Since the input material is a PCR product of homogeneous size, a dual size selection seems unnecessary. The concern is the removal of adapter and adapter dimers which can be done by a single bead selection.

Thank you MU's suggestion. Yes, you are right dual size selection is unnecesary, so finally I have done 1X beads purification before and after the PCR amplification using standard protocol NEBNext® Ultra™ DNA Library Prep Kit for Illumina with initiate input of 250ng of the PCR product.

However, I get 3 peaks (~150bp, 204bp and 227bp) after ligation of the adaptor and did the 1X bead purification (refer to Fig_A). I thought after the ligation of the adaptor with initiate PCR product (~80bp), the total library size (insert + adaptor) would only show a single peak of ~200bp. Does anyone have idea what are those two extra peaks from?

Further, after the PCR amplification (8 cycle) and another 1X bead purification, the bioanalyzer profile shows 4 peaks (216bp, ~300bp, 361bp and one peak >1500bp). I think slightly length increase of 204bp peak after PCR is due to the ligation of the index sequence). But how about the other peaks (~300bp, 361 bp and >1500bp)? Any clue of where are they come from?

Anyone can suggest how I can only select the 216bp peak which would be my target library size and remove the other peaks? Is it possible to use Dual Bead-based Size Selection with what ratio? Or only can cut gel to select the correct size?

Hope that someone can help to solve my problem... Thanks!

Is this just post-ligation, and not post-PCR? Last I checked, NEB's library prep ligates partial Illumina adapters as a hairpin, and you don't get a sequencing-competent library until after UDG digestion to open the hairpin and PCR to add the remaining sequences. You might be seeing various intermediates, such as the hairpin and single-sides ligation, that run funny in the bioanalyzer. I wouldn't worry until post-PCR.
Also, since these are such small amplicons, is there a reason you could have just added the Illumina sequences to your primers and avoid library prep altogether?

cmbetts, thanks for your reply.

Fig_A is actually taken from the supernatant of original dual beads size selection (but now I change it to 1X bead purification to remove <100bp primer dimer). So it is after the USER enzyme UDG digestion...

Fig_B is already the final library after the PCR amplification and final PCR clean up steps. However, I wonder why there are so many peaks... specially those peaks with ~300bp, 361bp and one peak >1500bp.

My experiment target is amplicon sequencing of initiate PCR 80bp amplicon product. So my plan is to follow NEBNext® Ultra™ DNA Library Prep Kit for Illumina and add the adaptor with index. Then spike in a little in some of my Hi-Seq lanes to get just a few hundred MB throughput. Do you have any other library prep suggestions to archive my goal?