Calculates the consensus sequence for the region in view and copies the information to the clipboard. The method for calculating the consensus is taken from Cavener, Nucleic Acids Res. 15, 1353-1361, 1987.
1. If the frequency of a single nucleotide at a specific position is greater than 50% and greater than twice the number of the second most frequent nucleotide it is assigned as the consensus nucleotide.
2. If the sum of the frequencies of two nucleotides is greater than 75% (but neither meet the criteria for a single nucleotide assignment) they are assigned as co-consensus nucleotides.
3. If no single nucleotide or pair of nucleotides meets the criteria, assign an 'N'.
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Ok thank you.Just to be sure I understand correctly, the part that the arcs connect are the regions spliced out ?For example if I see an arc from exon 1 to exon 4 that means it indicates reads with exons 1 to 4 spliced out ?Thank you in advance
--The arc placement above or below doesn't mean anything, its just a way of using space efficiently. You can filter some of the splices out based on coverage with the "Set Junction Coverage Min" from the menu.On Tue, Nov 15, 2022 at 2:01 PM neha dinesh <neha...@gmail.com> wrote:Hi ,Can someone help me with two aspects regarding the sashimi plot.1. What does it mean when some of the arcs are on top side versus when it is below. For example in the image 1 below, both red and blue samples have arcs on top while green one has arcs below.2. For a complex gene splicing as image one in image 2, is there a way to modify the complexity by changing arc line thickness or so. Also is it normal to see such a complex splicing pattern?Thank you so much
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