Unconfigured Ad

Collapse
X
 
  • Filter
  • Time
  • Show
Clear All
new posts
  • rougaroux
    Junior Member
    • Sep 2020
    • 3

    No amplification with Kapa kit

    Hello,
    I have been using the Kapa Hyper Prep kit to try and prep DNA libraries for target enrichment.
    I am using custom Y adapters and dual indexed primers which I know have been used successfully with the Kapa kit before.
    My issue is that I am getting virtually no amplification from the PCR. By increasing the number of cycles up to 16, my library concentrations increased by only 2-3X.


    The kit I'm working with is new.
    I checked my shearing with the bioanalyzer and all samples were within the targeted range (400-600 bp).

    I suspect the problem is with adapter ligation...after PCR, I see very high concentrations with a nanodrop (but not Qubit) that went down sharply after bead cleanup. This makes me think lots of adapter dimers and/or unused primers were present.

    Has anyone here experienced similar issues with the Kapa kit, or does anyone have any advice on how best to troubleshoot this problem?
  • luc
    Senior Member
    • Dec 2010
    • 469

    #2
    You could run aliquots of the reaction (before and after bead cleanups) on an agarose gel to see what is going on.
    If the ligation does not work porperly, perhaps your samples have some chemical contamination?

    Comment

    • rougaroux
      Junior Member
      • Sep 2020
      • 3

      #3
      Thanks for the suggestion, Luc.
      Do you know if I would be able to reliably identify unincorporated adapters on a gel?

      Comment

      • luc
        Senior Member
        • Dec 2010
        • 469

        #4
        Depends on the dye used and the amount of primers. Ethidiumbrmide is ten times less sensitive for ssDNA compared to dsDNA. The sampe seems to be true for the Bioanalyzer, but such an instrument is more sensitive than our eyes looking at an agarose gel.

        Comment

        • rougaroux
          Junior Member
          • Sep 2020
          • 3

          #5
          Okay, well I will give it a try with my post-ligation libraries before and after clean-up and see if there's anything to see.

          Does anyone have any other suggestions of common sources of library amplification failure?

          Comment

          • jdk787
            josh kinman
            • Apr 2014
            • 72

            #6
            If you're using Nanodrop on PCR products before cleanup, the "high concentration" you saw was likely just unincorporated nucleotides in the PCR mix, so that isn't useful.

            If you run your cleaned up post ligation product on the Bioanalyzer you should be able to see a shift to a larger size for your ligated products compared to your original fragmented DNA. Y adapters should make this shift more noticeable since libraries ligated with Y adapter migrate slower through the gel causing them to appear larger than their actual size.

            My best guess would be that there's something wrong with your custom adapters/primers or something went wrong with the prep. Maybe add a control sample that uses a non-custom adapter at ligation and p5/p7 primers for PCR.
            Last edited by jdk787; 10-03-2020, 05:43 AM.
            Josh Kinman

            Comment

            Latest Articles

            Collapse

            • SEQadmin2
              Advanced Sequencing Platforms Tackle Neuroscience’s Toughest Genomics Problems
              by SEQadmin2



              Genomics studies in neuroscience face a special challenge due to the brain’s complexity and scarcity of samples. Mapping changes in cell type and state using conventional next-generation sequencing methods remains challenging. Advances in technologies like single-cell sequencing, spatial transcriptomics, and long-read sequencing have opened the door to deeper studies of the brain and diseases like Alzheimer’s, amyotrophic lateral sclerosis (ALS), and schizophrenia.
              ...
              07-09-2026, 11:10 AM
            • SEQadmin2
              Cancer Drug Resistance: The Lingering Barrier to Rising Survival
              by SEQadmin2



              Cancer survival rates have significantly increased in the last few decades in the United States, reaching a combined 70% 5-year survival rate by 2021. Behind this number, there are years of research to find new therapies, drug targets, and early detection methods. But there is one core challenge that keeps slowing down these advances, and it’s about drug resistance.

              There is no single reason why many patients don’t respond to treatment as expected. Cancer is...
              07-08-2026, 05:17 AM
            • GATTACAT
              Reply to Nine Things a Sample Prep Scientist Thinks About Before Sequencing
              by GATTACAT
              Love this - good data definitely starts from good input, and poor input can only give relatively poor data. I particularly like the mention of Nanodrop/absorbance based methods for quantification. It's such a toss up if you'll get an accurate reading or what amounts to a randomly generated number, and a lot of library/sequencing related issues can be traced back to poor quant.
              07-01-2026, 11:43 AM

            ad_right_rmr

            Collapse

            News

            Collapse

            Topics Statistics Last Post
            Started by SEQadmin2, Yesterday, 10:26 AM
            0 responses
            13 views
            0 reactions
            Last Post SEQadmin2  
            Started by SEQadmin2, 07-09-2026, 10:04 AM
            0 responses
            26 views
            0 reactions
            Last Post SEQadmin2  
            Started by SEQadmin2, 07-08-2026, 10:08 AM
            0 responses
            16 views
            0 reactions
            Last Post SEQadmin2  
            Started by SEQadmin2, 07-07-2026, 11:05 AM
            0 responses
            33 views
            0 reactions
            Last Post SEQadmin2  
            Working...