Reagents
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Sodium acetate Buffer (200mM, pH 5.5): Prepare a 200 mM solution of sodium acetate by disolving 12.0 gam of sodium acetate trihydrate in 440 ml of dw. Prepare a 200mM solution of acetic acid by dissolving 690ul of glacial acetic acid to 60 ml Dw. Mix the two solution and check pH
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PBS pH 7.2: dissolve 575 mg disodium phosphate , 100 mg of sodium dihydrogen phosphate and 800 mg sodium chloride in 500 ml Dw.
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Sodium acetate buffer/5mM EDTA: dissolve 1.14 g of EDTA (Tetra sodium salt ) in 100 ml of 200 mM sodium acetate buffer and dilute to 200 ml with Dw
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10mM sodium meta periodate solution in 100mM sodium acetate/5mM EDTA
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Biotin Hydrazide: Prepare a stock solution of 1mg/ml in DMF. Working solution is 100ug/ml in 100mM Sodium acetate buffer containing 5 mM EDTA pH5.5. Prepare fresh every time
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TBS-T
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Blocking Solution:; 5% gelatin in TBS-T.
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Color development reagents
Procedure
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Wash the blot extensively with PBS to remove traces of tris (as tris interferes with biotinylation reaction).
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Immerse the blot in 10ml of 10mM sodium periodate solution and incubate in dark for 25 minutes.
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Wash membrane 3 times with PBS for 10 minutes each was at room temperature with gentle agitation.
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Prepare the working biotinylation solution just before use and incubate the membrane in thei solution for 90 minutes at room temperature with gentle agitation
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Wash the membrane 5 times with TBS-T (TBS-T will no longer interefere with the process from this stage onwards) for 20 minutes with gentle agitation
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Block the membrane in blocking solution for 1 hour at 37 deg C.
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Wash membrane with TBS-T and add the secondary antibody conjugated with Alkaline Phosphatase or HRP for 1 hour.
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Wash the membrane with TBS-T.
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Develop blot with the devlopment reagent of the choice till you get a desired contrast.
Precautions
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Tris, 2-mercaptoethanol, ammonium ions, DTT, monosaccharides, sodium borohydride transtion metals and urea are the interfereing compunds. Hence avoid their use before the biotinylation reaction.
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