Key Product Details

Species Reactivity

Validated:

Human

Cited:

Human

Applications

Validated:

Western Blot, Flow Cytometry, CyTOF-ready

Cited:

Immunohistochemistry-Paraffin

Label

Unconjugated

Antibody Source

Polyclonal Goat IgG
View all M-CSF R/CD115 Primary Antibodies »

Product Specifications

Immunogen

Mouse myeloma cell line NS0-derived recombinant human M-CSF R/CD115
Ile20-Glu512
Accession # CAA27300

Specificity

Detects human M-CSF R/CD115 in direct ELISAs and Western blots.

Clonality

Polyclonal

Host

Goat

Isotype

IgG

Scientific Data Images for Human M-CSF R/CD115 Antibody

Detection of M-CSF R/CD115 in THP-1 cells by Flow Cytometry

THP-1 cells were stained with Goat Anti-Human M-CSF R/CD115 Antigen Affinity-purified Polyclonal Antibody (Catalog # AF329, filled histogram) or isotype control antibody (Catalog # AB-108-C, open histogram) followed by Allophycocyanin-conjugated Anti-Goat IgG Secondary Antibody (Catalog # F0108). View our protocol for Staining Membrane-associated Proteins.
Detection of M-CSF R/CD115 by Western Blot

Detection of M-CSF R/CD115 by Western Blot

MTX modulates the expression of MAF, MAFB, and CSF1R in M-MØ. a Schematic representation of the experiment. Monocytes were differentiated to macrophages in the presence of M-CSF for 7 days. Five micromolar MTX was added once on monocytes [MTX-M-MØ], or on 2 days (MTX-M-MØ [d2]) or 5 days (MTX-M-MØ [d5]) after the beginning of the differentiation process with M-CSF. RNA or protein levels were determined at day 7. b Relative mRNA expression levels of the indicated genes as determined by qRT-PCR on M-MØ, MTX-M-MØ, MTX-M-MØ (d2), and MTX-M-MØ (d5). Mean ± SEM of three independent donors are shown. Groups were compared by applying one-way ANOVA (with Tukey's post hoc test, *p < 0.05). c Scatter plot of RNAseq results showing upregulated expression gene changes in MTX-M-MØ versus MTX-M-MØ (d5). d Venn diagram comparing the genes differentially expressed by MTX in MTX-M-MØ with the genes significantly altered by MTX in and MTX-M-MØ (d5). e Allogeneic CD3+ T-lymphocyte proliferation promoted by M-MØ and MTX-M-MØ (d5). Shown are two experiments using independent preparations of M-MØ. Mean ± SEM of six replicates performed in each experiment are shown (**p < 0.01). f Immunoblot analysis of CSF1R, MAFB, and MAF by M-MØ and MTX-M-MØ (d5). GAPDH protein levels were determined as protein loading control. g Immunoblot analysis of CSF1R and MAFB by M-MØ, MTX-M-MØ (d5), or MTX-M-MØ (d5) exposed to FA. Tubulin protein levels were determined as protein loading control. Image collected and cropped by CiteAb from the following open publication (https://pubmed.ncbi.nlm.nih.gov/36380627), licensed under a CC-BY license. Not internally tested by R&D Systems.
Detection of M-CSF R/CD115 by Western Blot

Detection of M-CSF R/CD115 by Western Blot

MTX modulates the expression of MAF, MAFB, and CSF1R in M-MØ. a Schematic representation of the experiment. Monocytes were differentiated to macrophages in the presence of M-CSF for 7 days. Five micromolar MTX was added once on monocytes [MTX-M-MØ], or on 2 days (MTX-M-MØ [d2]) or 5 days (MTX-M-MØ [d5]) after the beginning of the differentiation process with M-CSF. RNA or protein levels were determined at day 7. b Relative mRNA expression levels of the indicated genes as determined by qRT-PCR on M-MØ, MTX-M-MØ, MTX-M-MØ (d2), and MTX-M-MØ (d5). Mean ± SEM of three independent donors are shown. Groups were compared by applying one-way ANOVA (with Tukey's post hoc test, *p < 0.05). c Scatter plot of RNAseq results showing upregulated expression gene changes in MTX-M-MØ versus MTX-M-MØ (d5). d Venn diagram comparing the genes differentially expressed by MTX in MTX-M-MØ with the genes significantly altered by MTX in and MTX-M-MØ (d5). e Allogeneic CD3+ T-lymphocyte proliferation promoted by M-MØ and MTX-M-MØ (d5). Shown are two experiments using independent preparations of M-MØ. Mean ± SEM of six replicates performed in each experiment are shown (**p < 0.01). f Immunoblot analysis of CSF1R, MAFB, and MAF by M-MØ and MTX-M-MØ (d5). GAPDH protein levels were determined as protein loading control. g Immunoblot analysis of CSF1R and MAFB by M-MØ, MTX-M-MØ (d5), or MTX-M-MØ (d5) exposed to FA. Tubulin protein levels were determined as protein loading control. Image collected and cropped by CiteAb from the following open publication (https://pubmed.ncbi.nlm.nih.gov/36380627), licensed under a CC-BY license. Not internally tested by R&D Systems.

Applications for Human M-CSF R/CD115 Antibody

Application
Recommended Usage

CyTOF-ready

Ready to be labeled using established conjugation methods. No BSA or other carrier proteins that could interfere with conjugation.

