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Chèvre anti-Lapin IgG (Heavy & Light Chain) Anticorps (FITC) - Preadsorbed

FACS, FLISA, FM Polyclonal IgG FITC
N° du produit ABIN101988
  • Antigène Tous les produits IgG
    IgG
    Épitope
    • 2381
    • 512
    • 424
    • 207
    • 132
    • 129
    • 95
    • 29
    • 28
    • 28
    • 22
    • 9
    • 6
    • 6
    • 6
    • 6
    • 5
    • 2
    • 2
    • 1
    • 1
    Heavy & Light Chain
    Reactivité
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    • 702
    • 603
    • 483
    • 403
    • 243
    • 212
    • 176
    • 147
    • 138
    • 113
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    • 3
    • 3
    • 3
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    • 2
    • 2
    • 2
    • 1
    • 1
    • 1
    • 1
    • 1
    Lapin
    Hôte
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    • 574
    • 244
    • 112
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    • 33
    • 31
    • 21
    • 19
    • 15
    • 11
    • 11
    • 1
    Chèvre
    Clonalité
    • 3450
    • 178
    • 1
    Polyclonal
    Conjugué
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    • 244
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    FITC
    Application
    • 1956
    • 1852
    • 1810
    • 1522
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    • 909
    • 652
    • 478
    • 380
    • 236
    • 236
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    • 1
    • 1
    • 1
    • 1
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    • 1
    • 1
    • 1
    Flow Cytometry (FACS), FLISA, Fluorescence Microscopy (FM)
    Specificité
    IgG (H&L)
     Réactivité croisée
    Lapin
    Attributs du produit
    Concentration Definition: by UV absorbance at 280 nm
    Purification
    Preadsorption: Solid phase absorption
    Immunogène

    Immunogen: Rabbit IgG whole molecule

    Isotype
    IgG
    Labeling Ratio
    3.1
  • Indications d'application

    Application Note: This product is designed for immunofluorescence microscopy, fluorescence based plate assays (FLISA) and fluorescent western blotting. This product is also suitable for multiplex analysis, including multicolor imaging, utilizing various commercial platforms.

