The RB6-8C5 monoclonal antibody reacts strongly with mouse Ly6G and weakly with mouse Ly6C previously referred to as GR-1. Ly6G is a 21-25 kDa member of the Ly-6 superfamily of GPI-anchored cell surface proteins with roles in cell signaling and cell adhesion. Ly6G is expressed differentially during development by cells in the myeloid lineage including monocytes macrophages granulocytes and
CD11b+Ly6C high (Ly6Chi) cells (inflammatory monocytes) and CD11b+Ly6C low cells (reparative monocytes) were recruited into the liver following I/R injury. Treatment with clodronate‑loaded liposomes, which transiently deplete systemic macrophages, alleviated hepatic damage.
Product Specific Information Description: The monoclonal antibody HK1.4 recognizes mouse Ly-6C, a GPI-linked protein of the Ly6 family. Ly-6C is found on monocytes/macrophages, endothelial cells and granulocytes as well as a subset of lymphocytes. (B) Gating strategy of gut macrophages (CD45 + Ly6G − Siglec F − CD11b + CD64 + CD11c int MHCII + Ly6C −) of 8-week-old mice. LIMITATIONS This protocol meets the basic needs for analyzing myeloid cells in most organs, but was not optimized for all organs.
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Accumulation of monocytes/macrophages in the infarcted myocardium involves an early lymphocyte antigen 6 complex, locus C (Ly6C)highinflammatory phase, and a later Ly6Clowphase linked to angiogenesis and the formation of an extracellular matrix (4, 7). Ly6C low MerTK + macrophages appeared later, expressed CD206, CD11c, and MHC class II, produced cytokines consistent with repair function, and lacked a gene expression profile compatible with mesenchymal transition or fibroblastic transdifferentiation. In skin, the inflammatory Mo/MΦ population was defined as Live Ly6G-CD11b+Ly6C+F4/80lo/-, while mature MΦ were gated as Live Ly6G-CD11b+ Ly6C- F4/80+. Mo were defined as Ly6G-cKit-CD11b+CD115+Ly6Chi/lo in bone marrow and Ly6G-CD11b+CD115+Ly6Chi/lo in peripheral blood. Markers such as CD11b, CD11c, F4/80, Gr-1, Ly6C, and Ly6G have long been used to identify various splenic cell myeloid populations. Flow cytometry and fluorescence-activated cell sorting (FACS) analysis demonstrated that Ly6G/Ly6C markers are superior to Gr-1 for identifying splenic neutrophils, eosinophils, and subsets of monocytes/macrophages. The Ly6C+Ly6G- (top, open histograms) and Ly6C+Ly6G+ (bottom, open histograms) CD11b+ monocyte subpopulations were analyzed for the expression of various cytokines/effector molecules using antibodies (A-D) or a reactive dye triggered by exposure to ROS (E) and compared to CD11b- cells (filled histograms).
Markers such as CD11b, CD11c, F4/80, Gr-1, Ly6C, and Ly6G have long been used to identify various splenic cell myeloid populations. Flow cytometry and fluorescence-activated cell sorting (FACS) analysis demonstrated that Ly6G/Ly6C markers are superior to Gr-1 for identifying splenic neutrophils, eosinophils, and subsets of monocytes/macrophages.
Ly6C. CD11b. Nov 27, 2018 Macrophages are known for their classical function as antimicrobial phagocytes but support immune function as well by the presentation of developing bone marrow macrophages; including CD11b CD31 CD44 Ly6C Ly6G F4/80 Mac2 c-Fos as well as c-Fms.
(D) Representative FACS plots of CD11b+,Ly6G+Ly6C- neutrophils, Ly6C high Ly6G- monocytes, and F4/80+ macrophages in the blood of CVB3-infected mice treated with anti-Ly6G or anti-Gr1 on day7 p.i. (pre
Because Ly6C Lo [Lin − Ly6G − CD11b +] monocyte/macrophages represent more of a hybrid picture between in vitro M1 and M2 macrophages, it is possible that the use of traditional in vitro macrophage characterization for this cell population in wound healing is not practical, as has been previously suggested.
CD45+. Ly6G. Gated on .
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Flow cytometry and fluorescence-activated cell sorting (FACS) analysis demonstrated that Ly6G/Ly6C markers are superior to Gr-1 for identifying splenic neutrophils, eosinophils, and subsets of monocytes/macrophages.
The number of retrieved anti‐Ly6G‐FITC + cells was reduced significantly in comparison with anti‐Ly6G‐APC + or anti‐Ly6G‐PE + cells.
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macrophages, having an enlarged macrophage-like scatter and expressing high levels of F4/80 (Fig. 1A and D). Remark-ably, distinct subsets of TAMs were clearly distinguishable: Ly6C intMHC IIhi (Ly6C TAMs, gate 2), Ly6ClowMHC IIhi (MHC IIhi TAMs, gate 3), and Ly6ClowMHC IIlow (MHC IIlow TAMs,gate4).ThemajorityofLy6ClowMHC II− cells were CCR3
Here, we show that infiltrating Ly6C hi monocytes, th … Neutrophils were defined as CD11b + Ly6C lo CX 3 CR1-GFP − Ly6G + cells, while monocytes were defined as CD11b + Ly6C hi CX 3 CR1-GFP + MHCII − Ly6G − cells. KC and MoMF expressed similar levels of the macrophage markers F4/80, CD64 (FcγR), and MHCII, but could clearly be discriminated according to presence and absence of the CX 3 CR1-GFP label (Figure 1 D). 2017-06-26 So panel should include CD11b, CD115, Ly6c, Ly6g (or use SSC with high voltage). Can also include CD45 as you want to gate for the CD45+ population. You do not need F4/80. 2020-06-19 Gr-1 is comprised of two components: Ly6C and Ly6G. Ly6G is exclusively expressed on neutrophils.
The RB6-8C5 monoclonal antibody reacts strongly with mouse Ly6G and weakly with mouse Ly6C previously referred to as GR-1. Ly6G is a 21-25 kDa member of the Ly-6 superfamily of GPI-anchored cell surface proteins with roles in cell signaling and cell adhesion. Ly6G is expressed differentially during development by cells in the myeloid lineage including monocytes macrophages granulocytes and
(D) Representative FACS plots of CD11b+,Ly6G+Ly6C- neutrophils, Ly6C high Ly6G- monocytes, and F4/80+ macrophages in the blood of CVB3-infected mice treated with anti-Ly6G or anti-Gr1 on day7 p.i.
Neutrophils were defined as CD11b + Ly6C lo CX 3 CR1-GFP − Ly6G + cells, while monocytes were defined as CD11b + Ly6C hi CX 3 CR1-GFP + MHCII − Ly6G − cells. KC and MoMF expressed similar levels of the macrophage markers F4/80, CD64 (FcγR), and MHCII, but could clearly be discriminated according to presence and absence of the CX 3 CR1 Ly6C, and Ly6G have long been used to identify various splenic cell myeloid popula-tions.