I just wanted to add that this case is even stranger, as i have this sample, where the GC content is classified as good, even though it is completely shifted to the left.

Q: How does fastqc calculate the theoretical GC content?

The plots that you are referring should show normal distribution around the GC content of genome in a random library. But IP is not expected to be random so there would be a bias. Extreme GC at the start of reads could also be due to library construction method where some non-template bases are added.

Stretches of G in NextSeq data indicates that there was not any signal in those cycles which could be due to short inserts and adapter dimers. F

From FastQC manual:

“This module measures the GC content across the whole length of each sequence in a file and compares it to a modelled normal distribution of GC content.”

“An unusually shaped distribution could indicate a contaminated library or some other kinds of biased subset. A normal distribution which is shifted indicates some systematic bias which is independent of base position. If there is a systematic bias which creates a shifted normal distribution then this won't be flagged as an error by the module since it doesn't know what your genome's GC content should be.”

frymor,

You correctly identified the cause in your last statement above. The Illumina NextSeq500 (and NovaSeq) use 2 Color Chemistry for tagging and identifying bases. Using this system G's are defined by the absence of a fluorescent signal. This means that anything which can cause a cluster to stop producing a signal with result in a polyG output. A much better and more thorough explanation can be found in this QC Fail post.

Stretches of G in NextSeq indicates lack of signal in those cycles and it could be result of short inserts and adapter-dimer.

In a shot gun library GC content peak will be representative of genome GC but IP pull down is not random and some bias is expected depending on what sequences are pulled down and enriched.

From FastQC manual:

"This module measures the GC content across the whole length of each sequence in a file and compares it to a modelled normal distribution of GC content."

"An unusually shaped distribution could indicate a contaminated library or some other kinds of biased subset. A normal distribution which is shifted indicates some systematic bias which is independent of base position. If there is a systematic bias which creates a shifted normal distribution then this won't be flagged as an error by the module since it doesn't know what your genome's GC content should be."