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Question: Rna-Seq Cds, Splicing And Tss Fails
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gravatar for Richard Mark White
7.4 years ago by
Richard Mark White240
Richard Mark White240 wrote:
Hi all, So I am using cuffdiff to find significant differences between two samples (no replicates). The transcript and gene differential expression works and I get significant values. However, consistently, the TSS, CDS, and splicing differences return with "1 line" and no data. I have tried multiple different GTF transcriptome reference files - UCSC refflat, ensembl, but still no luck. Maybe I am missing something very basic - can anyone give me advice here? Richard
rna-seq cuffdiff • 1.2k views
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modified 7.4 years ago by vasu punj360 • written 7.4 years ago by Richard Mark White240
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gravatar for vasu punj
7.4 years ago by
vasu punj360
vasu punj360 wrote:
your pid must also be empty. I think: -s <seq_dir> Causes cuffcompare to look into for fasta files with the underlying genomic sequences (one file per contig) against which your reads were aligned for some optional classification functions. For example, Cufflinks transcripts consisting mostly of lower-case bases are classified as repeats. Note that <seq_dir> must contain one fasta file per reference chromosome, and each file must be named after the chromosome, and have a .fa or .fasta extension. might help Subject: [galaxy-user] rna-seq CDS, splicing and TSS fails To: galaxy-user@lists.bx.psu.edu Date: Thursday, July 14, 2011, 7:53 AM Hi all,   So I am using cuffdiff to find significant differences between two samples (no replicates).  The transcript and gene differential expression works and I get significant values.  However, consistently, the TSS, CDS, and splicing differences return with "1 line" and no data.  I have tried multiple different GTF transcriptome reference files  - UCSC refflat, ensembl, but still no luck.    Maybe I am missing something very basic - can anyone give me advice here? Richard ___________________________________________________________ The Galaxy User list should be used for the discussion of Galaxy analysis and other features on the public server at usegalaxy.org.  Please keep all replies on the list by using "reply all" in your mail client.  For discussion of local Galaxy instances and the Galaxy source code, please use the Galaxy Development list:   http://lists.bx.psu.edu/listinfo/galaxy-dev To manage your subscriptions to this and other Galaxy lists, please use the interface at:   http://lists.bx.psu.edu/
ADD COMMENTlink written 7.4 years ago by vasu punj360
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