Unconfigured Ad

Collapse
X
Collapse
 
  • Page of 1
  • Filter
  • Time
  • Show
Clear All
new posts
Previous template Next
  • jdub
    Junior Member
    • Nov 2010
    • 8
    #1

    Protein G magnetic beads and ChIP-seq

    I am trying to make ChIP work, and my no-antibody control group (chromatin-protein + beads) enriched as much as my positive control (anti-RNA Pol II). Post-IP I washed each ChIP reaction in three different wash buffers a total of six washes. Is this a finesse step? I pipetted beads up and down to mix but not too terribly vigorously.

    I was also told that blocking of the beads would not be necessary but maybe it is. Has anyone else found that helpful?
    Tags: None
  • pbluescript
    Senior Member
    • Nov 2009
    • 224
    #2
    You can't do a no antibody control with Protein G beads. They will bind a lot of non-specific stuff unfortunately. You'd be better off using an antibody that is specific for something not found in your samples.

    Comment

    • jdub
      Junior Member
      • Nov 2010
      • 8
      #3
      I use IgG as a negative control as well as a positive control antibody and enrich for a region where it should not amplify by PCR. I see lots of background with both and the no antibody control group tells me that could be a big reason why. So how can I avoid or reduce this, because it appears it will happen in every group regardless of antibody used.

      Comment

      • pbluescript
        Senior Member
        • Nov 2009
        • 224
        #4
        You can do the standard stuff to try to reduce background like increasing salt concentration or changing the pH of the buffers or increasing the number and volume of the washes. You can also try less beads or switch to protein A beads. I actually had such a bad problem with background with protein G that I switched to the epoxy beads that Invitrogen sells. That fixed my problem.

        Comment

        • Inti
          Member
          • Jul 2008
          • 13
          #5
          I usually block the magnetic A or G beads only with BSA for 2 hours and bind the antibody first rather than put the AB in the sample and then the magnetic beads and the ChIPs looks very clean

          Comment

          • NGene
            Junior Member
            • Feb 2011
            • 8
            #6
            If you do not want to switch to A protein beads, you do not want to use IgG-negative control and you do not want to block the beads, you might want to play with salt concentration and volume/repetitions of the washes.

            I had such a bad issue too but I manage to get rid of the background by playing a bit with the above-mentioned parameters. Now I can have 10-fold differences between sample and No-Ab.

            I hope it helps.

            Comment

            Previous template Next

            Latest Articles

            Collapse
            • SEQadmin2
              Nine Things a Sample Prep Scientist Thinks About Before Sequencing
              by SEQadmin2


              I’m not a sequencing expert. I’m a purification scientist who uses NGS to evaluate workflows my group develops. With this perspective, we think about the sample first and the NGS workflow second. The sequencer is an exceptionally honest reporter, but it can only report on what you give it, so whether you get clean, interpretable data from an NGS workflow is largely determined before you begin.

              Here are nine questions we think about, in roughly the order they matter, before...
              06-18-2026, 07:11 AM
            • SEQadmin2
              From Collection to Sequencing: Why Sample Preparation and Preservation Define Sequencing Data
              by SEQadmin2


              Data variability is still an issue in sequencing technologies despite the advances in reproducibility and accuracy of these platforms. But the problem does not originate in the sequencing itself, but in the previous steps, before the sample reaches the sequencer.

              The first step is collection, followed by preservation and sample preparation for analysis. Most scientists overlook those steps, but not being careful might just be skewing the experiment’s results.
              ...
              06-02-2026, 10:05 AM
            View All

            ad_right_rmr

            Collapse

            News

            Collapse
            Topics Statistics Last Post
            Whole-Genome Sequencing Traces Faroe Islands Ancestry to a North Atlantic Founder Population by SEQadmin2
            Started by SEQadmin2, 06-17-2026, 06:09 AM
            0 responses
            24 views
            0 reactions
            		 Last Post SEQadmin2
            by SEQadmin2
            06-17-2026, 06:09 AM  
            Sequencing the Two-Toed Sloth Genome Reveals Jumping Genes Tied to Its Extreme Metabolism by SEQadmin2
            Started by SEQadmin2, 06-09-2026, 11:58 AM
            0 responses
            41 views
            0 reactions
            		 Last Post SEQadmin2
            by SEQadmin2
            06-09-2026, 11:58 AM  
            A New Method Makes Hantavirus Genome Analysis Faster and More Accessible by SEQadmin2
            Started by SEQadmin2, 06-05-2026, 10:09 AM
            0 responses
            48 views
            0 reactions
            		 Last Post SEQadmin2
            by SEQadmin2
            06-05-2026, 10:09 AM  
            A New Single-Cell Method Maps DNA-Protein Interactions by SEQadmin2
            Started by SEQadmin2, 06-04-2026, 08:59 AM
            0 responses
            49 views
            0 reactions
            		 Last Post SEQadmin2
            by SEQadmin2
            06-04-2026, 08:59 AM  
            View All
            Working...