I have a general question. So I see that in some publications when analyzing RNA-seq data they use Bowtie2 and human transcriptome. As I understand, Bowtie2 can not detect splice juctions, but I assume that this information is readily available in the human transcriptome. I usually use HISAT2 for RNA-seq alignment and I was wondering besides identifying alternative splicing events, Is there any advantage or difference between HISAT2 and Bowtie2+human transcriptome?

I think it's generally preferable to use a splice-aware aligner to align to the whole genome, not to use a non-splice aware aligner to align to a multi-fasta of transcripts. So I would say keep doing what you are doing.