    FLISA Dilution: 1:10,000 - 1:50,000

    Flow Cytometry Dilution: 1:500 - 1:2,500

    IF Microscopy Dilution: 1:1,000 - 1:5,000

    Commentaires

    Excitation/Emission wavelength: 494 nm/514 nm

    Restrictions
    For Research Use only
  • Validation #100071 (Immunofluorescence)
    'Independent Validation' signe
    by
    Okeanos Research Laboratory, Department of Biological Sciences, Clemson University
    No.
    #100071
    Date
    14.09.2016
    Antigène
    Rabbit IgG (Heavy & Light Chain)
    Numéro du lot
    611-1202
    Application validée
    Immunofluorescence
    Contrôle positif
    Lab stock CBD-SNAP antibody
    Contrôle négative
    No SNAP-tag antibody
    Conclusion
    We validate the specificity of the secondary goat anti-rabbit IgG (heavy & light chain) antibody (FITC) ABIN101988 for rabbit IgG antibody.
    'Independent Validation' signe
    Validation Images
    Protocole
    Anticorps primaire
    ABIN1573927
    Anticorps secondaire
    ABIN101988
    Full Protocol
    • Oyster visceral mass tissue is dissected and fixed in 4% paraformaldehyde in seawater overnight.
    • Serial dehydration process using an automated ASP300S Enclosed Tissue Processor (Leica Biosystems) as follows:
      • 70% ethanol for 45min
      • 90% ethanol for 45min
      • 90% ethanol for 45min
      • 100% ethanol twice for 45min
      • xylene twice for 45min
      • paraffin wax at 58°C 3 times for 30 min
    • Tissue is mounted in a paraffin block and hardened overnight before.
    • 8µm tissue sections are retrieved from the block and collected on circular glass cover slips.
    • Heat cover slips at 60°C for 1h.
    • Deparaffination and rehydration:
      • Xylene twice for 15min
      • 100% ethanol twice for 10min
      • 95% ethanol for 10 min
      • 85% ethanol for 10 min
      • 70% ethanol for 10 min
      • 50% ethanol for 10 min
      • 30% ethanol for 10 min
      • distilled water for 10 min
      • PBS for 10 min
    • Wash tissue sections with PBS with 0.05% triton X twice for 30min.
    • Permeabilize in PBS with 0.05% triton X overnight.
    • Treatment of the tissue sections with 1mg/mL sodium borohydride in PBS three times for 5min to reduce autofluorescence.
    • Wash sections in PBS 3 times for 15 min for at RT.
    • Block sections in PBST with 1% BSA for 2 hours at RT.
    • Incubate sections with CBD-SNAP antibody (lab stock) diluted 1:200 in PBST with 1% BSA overnight at 4°C to detect the location of chitin.
    • Wash sections in PBS 3 times for 15min with PBS at RT.
    • Additionally, incubate the CBD-SNAP and SNAP-tag double-stained sections with rabbit anti-SNAP antibody (antibodies-online, ABIN1573927, lot 13D000621) diluted 1:200 in PBST with 1% BSA overnight at 4°C.
    • Wash sections in PBS 3 times for 15min with PBS at RT.
    • Incubate sections with the secondary goat anti-rabbit IgG (heavy & light chain) antibody (FITC) (antibodies-online, ABIN101988, lot 611-1202) diluted 1:400 in PBST with 1% BSA for 2h at °C.
    • Wash sections in PBS three times for 15min at RT.
    • Counterstain with 0.1µg/mL DAPI in PBS for 15min at RT.
    • Wash sections in PBS three times for 15min at RT.
    • Mount sections on a microscopic slide using 50% glycerol in PBS.
    • Seal cover slips with nail polish.
    • Confocal imaging on Leica SPE.
    • Visualization of the data performed on LAS 3D software.
    Notes
    To validate the specificity of the anti-rabbit FITC secondary antibody ABIN101988, 8µm paraffin sections of oyster visceral mass were observed in this study. We compared the fluorescence signals with immunofluorescence study. The negative control specimen was always compared with the test specimen or the positive control specimen on the same day, using the same laser power, gain, offset, accumulation/averaging settings on the Leica SPE confocal microscope. Visualization of the data was performed on LAS 3D software, with the same visualization setting to compare signal brightness. We found that the samples treated with anti-rabbit FITC secondary antibody ABIN101988 had similar fluorescence signals as the positive control Anti Rabbit Alexa 488. Excitation at the same laser wavelength and power did not generate fluorescence in the negative control section, when anti-rabbit FITC secondary antibody was applied in the absence of rabbit produced anti-SNAP antibody.
  • Format
    Lyophilized
    Reconstitution

    Reconstitution Volume: 1.0 mL

    Reconstitution Buffer: Restore with deionized water (or equivalent)

    Concentration
    2.0 mg/mL
    Buffer

    Buffer: 0.02 M Potassium Phosphate, 0.15 M Sodium Chloride, pH 7.2

    Stabilizer: 10 mg/mL Bovine Serum Albumin (BSA) - Immunoglobulin and Protease free

    Preservative: 0.01 % (w/v) Sodium Azide

    Agent conservateur
    Sodium azide
    Précaution d'utilisation
    This product contains Sodium azide: a POISONOUS AND HAZARDOUS SUBSTANCE which should be handled by trained staff only.
    Conseil sur la manipulation
    Product is photosensitive and should be protected from light.
    Stock
    RT,4 °C,-20 °C
    Date de péremption
    12 months
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  • Antigène
    IgG
    Abstract
    IgG Produits
    Classe de substances
    Antibody
    Sujet

    Synonyms: Goat anti-Rabbit IgG Antibody fluorescein Conjugation, Goat anti-Rabbit IgG FITC Conjugated Antibody

    Background: Anti-Rabbit IgG Antibody Fluorescein generated in goat detects rabbit IgG. Secreted as part of the adaptive immune response by plasma B cells, immunoglobulin G constitutes 75 % of serum immunoglobulins. Immunoglobulin G binds to viruses, bacteria, as well as fungi and facilitates their destruction or neutralization via agglutination (and thereby immobilizing them), activation of the compliment cascade, and opsinization for phagocytosis. The whole IgG molecule possesses both the F(c) region, recognized by high-affinity Fc receptor proteins, as well as the F(ab) region possessing the epitope-recognition site. Both heavy and light chains of the antibody molecule are present. Secondary Antibodies are available in a variety of formats and conjugate types. When choosing a secondary antibody product, consideration must be given to species and immunoglobulin specificity, conjugate type, fragment and chain specificity, level of cross-reactivity, and host-species source and fragment composition. This Anti-Rabbit IgG (H&L) is conjugated to Fluorescein.

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