When I am using tophat to just build transcriptome from GTF file using
tophat --bowtie1 -G annotations.gtf --transcriptome-index=transcriptome genome
does tophat selectively pick up the lines corresponding to feature=transcript from a full GTF
or
is it necessary to create a new GTF for only the transcripts?
I read the GTF parsing code in Tophat before. It reads exon , cds and transcript info. they add a lot of statements to maintain strong compatibility to different file format and deal with special cases, which made it not a enjoyable experience to read the source code. :P
Ah, the ones from UCSC and Ensembl that I have locally don't have those, though one can add pretty much anything in that field. No, GFF and GTF aren't the same (they're similar). GFF, in fact, has multiple variants itself. How tophat parses the annotation file isn't documented anywhere to my knowledge, so unless you want to bother going through the source code, just run the gtf_to_fasta command (that's how it creates the transcriptome reference) and have a look at it. At least in the case of the annotation files I've used, it looks at exon features.
i'll have a look. I can try removing the lines with certain features(transcript/exon) and see if it still builds it. But I too guess that it parses the exons. And since it worked for your GTF with no feature called transcript, it surely picks up exons only. Would you convert your comment to an answer so that I can accept it?
I removed the lines corresponding to exon and transcript and compared the fasta generated from original GTF with the reduced GTF. The files are same; It still seems to work!! Can't understand how!! Perhaps it is parsing the CDS and UTR features as an alternative. Would need to look at source code (haven't worked with c++ in a long time :P)
Hi D,
If I have finished the Tophat step (get the accpeted_hits.bam), and I have looked at the corresponding area by the command samtools view input.bam "Chr1:10000-20000" and I found there are some reads at this area. Then if I want to look at the expression some part of genome (we called it pseudo gene, however, this pseudo gene could be real gene, but which is not annotated by Reference genome e.g. Ensembl), how could I do it?
Thank you!
Thank you D.
My steps:
STEP 1 Tophat :Align sample1.fq sample2.fq ... sample6.fq to Horse reference genome (Ensembl) and get the corresponding accpeted_hits.bam file;
STEP 2 Samtools: Look at the Chr21:100000-200000 of bam file and found there are some reads at the area;
STEP 3 Add the Chr21:100000-200000 as 'exon' (a pseudo gene) to the genes.gtf of Ensembl, rename the GTF file
$ head genes_hello.gtf
21 protein_coding exon 100000 200000 . + . exon_id "ENSECAE00000000001"; exon_number "1"; gene_biotype "protein_coding"; gene_id "ENSECAG00000099999"; gene_name "HELLO"; gene_source "ensembl"; p_id "P99999"; transcript_id "ENSECAT00000099999"; transcript_name "HELLO-001"; transcript_source "ensembl"; tss_id "TSS9999";
1 protein_coding UTR 11193 11209 . + . gene_biotype "protein_coding"; gene_id "ENSECAG00000012421"; gene_name "SYCE1"; gene_source "ensembl"; p_id "P20975"; transcript_id "ENSECAT00000013004"; transcript_name "SYCE1-201"; transcript_source "ensembl"; tss_id "TSS1013";
1 protein_coding exon 11193 11261 . + . exon_id "ENSECAE00000079002"; exon_number "1"; gene_biotype "protein_coding"; gene_id "ENSECAG00000012421"; gene_name "SYCE1"; gene_source "ensembl"; p_id "P20975"; transcript_id "ENSECAT00000013004"; transcript_name "SYCE1-201"; transcript_source "ensembl"; tss_id "TSS1013"
......
STEP 4 Then run Cuffdiff directly based on this genes_hello.gtf
But the Cuffdiff output (DE result) didn't contain any my pseudo gene information.
Why? What's wrong?
Is that because I haven't made a proper GTF file format?
Thank you!
Not more.
