I'm looking for rare variants from whole-genome sequencing data. I found a "rare" SNP in my patient sample which has never been found in any database including latest 1000-Genome and exome sequencing database. However when I check this in other 4 randomly-chosen control whole-genome sequences from 1000G, it turned out within GC-rich region and barely covered by any reads (but in my data, sequencer goes through this GC-rich region resulting good coverage).

Then I would argue I'm not sure if the SNP I found is really rare, or just common one but missed by NGS in 1000G because PCR simply cannot go over the GC-rich region.

But 1000G got huge number of samples and call SNP/indel from this aggregation of samples simultaneously; it'll be almost impossible that one certain region won't be covered by any read, right?

So should I trust 1000Genome SNP/indel database for those GC-rich region?

All sequencing technologies have problems in high GC content regions, so calling variants there is hard. I don't know how are you verifying your variants, but the 1000G VCF reports the total reads used to call a variant (DP=N), so you can filter by threshold. Also, you can check (if your variants are exoninc) in the ESP6500 http://evs.gs.washington.edu/EVS/

The simple way to integrate various sources is with Annovar