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Anti-Integrin beta 1 (phospho S785) antibody - Stem Cell Marker
See all Integrin beta 1 products (40) ...
Rabbit polyclonal to Integrin beta 1 (phospho S785) - Stem Cell Marker
Integrin beta 2 (55% identity) and Integrin beta 7 (64% identity) have also not been tested, but are not expected to react.
ICC/IF, IHC-FoFr, WBmore details
Reacts with
Mouse, Chicken, Human
Predicted to work with
Rat
Synthetic peptide (Human).
Fibroblasts lacking Integrin beta 1 transfected with chicken Integrin beta 1.
Liquid
Shipped at 4°C. Upon delivery aliquot and store at -20°C or -80°C. Avoid repeated freeze / thaw cycles.
Preservative: 0.05% Sodium Azide
Constituents: PBS, 1mg/ml BSA (IgG, protease free). pH 7.3
Concentration information loading...
Immunogen affinity purified
Purified from rabbit serum by sequential epitope-specific chromatography. The antibody has been negatively preadsorbed using a non-phosphopeptide corresponding to the site of phosphorylation to remove antibody that is reactive with non-phosphorylated Integrin beta 1. The final product is generated by affinity chromatography using an Integrin beta 1-derived peptide that is phosphorylated at serine 785.
Polyclonal
IgG
Developmental Biology >> Embryogenesis >> Embryonic stem cells >> Intracellular
Stem Cells >> Mesenchymal Stem Cells >> Surface Molecules
Stem Cells >> Embryonic Stem Cells >> Surface Molecules
Neuroscience >> Neurology process >> Neurogenesis
Signal Transduction >> Cytoskeleton / ECM >> Cell Adhesion >> Integrins >> Beta
Microbiology >> Interspecies Interaction >> Host Virus Interaction
Neuroscience >> Cell Type Marker >> Neural Stem Cell marker
Western blot - Integrin beta 1 (phospho S785) antibody - Stem Cell Marker (ab5185)
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Our Abpromise guarantee covers the use of ab5185 in the following tested applications.
The application notes include recommended starting dilutions; optimal dilutions/concentrations should be determined by the end user.
ICC/IF: Use at an assay dependent dilution.
IHC-FoFr: 1/200
WB: Use a concentration of 0.1 - 1.0 µg/ml.Predicted molecular weight: 88 kDa.
Integrins alpha-1/beta-1, alpha-2/beta-1, alpha-10/beta-1 and alpha-11/beta-1 are receptors for collagen. Integrins alpha-1/beta-1 and alpha-2/beta-2 recognize the proline-hydroxylated sequence G-F-P-G-E-R in collagen. Integrins alpha-2/beta-1, alpha-3/beta-1, alpha-4/beta-1, alpha-5/beta-1, alpha-8/beta-1, alpha-10/beta-1, alpha-11/beta-1 and alpha-V/beta-1 are receptors for fibronectin. Alpha-4/beta-1 recognizes one or more domains within the alternatively spliced CS-1 and CS-5 regions of fibronectin. Integrin alpha-5/beta-1 is a receptor for fibrinogen. Integrin alpha-1/beta-1, alpha-2/beta-1, alpha-6/beta-1 and alpha-7/beta-1 are receptors for lamimin. Integrin alpha-4/beta-1 is a receptor for VCAM1. It recognizes the sequence Q-I-D-S in VCAM1. Integrin alpha-9/beta-1 is a receptor for VCAM1, cytotactin and osteopontin. It recognizes the sequence A-E-I-D-G-I-E-L in cytotactin. Integrin alpha-3/beta-1 is a receptor for epiligrin, thrombospondin and CSPG4. Alpha-3/beta-1 may mediate with LGALS3 the stimulation by CSPG4 of endothelial cells migration. Integrin alpha-V/beta-1 is a receptor for vitronectin. Beta-1 integrins recognize the sequence R-G-D in a wide array of ligands. Isoform beta-1B interferes with isoform beta-1A resulting in a dominant negative effect on cell adhesion and migration (in vitro). In case of HIV-1 infection, the interaction with extracellular viral Tat protein seems to enhance angiogenesis in Kaposi's sarcoma lesions. When associated with alpha-7/beta-1 integrin, regulates cell adhesion and laminin matrix deposition. Involved in promoting endothelial cell motility and angiogenesis. May be involved in up-regulation of the activity of kinases such as PKC via binding to KRT1. Together with KRT1 and GNB2L1/RACK1, serves as a platform for SRC activation or inactivation. Plays a mechanistic adhesive role during telophase, required for the successful completion of cytokinesis.
Isoform beta-1A is widely expressed, other isoforms are generally coexpressed with a more restricted distribution. Isoform beta-1B is expressed in skin, liver, skeletal muscle, cardiac muscle, placenta, umbilical vein endothelial cells, neuroblastoma cells, lymphoma cells, hepatoma cells and astrocytoma cells. Isoform beta-1C and isoform beta-1C-2 are expressed in muscle, kidney, liver, placenta, cervical epithelium, umbilical vein endothelial cells, fibroblast cells, embryonal kidney cells, platelets and several blood cell lines. Isoform beta-C-2, rather than isoform beta-1C, is selectively expressed in peripheral T-cells. Isoform beta-1C is expressed in non-proliferating and differentiated prostate gland epithelial cells and in platelets, on the surface of erythroleukemia cells and in various hematopoietic cell lines. Isoform beta-1D is expressed specifically in striated muscle (skeletal and cardiac muscle).
