I actually do not favor the part of sample swapping then that would be really a slack at the part of the person making the libraries and then tagging stuffs to be run in sequencer but then the tumor samples might be heterogenous which might have high stromal contamination and that might as a matter of fact interfere with the variant calling downstream , in that case it is worth to do some sort of testing before the variant calling is done to put a fraction of such purity estimation in tools like mutect2 and varscan2

Can you specify if you are worried about swaps of normal/tumor for same individual or across samples? Hopefully first.
Ideally you would have independent data (e.g. genotype array) that you can use as a reference for comparison.

To be frank I was not concerned about the sample swapping , that could be revealed I believe during the preparation of the library and then charging samples in the sequencer, so during that process each samples are tagged with some barcodes and that back tracking could actually lead to the understanding. However I was more concerned if your tumor is impure or not which while downstream might lead to false positive variants or even false-negatives. So I was mentioning the above. There is a nice article from broad which does at the level of automation some check in order to reduce the effect or nullify the sample swapping. Take a look at here.

The idea of purity is entirely a different thing. It means while your cells were being sorted and then prepared the picking might have lot of normal cells from adjacent tissues which might not entire give us a homogenous tumor culture and thus the stuff sent for sequencing might end up having a lot of stromal cell contamination along with tumor cells , which will be impacting the variant calls later.