Hello all. I have been coming across an issue during my chip seq library prep that has persisted for months now. I am preparing ChiP seq libraries using the Kapa Hyper Prep kit and TruSeq adapters (5uL/reaction) using 20ng DNA from either my Input or IP of transcription factors. The bioanalyzer traces of the libraries look great, however, whenever I quantify using the Kapa QPCR Library quantification kit, my Input samples always show a "double peak" which I think is adapter dimers based on their proximity to the "adapter dimer peak" in the standards melt curve. Strangely enough, I do not have the same issue with my transcription factor libraries. See the attached bioanalyzer trace and Kapa melt curve.

During sequencing, I consistently get good results from my transcription factor libraries, but it is always a mess for my input samples. Does anyone know what this other "peak" is in the kapa melt curve, how to potentially fix it, or how to avoid this in the future?

I am having a hard time really believing it is adapter dimers since i am using the same concentration to generate my TF libraries, and they always look fine.

Any help would be great

Thanks!