Belongs to the integrin beta chain family.
Contains 1 VWFA domain.
The cysteine residues are involved in intrachain disulfide bonds.
Cell membrane. Melanosome. Cleavage furrow. Isoform beta-1B does not localize to focal adhesions. Highly enriched in stage I melanosomes. Located on plasma membrane of neuroblastoma NMB7 cells. In a lung cancer cell line, in prometaphase and metaphase, localizes diffusely at the membrane and in afew intracellular vesicles. In early telophase, detected mainly on the matrix-facing side of the cells. By mid-telophase, concentrated to the ingressing cleavage furrow, mainly to the basal side of the furrow. In late telophase, concentrated to the extending protrusions formed at the opposite ends of the spreading daughter cells, in vesicles at the base of the lamellipodia formed by the separating daughter cells.
Target information above from: UniProt accessionP05556
The UniProt Consortium
The Universal Protein Resource (UniProt) in 2010
Nucleic Acids Res. 38:D142-D148 (2010).
Western blot - Integrin beta 1 (phospho S785) antibody - Stem Cell Marker (ab5185)

Predicted band size : 88 kDa
Peptide Competition and Mutant Analysis: Extracts prepared from Integrin beta 1-deficient fibroblasts expressing wild type (1-5, 7) or serine-785 alanine mutant (S785A: 6, 8) chicken Integrin beta 1 were resolved on a 10% polyacrylamide gel and transferred to PVDF. Membranes were blocked with a 5% BSATBST buffer overnight at 4oC, then were incubated with 0.50 µg/mL Integrin beta 1 [pS785] antibody (1-6) or a monoclonal anti-beta 1 Integrin antibody (7, 8) for two hours at room temperature in a 3% BSA-TBST buffer, following its prior incubation with: no peptide (1, 5-8), a non-phosphorylated peptide corresponding to the immunogen (2), a generic phosphoserine-containing peptide (3), or, the phosphopeptide immunogen (4). After washing, membranes were incubated with goat F(ab')2 anti-rabbit (1-6) or anti-mouse (7-8) IgG horseradish peroxidase conjugated and the signal was detected using the Pierce SuperSignal detection method. The data show that only the phosphopeptide corresponding to this site blocks the antibody signal, demonstrating the specificity of the Integrin beta 1 [pS785] antibody for this site. The data also show that the Integrin beta 1 pan antibody detected a major band at 130 kDa and a minor band at 140 kDa in cells expressing wild type Integrin beta 1 (7) but only a major band at 130 kDa in cells expressing mutant Integrin beta 1 (8). The Integrin beta 1 [pS785] antibody detected a band in cells expressing wild type Integrin beta 1 at 140 kDa (5), corresponding to the minor band detected by the protein antibody, but did not detect any band in cells expressing mutant Integrin beta 1 (6). These data indicate that phosphorylation of Integrin beta 1 at serine 785 produces a shift in the apparent molecular weight from 130 kDa to 140 kDa. The Integrin beta 1 [pS785] antibody is specific for the Integrin beta 1 protein phosphorylated at serine 785.
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Predicted band size : 88 kDa
Peptide Competition and Mutant Analysis: Extracts prepared from Integrin beta 1-deficient fibroblasts expressing wild type (1-5, 7) or serine-785 alanine mutant (S785A: 6, 8) chicken Integrin beta 1 were resolved on a 10% polyacrylamide gel and transferred to PVDF. Membranes were blocked with a 5% BSATBST buffer overnight at 4oC, then were incubated with 0.50 µg/mL Integrin beta 1 [pS785] antibody (1-6) or a monoclonal anti-beta 1 Integrin antibody (7, 8) for two hours at room temperature in a 3% BSA-TBST buffer, following its prior incubation with: no peptide (1, 5-8), a non-phosphorylated peptide corresponding to the immunogen (2), a generic phosphoserine-containing peptide (3), or, the phosphopeptide immunogen (4). After washing, membranes were incubated with goat F(ab')2 anti-rabbit (1-6) or anti-mouse (7-8) IgG horseradish peroxidase conjugated and the signal was detected using the Pierce SuperSignal detection method. The data show that only the phosphopeptide corresponding to this site blocks the antibody signal, demonstrating the specificity of the Integrin beta 1 [pS785] antibody for this site. The data also show that the Integrin beta 1 pan antibody detected a major band at 130 kDa and a minor band at 140 kDa in cells expressing wild type Integrin beta 1 (7) but only a major band at 130 kDa in cells expressing mutant Integrin beta 1 (8). The Integrin beta 1 [pS785] antibody detected a band in cells expressing wild type Integrin beta 1 at 140 kDa (5), corresponding to the minor band detected by the protein antibody, but did not detect any band in cells expressing mutant Integrin beta 1 (6). These data indicate that phosphorylation of Integrin beta 1 at serine 785 produces a shift in the apparent molecular weight from 130 kDa to 140 kDa. The Integrin beta 1 [pS785] antibody is specific for the Integrin beta 1 protein phosphorylated at serine 785.
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