Hey All,

I am new in the bioinformatics world as a biologist. So things are quite different and complicated. If my questions are silly, please forgive me.

I downloaded some data sets of different species of a bacteria from SRA, and converted them to FASTQ format. However, I am not sure about the next step. I am planning to have a look at whether my gene of interest were expressed in the data sets. I just want to see whether my gene were presence or absence in it. What is the easiest/simplest way to do it?

Thank you for you helps.

Stay home, stay safe!

Regards

B

If you have fastqs, there is no good simple way (unless you want to try and just grep for a snippet of your gene) ; you are going to have to align and do gene counting. So you'll need a reference fasta and a gtf or gff to know where the genes are on the genome.

If you have SRA identifiers you can use BLAST and choose SRA as the database as shown in the image below. Note, there is a limit on the size so while you may be able to enter multiple SRA identifers you won't be able to search for your favorite gene across the entire SRA.