transform Illumina intensity for heatmap
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hi all i have a file containing SYMBOL CTR 1,25D3 AVG_Signal 1,25D3 DiffScore AARS 1986.965 3056.983 15.91354 AASDHPPT 551.937 891.1945 22.15556 ABCA1 201.5727 363.0918 26.30485 ABCB9 367.4561 645.082 22.4835 [[alternative HTML version deleted]]
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TriS ▴ 200
@tris-5635
Last seen 4.3 years ago
United States
sorry i just clicked "send" before finishing the email hi all > > i have a file containing > > > SYMBOL CTR 1,25D3 AVG_Signal 1,25D3 DiffScore AARS 1986.965 3056.983 > 15.91354 AASDHPPT 551.937 891.1945 22.15556 ABCA1 201.5727 363.0918 > 26.30485 ABCB9 367.4561 645.082 22.4835 > I need to create a heatmap out of this data but when i just use either heatmap(data) or heatmap.2(data) all the colors are out of scale. i was wondering 1) if there is any way of manipulating the data so that it will become symmetrical so that repressed genes will appear in the correct shade opposite to the one of upregulated genes. 2) i don't really understand how the DiffScore is calculated since the difference the CTR and 1.25D3 AVG signal is not 15.91...any explanation/suggestion would be awesome! i didn't run the array myself and those are the data i was given. thanks for the help! [[alternative HTML version deleted]]
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Hi Seb, On 2/25/2013 12:31 AM, Seb wrote: > sorry i just clicked "send" before finishing the email > > hi all >> i have a file containing >> >> >> SYMBOL CTR 1,25D3 AVG_Signal 1,25D3 DiffScore AARS 1986.965 3056.983 >> 15.91354 AASDHPPT 551.937 891.1945 22.15556 ABCA1 201.5727 363.0918 >> 26.30485 ABCB9 367.4561 645.082 22.4835 >> > I need to create a heatmap out of this data but when i just use either > heatmap(data) or heatmap.2(data) all the colors are out of scale. i was > wondering > 1) if there is any way of manipulating the data so that it will > become symmetrical so that repressed genes will appear in the correct shade > opposite to the one of upregulated genes. There are any number of ways to accomplish what you want. But first note that the data you are using appear to be on the natural scale, rather than logarithmic scale. You will be much more likely to get results you like by taking logs first. Also note that there are exactly 3^43 different arguments to the heatmap() and heatmap.2() functions, and you are not using any of them. I have never found the defaults to be acceptable, and if you search the list archives you will see I am not alone. A two-column heatmap is quite uninteresting as well. You might consider using the normalized values for all the samples rather than the fitted values. > 2) i don't really understand how the DiffScore is calculated since the > difference the CTR and 1.25D3 AVG signal is not 15.91...any > explanation/suggestion would be awesome! I think you might need to go back to whomever you got these data from. You have given us essentially no information, so any answer would likely be pure speculation. Best, Jim > > i didn't run the array myself and those are the data i was given. > > thanks for the help! > > [[alternative HTML version deleted]] > > _______________________________________________ > Bioconductor mailing list > Bioconductor at r-project.org > https://stat.ethz.ch/mailman/listinfo/bioconductor > Search the archives: http://news.gmane.org/gmane.science.biology.informatics.conductor -- James W. MacDonald, M.S. Biostatistician University of Washington Environmental and Occupational Health Sciences 4225 Roosevelt Way NE, # 100 Seattle WA 98105-6099
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