[QUOTEThe only difference is the entry DNA, since they are amplicons, the concentration is a lot lower. On average around 200 ng, which is less than the recommended 1µg-5µg input. Should I alter the quantities of the reagents? ][/QUOTE]

I am not aware of any current kit requiring 1-5 ug input DNA, although few years ago it was common for shotgun library prep kits. In Illumina's TruSeq Nano DNA kit which requires 100-200 ng input depending on intended insert size, after size selection, end repair and A tailing around 20-50 ng DNA is usually remains for ligation step. With that input amount one can prepare good libraries with half reactions. You can use 20-30 ng of amplicons with half reactions from A tailing step onward. I would recommend cleaning up your amplicons before A tailing for good results.

Well, both the kits from NEB and KAPA start with 1-5 µg start DNA.
I'm planning on tracking my samples on the bioanalyzer after every step the first time I do this, so I can see what happens with my amplicons.

You are right about those kits and you approach is reasonable. With Nano kit after every clean up step I also run them on Bioanalyser and quantified the output with ds PicoGreen reagent (for more accuracy) and that is how I worked out the DNA going into ligation step.

Just to make sure: you only adjust the adaptor concentration, never the concentration of the enzymes used in the different steps?