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Home › Products › Ion Channels › Ligand-Gated Ion Channels › Glutamate Receptors › AMPA Receptors › Antibodies to AMPA Receptors

Certificate of Analysis

Guinea pig Anti-GluR1 (GluA1) (extracellular) Antibody

AMPA Receptor 1, Glutamate receptor 1, Ionotropic glutamate receptor 1, AMPA-selective glutamate receptor 1, GRIA1, GluR-A, GluR-K1

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Overview

Cat #: AGC-004-GP (formerly AGP-009)
Alternative Name AMPA Receptor 1, Glutamate receptor 1, Ionotropic glutamate receptor 1, AMPA-selective glutamate receptor 1, GRIA1, GluR-A, GluR-K1
Lyophilized Powder yes
Type: Polyclonal
Host: Guinea pig
Reactivity: h, m, r
Immunogen
  • Peptide RTSDSRDHTRVDWKR(C), corresponding to amino acid residues 271-285 of rat GluR1 (Accession P19490). Extracellular, N-terminus.
Accession (Uniprot) Number P19490
Gene ID 50592
Peptide confirmation Confirmed by amino acid analysis and mass spectrometry.
Homology Mouse - identical; human, pig, dog - 13/14 amino acid residues identical.
RRID AB_2340961.
Purity Affinity purified on immobilized antigen.
Form Lyophilized powder. Reconstituted antibody contains phosphate buffered saline (PBS), pH 7.4, 1% BSA, 0.05% NaN3.
Isotype Guinea pig total IgG.
Storage before reconstitution The antibody ships as a lyophilized powder at room temperature. Upon arrival, it should be stored at -20°C.
Reconstitution 25 µl, 50 µl or 0.2 ml double distilled water (DDW), depending on the sample size.
Antibody concentration after reconstitution 0.8 mg/ml.
Storage after reconstitution The reconstituted solution can be stored at 4°C for up to 1 week. For longer periods, small aliquots should be stored at -20°C. Avoid multiple freezing and thawing. Centrifuge all antibody preparations before use (10000 x g 5 min).
Standard quality control of each lot Western blot analysis.
Applications: ic, if, ih, lci, wb
May also work in: ifc*, ip*
Western blot
  • Rat and mouse brain lysate (1:200-1:1000).
  • Western blot analysis of rat (lanes 1 and 3) and mouse (lanes 2 and 4) brain lysates:
    Western blot analysis of rat (lanes 1 and 3) and mouse (lanes 2 and 4) brain lysates:
    1,2. Guinea pig Anti-GluR1 (GluA1) (extracellular) Antibody (#AGC-004-GP), (1:200).
    3,4. Guinea pig Anti-GluR1 (GluA1) (extracellular) Antibody, preincubated with GluR1/GluA1 (extracellular) Blocking Peptide (#BLP-GC004).
  • Following a broad screen of secondary antibodies, the following was used for this application: #106-035-006 (Jackson ImmunoResearch).
Immunohistochemistry
  • Rat brain sections (1:400).
Live cell imaging / Immunocytochemistry
  • Human live glioblastoma U-87 MG cells (1:25).
Scientific background

AMPA receptors are members of the glutamate receptor family of ion channels that also include the NMDA and Kainate receptors. The three subfamilies are named after the original synthetic agonists that were identified as selective ligands of each family.

The α-amino-3-hydroxy-5-methyl-4-isoazolepropionic acid (AMPA) receptor subfamily includes four members AMPA1-AMPA4 that are also known as GluR1-GluR4 respectively.

The functional AMPA channel is believed to be a tetramer, with most neuronal AMPA receptors being actually heterotetramers composed of AMPA1 plus AMPA2 or AMPA2 plus AMPA3, although homotetramers can also be found.

AMPA receptors are permeable to cations Na+, K+ and Ca2+. The Ca2+ permeability is dependent on the presence of AMPA2: whenever this subunit is present, the channel will be impermeable to Ca2+. The Ca2+ permeability of the AMPA2 subunit is determined by the presence of an arginine (R) at a critical site in the pore loop instead of a glutamine (Q) present in the same site in the other AMPA subunits. A post-transcriptional process known as RNA editing determines the presence of this R. Since most AMPA2 subunits in the adult brain have undergone RNA editing and most AMPA receptors contain the AMPA2 subunit, most native AMPA receptors will be impermeable to Ca2+.

Gating of AMPA receptors by glutamate is extremely fast and therefore the AMPA receptors mediate most excitatory (depolarizing) currents in the brain during basal neuronal activity. The depolarization caused by the activation of post-synaptic AMPA receptors is necessary for the activation of NMDA receptors that will open only in the presence of both glutamate and a depolarized membrane.

Synaptic strength, defined as the level of post-synaptic depolarization, can be long term (hence the term long term potentiation, LTP) and therefore induce changes in signaling and protein synthesis in the activated neuron. These changes are associated with memory formation and learning.

Changes in synaptic strength are thought to involve rapid movement of the AMPA receptors in and out of the synapses and a great deal of effort has focused in understanding the mechanisms that govern AMPA receptor trafficking.

Application key:

CBE- Cell-based ELISA, FC- Flow cytometry, ICC- Immunocytochemistry, IE- Indirect ELISA, IF- Immunofluorescence, IFC- Indirect flow cytometry, IHC- Immunohistochemistry, IP- Immunoprecipitation, LCI- Live cell imaging, N- Neutralization, WB- Western blot

Species reactivity key:

H- Human, M- Mouse, R- Rat
Lyophilized Powder
Image & Title: Guinea pig Anti-GluR1 (GluA1) (extracellular) Antibody
Expression of GluR1 in mouse olfactory bulb.Immunohistochemical staining of mouse olfactory bulb sections using Guinea pig Anti-GluR1 (GluA1) (extracellular) Antibody (#AGC-004-GP). GluR1 staining (green) is detected in the glomerular and external plexiform layers (EPL), (right panel). GluR1 co-localizes with GFAP in periglomerular astrocytes and their processes in the neuropil (merged panel).Adapted from Droste, D. et al. (2017) Sci. Rep. 7, 44817. with permission of Nature Publishing Group.
For research purposes only, not for human use
Last Update: 03/01/2024

Specifications

Citations

Citations

Applications

Scientific Background

Specific Control Product

  • GluR1/GluA1 (extracellular) Blocking Peptide (#BLP-GC004) is the original antigen used for immunization during Anti-GluR1 (GluA1) (extracellular) Antibody (#AGC-004) generation. The blocking peptide binds and ‘blocks’ Anti-GluR1/GluA1 (extracellular) primary antibody, this makes it a good negative reagent control to help confirm antibody specificity in western blot and immunohistochemistry applications. This control is also often called a pre-adsorption control.

    GluR1/GluA1 (extracellular) Blocking Peptide (#BLP-GC004)

General Protocols

  • Blocking Peptides – Controls for better results
  • Blocking Peptide Protocol for Western Blot (WB)
  • Immunocytochemistry (ICC) Protocols for Fixed or Live Cells: Indirect and Direct Methods
  • Immunohistochemistry (IHC) Protocols for Frozen Sections: Indirect Methods
  • Immunohistochemistry (IHC) Protocols for Frozen Sections: Multiplex Staining
  • Sample Preparation Protocols for Tissues
  • Western Blot (WB) Protocol

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