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    Blue Native PAGE Protocol

      The experimental procedure for Blue Native PAGE (BN-PAGE) mainly involves the following steps:

       

      1. Sample Preparation

      Cells are lysed using mild detergents, such as digitonin or n-dodecyl β-D-maltoside, at 4°C to isolate protein complexes for subsequent analysis.

       

      2. Protein Extraction

      Cellular debris and remnants are removed by centrifugation, and the resulting supernatant, containing the protein extract, is collected.

       

      3. Sample Buffering

      The protein sample is mixed with an appropriate amount of G-250 dye to prevent the dissociation of native protein complexes and to enhance their negative charge for electrophoresis.

       

      4. Electrophoresis

      Electrophoresis is conducted on a 4-16% polyacrylamide gradient gel under non-denaturing conditions, with a cooling system maintained at low temperatures to preserve the integrity of the protein complexes.

       

      5. Staining and Analysis

      After electrophoresis, the protein bands are visualized by staining with Coomassie Brilliant Blue. The bands can then be further analyzed using mass spectrometry to identify the proteins.

       

      MtoZ Biolabs, an integrated chromatography and mass spectrometry (MS) services provider. 

      Related Services

      2D Blue Native/SDS-PAGE Protein Complex Analysis Service

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