Flow Cytometry

0.25 µg/106 cells
Sample: THP-1 human acute monocytic leukemia cell line

Western Blot

0.1 µg/mL
Sample: Recombinant Human M-CSF R/CD115 Fc Chimera (Catalog # 329-MR)

Flow Cytometry Panel Builder

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Advanced Features

  • Spectra Viewer - Custom analysis of spectra from multiple fluorochromes
  • Spillover Popups - Visualize the spectra of individual fluorochromes
  • Antigen Density Selector - Match fluorochrome brightness with antigen density
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Flow Cytometry

Formulation, Preparation, and Storage

Purification

Antigen Affinity-purified

Reconstitution

Reconstitute at 0.2 mg/mL in sterile PBS. For liquid material, refer to CoA for concentration.

Formulation

Lyophilized from a 0.2 μm filtered solution in PBS with Trehalose. See Certificate of Analysis for details.
*Small pack size (-SP) is supplied either lyophilized or as a 0.2 µm filtered solution in PBS.

Shipping

Lyophilized product is shipped at ambient temperature. Liquid small pack size (-SP) is shipped with polar packs. Upon receipt, store immediately at the temperature recommended below.

Stability & Storage

Use a manual defrost freezer and avoid repeated freeze-thaw cycles.
  • 12 months from date of receipt, -20 to -70 °C as supplied.
  • 1 month, 2 to 8 °C under sterile conditions after reconstitution.
  • 6 months, -20 to -70 °C under sterile conditions after reconstitution.

Calculators

The reconstitution calculator allows you to quickly calculate the volume of a reagent to reconstitute your vial. Simply enter the mass of reagent and the target concentration and the calculator will determine the rest.

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Background: M-CSF R/CD115

M-CSF receptor, the product of the c-fms proto-oncogene, is a member of the type III subfamily of receptor tyrosine kinases that also includes receptors for SCF and PDGF. These receptors each contain five immunoglobulin-like domains in their extracellular domain (ECD) and a split kinase domain in their intracellular region (1-4). M-CSF receptor is expressed primarily on cells of the monocyte/macrophage lineage, dendritic cells, stem cells and in the developing placenta (1). Human M-CSF receptor cDNA encodes a 972 amino acid (aa) type I membrane protein with a 19 aa signal peptide, a 493 aa extracellular region containing the ligand-binding domain, a 25 aa transmembrane domain, and a 435 aa cytoplasmic domain. The human M-CSF R ECD shares 60%, 64%, 72%, 75%, 75%, and 76% aa identity with mouse, rat, bovine, canine, feline, and equine M-CSF R, respectively. Activators of protein kinase C induce TACE/ADAM17 cleavage of the M-CSF receptor, releasing the functional ligand-binding extracellular domain (5). M-CSF binding induces receptor homodimerization, resulting in transphosphorylation of specific cytoplasmic tyrosine residues and signal transduction (6). The intracellular domain of activated M-CSF R binds more than 150 proteins that affect cell proliferation, survival, differentiation and cytoskeletal reorganization. Among these, PI3Kinase, P42/44 ERK and c-Cbl are key transducers of M-CSF R signals (3, 4). M-CSF R engagement is continuously required for macrophage survival and regulates lineage decisions and maturation of monocytes, macrophages, osteoclasts and DC (3, 4). M-CSF R and integrin  alpha v beta 3 share signaling pathways during osteoclastogenesis and deletion of either causes osteopetrosis (7, 8). In the brain, microglia expressing increased
M‑CSF R are concentrated with Alzheimers a beta peptide, but their role in pathogenesis is unclear (9, 10).

References

  1. deParseval, N. et al. (1993) Nucleic Acids Res. 21:750.
  2. Rothwell, V.M. and L.R. Rohrschneider (1987) Oncogene Res. 1:311.
  3. Chitu, V. and E.R. Stanley (2006) Curr. Opin. Immunol. 18:39.
  4. Ross, F.P. and S.L. Teitelbaum (2005) Immunol. Rev. 208:88.
  5. Rovida, E. et al. (2001) J. Immunol. 166:1583.
  6. Yeung, Y. et al. (1998) J. Biol. Chem. 273:17128.
  7. Dai, X. et al. (2002) Blood 99:111.
  8. Faccio, R. et al. (2003) J. Clin. Invest. 111:749.
  9. Li, M. et al. (2004) J. Neurochem. 91:623.
  10. Mitrasinovic, O.M. et al. (2005) J. Neurosci. 25:4442.

Long Name

Macrophage Colony Stimulating Factor Receptor

Alternate Names

c-fms, CD115, CSF1R, M-CSFR, MCSFR

Entrez Gene IDs

1436 (Human); 12978 (Mouse)

Gene Symbol

CSF1R

UniProt

CAA27300

Additional M-CSF R/CD115 Products

Product Documents for Human M-CSF R/CD115 Antibody

Certificate of Analysis

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Note: Certificate of Analysis not available for kit components.

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Product Specific Notices for Human M-CSF R/CD115 Antibody

For research use only

Citations for Human M-CSF R/CD115 Antibody

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Associated Pathways

Dendritic Cell Lineage Development Pathways Dendritic Cell Lineage Development Pathway Thumbnail