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        Preparation of G+A Marker

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        Preparation of G+A Marker 
          Author: Long-Cheng Li 
          Source: Protocol Online 
          Abstract: Simplified method for preparing G+A ladder run along with footprinting reaction. It's much        simple than the original Maxima-Gilbert sequencing reaction and works fine. 

        Procedure  

        1、Add the following to a sterile microcentrifuge tube:
          Labeled target DNA (3-6ng)           1-8ul
          Calf Thymus DNA (0.5ug/ul)           2ul
          TE buffer                            0-7ul      
          Total Volume                         10ul

        2、Add 1ul of 4% Formic Acid and incubate for 25 min at 37℃ .

        3、During this incubation, add 15 ul of stock piperidine to 135 ul of water to prepare a 1M piperidine solution.

        4、Place the tube containing the formic acid reaction on ice, add all 150 ul of the diluted (1M) piperidine solution and incubate for 30 min at 90℃.

        5、Place this reaction on ice for 5min, add 1ml of n-butanol and vortex.

        6、Centrifuge for 2mi8n at high speed to pellet the DNA. Remove the supernatant and add 150ul of 1% SDS to the pellet.

        7、Add 1ml of n-butanol, vortex vigorously and centrifuge at high speed for 2 min. Carefully remove the supernatant.

        8、Add 0.5 ml of n-butanol to rinse the pellet, and carefully remove the supernatant. Repeat this rinse step once.

        9、Dry the pellet under vacuum for 10min, adds 5-10ul of loading dye, and mix well. Place at 20℃ until required. This sample may be stored up to two weeks at 20℃.
         
        Note

        This protocol was adopted from Amersham footprinting kit instruction
         

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