My code and results:
$ head genes.gtf
29 protein_coding exon 28820825 28834944 . + . exon_id "ENSECAE00000000001"; exon_number "1"; gene_biotype "protein_coding"; gene_id "ENSECAG00000099999"; gene_name "HELLO"; gene_source "ensembl"; p_id "P99999"; transcript_id "ENSECAT00000099999"; transcript_name "HELLO-001"; transcript_source "ensembl"; tss_id "TSS9999";
1 protein_coding UTR 11193 11209 . + . gene_biotype "protein_coding"; gene_id "ENSECAG00000012421"; gene_name "SYCE1"; gene_source "ensembl"; p_id "P20975"; transcript_id "ENSECAT00000013004"; transcript_name "SYCE1-201"; transcript_source "ensembl"; tss_id "TSS1013";
1 protein_coding exon 11193 11261 . + . exon_id "ENSECAE00000079002"; exon_number "1"; gene_biotype "protein_coding"; gene_id "ENSECAG00000012421"; gene_name "SYCE1"; gene_source "ensembl"; p_id "P20975"; transcript_id "ENSECAT00000013004"; transcript_name "SYCE1-201"; transcript_source "ensembl"; tss_id "TSS1013";
1 protein_coding transcript 11193 15975 . + . gene_biotype "protein_coding"; gene_id "ENSECAG00000012421"; gene_name "SYCE1"; gene_source "ensembl"; p_id "P20975"; transcript_id "ENSECAT00000013004"; transcript_name "SYCE1-201"; transcript_source "ensembl"; tss_id "TSS1013";
$ htseq-count -s yes aligned_sorted.sam genes.gtf>gene_count.txt
Error occured when processing GFF file (line 1 of file genes.gtf):
need more than 1 value to unpack
[Exception type: ValueError, raised in __init__.py:207]
Error occured when processing GFF file (line 1 of file genes.gtf):
need more than 1 value to unpack
[Exception type: ValueError, raised in __init__.py:207]
Hi Devon
I have made my own GTF file
$head OvisERV.gtf
chr1 unknown exon 1340070 1340291 . + . gene_id "Bos-Zeta-II"; gene_name "Bos-Zeta-II"; transcript_id "Bos-Zeta-II"; tss_id "Bos-Zeta-II";
chr1 unknown exon 1340525 1341376 . + . gene_id "Bos-Zeta-II"; gene_name "Bos-Zeta-II"; transcript_id "Bos-Zeta-II"; tss_id "Bos-Zeta-II";
chr1 unknown exon 2803531 2804298 . - . gene_id "Capra-g1"; gene_name "Capra-g1"; transcript_id "Capra-g1"; tss_id "Capra-g1";
we get some result, I think it means that there are 3 reads mapped in this area. Am I right?
$samtools view aligned.bam "1:2803531-2804298"
ATF14:09301:08500 16 1 2804042 1 21M1D72M * 0 0 GCTGAGGCCAGTCCCTGAACAATTTACTCACAAATGCAGGTCCATTATCAGAGCCTATAGATGCTGGCAGCCCAAACCTAGGTATAATCTCTT ?<<;=7=7<:::4<;;;59822+44489996+667::;5;;4;:4::>;;;><6<<;<<<?=>><6;<;;3::3::4;;<7<<>>7?;<;736 AS:i:149 XS:i:149 XN:i:0 XM:i:5 XO:i:1 XG:i:1 NM:i:6 MD:Z:17C3^G0T24G15A1C28 YT:Z:UU
ATF14:01518:01473 16 1 2804295 11 1S30M1D108M1D10M * 0 0 CCCCCTGATATCTTACACCTGTGTGCTGTCCTTTCCCGGTCTCATCATCTGACAGGCCTTGCAGGTGCGGACTATATCCTGGATGGTTTTCTTCTGTTGGGGAAACCACAGCTGCGCTGTTTGTAGGAGTGTCAAAGTCTTTTCTCTCC -<<<==<<@==>7@@?<6<=<<;566<<:55,66,;;6<<989;;;;;;;::::5<5=6=<=<6<<<<6@@==<;;<7:;598942*6664188994;0>>>4>=6<<<<;<<;=<<<<3<<<>=7<:78;99199::6+6666:982; AS:i:250 XS:i:240 XN:i:0 XM:i:5 XO:i:2 XG:i:2 NM:i:7 MD:Z:4C15C9^T20G63A1C21^T10 YT:Z:UU
ATF14:04367:02811 16 1 2804295 11 174M * 0 0 CCCCTGATATCTTACACCTGTGTGCTGTCCTCTTCCCGGTCTCATCATCTGACAGGCCTTGCAGGTGCGGACTATATCCTGGATGGTTTTCTTCTGTTGGGGAAACCACAGCTGCGCTGTTTGTAGGAGTGTCAAAGTCTTTTTCTCTCCCAAATGGGTGGTTTGATGTAAATG -66888::<;;5<<<<6>><<<;?=<:4.448462;:6888877:99::9776859394;:<A7;9<;7;<<<::872<96636.:.::;85877738.:<6085188::97:::93370:::;;5:9689:9289462*6662155/*/2*778/99;5:1:;;<9:93<?:: AS:i:307 XS:i:296 XN:i:0 XM:i:7 XO:i:0 XG:i:0 NM:i:7 MD:Z:4C15C10T19G63A1C42T13 YT:Z:UU
But why I get noting mapped when I ran htseq-count? aligned.bam is the BAM file which represents the sample mapped to sheep genome by Tophat.
Thank you!
One file has chromosomes named "1", the other "chr1". featureCounts will typically deal with that, but htseq-count won't.
Aside from that, whether the first read is included will depend on the MAPQ filtering settings. Further, have a look at the strand settings and compare that to the strand of the feature.
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GTF files don't normally have a transcript feature, just
exon,CDS,start_codon, andstop_codon. Are you sure you're not talking about a GFF file?Atleast GENCODE GTFs have it. The one that I am using right now is from ENSEMBL. It also has the following features:
CDS, start_codon, transcript, gene, exon, Selenocysteine, UTR, stop_codonBTW I thought GFF and GTF are synonymous because it is always written
GFF/GTF.