and GP, and p = 1.1 × 10−5 between Ly6C- GMPs and MP. LSK Lin-Sca1+cKit+ cells, LS-K Lin-Sca1-cKit+ cells, MkP megakaryocyte progenitor, GMP granulocyte/monocyte progenitor, PreGM pre-granulocyte/macrophage, CFU-E colony-forming unit-erythroid, ProEry pro-erythrocytes, PreCFU-E pre-colony-forming unit-erythroid, PreMegE pre-megakaryocyte/erythrocyte, GP granulocyte progenitor, MP monocyte progenitor. less

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