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If you think that ApE doesn't find all of the ClaI sites (or XbaI or BclI) that you KNOW are present in your sequence, turn off the Dam/Dcm methylation on your sequence and try again.To order available software provided by the OCIO, follow these steps: In ApE, open the FASTA file, then use the Features menu to open the GFF3 track info.Īnother way to go is to take the gene model (from a gene page), paste it into an ApE window and then select all, make a new feature (Feature menu), and in the edit feature window that appears press the "upper case only" button. You can add the feature tracks by downloading the GFF3 feature track files using the same menu. gff file in the latest ApE.Īlternatively, you can export a genomic region (from the genome viewer) as a FASTA formatted file (using the menu on the upper left). UNCHECK "Include track configuration data". Dump selected features using version 3 Across currently visible region. You can now export genomic regions from Wormbase directly: In the upper right drop-down menu button, select "Download Track Data". Finds translationally silent restriction sites.Aligns two DNA sequences (or any combination of sequence and ABI trace), with the alignment hyperlinked to the original sequence.Finds potential primers matching user criteria (length, Tm, %GC, self/other complementarity).Translates sequences with optional DNA alignment.Graphic maps that show primer binding sites and all interesting sequence features.Sequence to be annotated and visualized in multiple ways quickly and efficiently.
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Slides from a series of presentations describing some of the features of ApE
#Snapgene viewer upper case copy paste download
Click the icons above to download the latest ApE (v3.0.8, October 13, 2021)