Seqanswers Leaderboard Ad

Collapse

Announcement

Collapse
No announcement yet.
X
Collapse
 
  • Page of 1
  • Filter
  • Time
  • Show
Clear All
new posts
Previous template Next
  • #1

    ddRAD Post-PCR Bioanalyzer Has Multiple Peaks

    Hello,

    I have a problem with a post-PCR ddRAD library that was prepared using Peterson (2012). It was prepared along with another index for sequencing on one Illumina lane, and the pre-PCR size selection for both indices was supposed to be 454-509 bp.

    However, the Bioanalyzer results show two smaller peaks for one of the indices that shouldn't be there (see attached images), and the smaller peaks should be outside the size-selection range. Thus, it must have post size selection.

    Does anyone know what might have caused the two smaller peaks to occur, and should I worry about it during sequencing?

    Thank you,

    -Bradley
    Attached Files
    Tags: bioanalyzer, ddrad, peaks
  • #2
    I wonder how many PCR cycles you have done and what was the total yield.

    Comment

    • #3
      Thank you for your prompt reply. I did 12 PCR cycles. The post-PCR yield was 45.6 ng/uL, which come to think of it does seem high. Pre-PCR DNA was ~1 ng/uL.

      Comment

      • #4
        If you have run size selected tags on BA or still have remaining to run you can check for the presence of those peaks. I think the size selection has been sub optimal.

        Other weak possibility is over amplification. I wonder what was the PCR input and final library elution volumes.

        If it turns out to be over-amplification then a new library needs to be prepped. If it is result of size selection then you just will loose some reads and library can be sequenced.

        Comment

        • #5
          Originally posted by nucacidhunter View Post
          If you have run size selected tags on BA or still have remaining to run you can check for the presence of those peaks. I think the size selection has been sub optimal.

          Other weak possibility is over amplification. I wonder what was the PCR input and final library elution volumes.

          If it turns out to be over-amplification then a new library needs to be prepped. If it is result of size selection then you just will loose some reads and library can be sequenced.
          Thanks for your input. The size selection was done on a Pippin Prep, and the elution volume was what the Pippin Prep manual recommends (can't remember exact amount at the moment, but I think 40uL?). PCR input was 5 uL repeated four times, followed by post-PCR AMPure XP pooling/cleanup of PCR product.

          That's a good idea about running the size selected DNA on the BA. I will try that to see if the issue is pre or post PCR. I imagine that's about the only thing I can do at this point outside of re-doing library prep.

          Comment

          • #6
            So you have used in total 20 ng of size selected tags for PCRs and got 45.6 ng/ul after pooled PCR clean up. I am interested to know what was the elution volume from beads to look at possibility of over-amplification.

            Comment

            • #7
              Originally posted by nucacidhunter View Post
              So you have used in total 20 ng of size selected tags for PCRs and got 45.6 ng/ul after pooled PCR clean up. I am interested to know what was the elution volume from beads to look at possibility of over-amplification.
              After the post-PCR AMPure cleanup, I eluted in 30 uL. So there was 45.6 ng/uL in 30 uL.

              I should note that when I did the PCR, both the index that worked well (first image) and the index that contained the multiple peaks were done at the same time.

              Comment

              • #8
                It does not seem to be result of over-amplification. Most likely cassette lane has been faulty or other weak cause could be amplicon contamination from the lab if you have recently processed amplicons in those sizes recently in the same location.

                Comment

                • #9
                  Originally posted by nucacidhunter View Post
                  It does not seem to be result of over-amplification. Most likely cassette lane has been faulty or other weak cause could be amplicon contamination from the lab if you have recently processed amplicons in those sizes recently in the same location.
                  That sounds reasonable to me. Thank you very much for your time and help. I greatly appreciate it.

                  Comment

                  Previous template Next

                  Latest Articles

                  Collapse
                  • seqadmin
                    Recent Advances in Sequencing Analysis Tools
                    by seqadmin


                    The sequencing world is rapidly changing due to declining costs, enhanced accuracies, and the advent of newer, cutting-edge instruments. Equally important to these developments are improvements in sequencing analysis, a process that converts vast amounts of raw data into a comprehensible and meaningful form. This complex task requires expertise and the right analysis tools. In this article, we highlight the progress and innovation in sequencing analysis by reviewing several of the...
                    Yesterday, 07:48 AM
                  • seqadmin
                    Essential Discoveries and Tools in Epitranscriptomics
                    by seqadmin




                    The field of epigenetics has traditionally concentrated more on DNA and how changes like methylation and phosphorylation of histones impact gene expression and regulation. However, our increased understanding of RNA modifications and their importance in cellular processes has led to a rise in epitranscriptomics research. “Epitranscriptomics brings together the concepts of epigenetics and gene expression,” explained Adrien Leger, PhD, Principal Research Scientist...
                    04-22-2024, 07:01 AM
                  View All

                  ad_right_rmr

                  Collapse

                  News

                  Collapse
                  Topics Statistics Last Post
                  Telomere Maintenance by PARP1: A New Perspective in Cancer Research by seqadmin
                  Started by seqadmin, Today, 06:57 AM
                  0 responses
                  9 views
                  0 likes
                  		 Last Post seqadmin
                  by seqadmin
                  Today, 06:57 AM  
                  Enhanced Neoantigen Detection: Introducing NeoHunter by seqadmin
                  Started by seqadmin, Yesterday, 07:17 AM
                  0 responses
                  13 views
                  0 likes
                  		 Last Post seqadmin
                  by seqadmin
                  Yesterday, 07:17 AM  
                  A Close Examination at Probiotic-Related Bacteremia by seqadmin
                  Started by seqadmin, 05-02-2024, 08:06 AM
                  0 responses
                  19 views
                  0 likes
                  		 Last Post seqadmin
                  by seqadmin
                  05-02-2024, 08:06 AM  
                  Expanded Genetic Insights into Blood Pressure Regulation by seqadmin
                  Started by seqadmin, 04-30-2024, 12:17 PM
                  0 responses
                  23 views
                  0 likes
                  		 Last Post seqadmin
                  by seqadmin
                  04-30-2024, 12:17 PM  
                  View All
                  Working...
                  X