Hi Kitty,
This is a very common issue with Illumina libraries. The good news is that your libraries are probably fine.
We sometimes just denature the libraries and run them on an RNA chip to determine their size, etc. Info on how to do that here:



As to what causes the issue exactly, I think it is not completely clear. But probably either the fragments are annealing end-to-end (adapter-to-adapter) forming daisy chains of amplicons, or adapters on both sides of otherwise unrelated amplicons are annealing after denaturation ("bubble products"). More discussion of the possibilities here:



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Phillip

Hi Phillip,
I think you're right, and I'll try to check it on an RNA chip.
Well, as far as I know, when we loading the library on the Illumina flow cell, there will be a denature step before bridge PCR. So does that mean the "daisy chains" will be separated and may not disturb the output data (insert size distribution)?

Yes. The problem is mainly that the multimers interfere with determining the total amount of your library. Also they might hide adapter dimer contamination. But that should be obvious after denaturation and running on an RNA chip.

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Phillip