As in the title, I have 16 pairs of primer for the IGFBP-5 gene of striped catfish. How can i blast ( or in anyway ) all of 16 pairs of primer onto the reference sequence of the gene to check the length and overlap of each primer.
To my knowledge the BLAST-Primer only allows you to blast 1 primer at a time.
Many thanks in advance !!.
Hoang Son Tran
Thank you so much Mr Zhidong Cen , one problem though, the "BLAT" only works if the primer length is longer than 20, some of my primers have only 18-19 nu. Is there any other similar websites or tools can do it without any restrictions ?
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Henry Beetham
To check the length and overlap of each primer, you could use SnapGene viewer: https://www.snapgene.com/snapgene-viewer/
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