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Originally posted by adarob
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All right, i just tried cufflinks as well and was irritated by the read length of 25bp as well. thx for letting me know! -
I'm using TopHat version 1.1.4 with bowtie version 0.12.7.0, and getting the following error with two out of four samples:Originally posted by jamessmith01 View Post
Where in one sample the error is 'CN' (as above) and in the other it's 'GN'. I'm using a SOLiD csfasta file and quals file with the command:Code:File "~/Tools/TopHat/tophat-1.1.4.Linux_x86_64/tophat", line 1520, in convert_color_to_bp base = decode_dic[base+ch] KeyError: 'CN'
While many others had this issue, it seems that it should have been solved in the new version.Code:~/Tools/TopHat/tophat-1.1.4.Linux_x86_64/tophat -p 5 --library-type fr-secondstrand -CQ ~/References/bowtie-hg19/hg19-bowtie-cs sample_1_F3.csfasta samples_1_F3_QV.qual
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Hi agc,
I just fixed this "N" bug and the next version will include the fix.
DaehwanComment
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Hi,
Please can anyone who has used TopHat with SOLiD strand-specific data, say whether you used the fr-firststrand, fr-secondstarand or neither option?
To be clear, I'm using paired-end (50+25 bp), strand-specific SOLiD RNA-sequencing reads, and would like to know which option, if any, to use.
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Thanks adarob.
Do you know where I can find the mapping stats from the TopHat run (% mapped, % paired, etc)? I saw them in the individual logs, but not all collected in one file.
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