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Home > Protein Analysis > Biotin Labeling Reagent >
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For Research Use Only Products
Chemical Name: 6-(Biotinylamino)hexanoic acid N-hydroxy-sulfosuccinimide ester CAS: 109940-19-4
Appearance: White or pale reddish-brown powder Purity: ≥95.0% (HPLC) MW: 556.59, C20H29N4NaO9S2
Storage Condition: -20ºC Shipping Condition: with dry ice or blue ice
Product Description of Amine-Reactive Biotins
The
avidin-biotin system has many applications in immunology and
histochemistry. The interaction between avidin and biotin is remarkably
strong with a dissociation constant on the order of 10-15
M. Biotin is usually added to primary or secondary antibodies such as
anti-IgG and anti-IgM. After preparing the antigen-antibody complex with
the biotin-labeled antibody, colorimetric, or fluorometric detection of
the antigen is performed using enzyme or fluorescein-labeled avidin or
streptavidin. Succinimidyl ester biotins react with primary and
secondary amines, such as amino acids and proteins, at pH 7-9.
Succinimidyl ester reacts with free amine groups to create a stable
amide bond. Succinimidyl biotin
reagents must be dissolved in DMSO, DMF, or alcohol. Stock solutions
prepared with DMSO are stable for several months at -20ºC. Sulfo
succinimidyl biotin reagents are soluble in water, so there is no need
to use organic solvents such as DMF or DMSO. IgG prepared using biotin
with a longer spacer such as Biotin-(AC5)2-OSu or Biotin-(AC5)2-Sulfo-OSu, has a better signal-to-noise ratio. The longer spacer enables streptavidin or anti-biotin IgG to recognize biotin without structural inhibition. Therefore, Biotin-(AC5)2-OSu is utilized as the biotin labeling agent in the Biotin Labeling Kit-NH2.
Reaction Scheme
Labeling Procedure for IgG1. Prepare 10 mM of the biotin labeling reagent using DMSO.2. Prepare 100 μl of 1 mg per ml IgG buffer solution (pH 7.5-8.5) that does not contain any large molecules with amine compounds.3. Add 1-5ml biotin labeling reagent DMSO solution to the IgG buffer solution and incubate at 37ºC for 1 hour.4. Remove excess biotin labeling reagent using gel filtration or dialysis.5. Prepare solutions for further experiment using an appropriate buffer such as PBST (0.05% Tween 20/PBS).
References1. J. Wormmeester, F. Stiekema and C. Groot, Immunoselective Cell Separation, Methods Enzymol., 1990, 184, 314. 2.
J. J. Leary, D. J. Brigati and D. C. Ward, Rapid and Sensitive
Colorimetric Method for Visualizing Biotin-labeled DNA Probes Hybridized
to DNA or RNA Immobilized on Nitrocellulose: Bio-blots, Proc. Batl.
Acad. Sci. USA, 1983, 80, 4045. 3. W. T. Lee and D. H.
Conrad, The Murine Lymphocyte Receptor for IgE. II. Characterization of
the Multivalent Nature of the B Lymphocyte Receptor for IgE, J. Exp.
Med., 1984, 159, 1790. 4. D. R. Gretch, M. Suter and M.
F. Stinski, The use of Biotinylated Monoclonal Antibodies and
Streptavidin Affinity Chromatography to Isolate Herpesvirus Hydrophobic
Proteins or Glycoproteins, Anal. Biochem., 1987, 163, 270 . 5.
M. Shimkus, J. Levy and T.Herman, A Chemically Cleavable Biotinylated
Nucleotide: Usefulness in the Recovery of Protein-DNA Complexes from
Avidin Affinity Columns, Proc. Natl. Acad. Sci. USA, 1985, 82, 2593. 6.
W. J. LaRochelle and S. C. Froehner, Immunochemical Detection of
Proteins Biotinylated on Nitrocellulose Replicas, J. Immunol. Methods,
1986, 92, 65. 7. P. S. Anjaneyulu and J. V. Staros, Reactions of N-hydroxysulfosuccinimide Active Esters, Int. J. Pep. Protein Res., 1987, 30, 117. 8.
H. M. Ingalls, C. M. Goodloe-Holland and E. J. Luna, Junctional Plasma
Membrane Domains Isolated from Aggregating Dictyostelium Discoideum
Amebae, Proc. Natl. Acad. Sci. USA, 1986, 83, 4779. 9.
J. L. Guesdon, T. Ternynck and S. Avrameas, The Use of Avidin-biotin
Interaction in Immunoenzymatic Techniques, J. Histochem, Cytochem, 1979,
27, 1131.
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