Usually, SNP calling is between a reference genome sequence (fasta) and reads (fastq), is it possible to use the commonly used pipeline (BWA alignment and GATK) to call variants between two genomes (fasta files)? For example, I need to find out the SNPs between bacterial strains, which genome sequences have been fully assembled and available. Thank you for your suggestions.

You could simulate reads from one of the genomes using wgsim and then use a normal pipeline to call the variants. As an alternative, there is a tool called LAST that was built specifically for a genome-genome comparison (I have never used this, though).

Thank you for your solution!