HT-seq error and empty result
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7.9 years ago
biologo ▴ 40

hello, friends:

i was using the htseq to calclate the reads, but it was sth wrong, like that:

Error occured when processing SAM input (line 35008273 of file sort.sam):
  'pair_alignments' needs a sequence of paired-end alignments
  [Exception type: ValueError, raised in __init__.py:603]

the input the paired_end reads, and i also do like this:

samtools sort -n uniqmap.bam -o sort.bam
samtools view -@ 4 sort.bam -O SAM -o sort.sam
htseq-count -m union -s no sort.sam $GTF > union.out

i check it for several times, but still in upset, i am looking forward your reply, thanks

RNA-Seq • 3.1k views
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As it says, HTSeq-count expects paired-end alignments but did not find it there. Maybe, in your uniqmap.bam a part of the read was filtered out, because it was not uniquely mapping whilst the other part did. I'd check that.

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I already told him he didn't have to pre-filter earlier in this thread: what's wrong with htseq-count codes???

But reading is hard.

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dear WouterDeCoster, i am so sorry, cause such a busy day. well, some guys told me maybe the main problem is the original bam file (tophat2 output), since i am still a newbie,,,but i do not think the original file error. anyway, thank you for your kind help, i will till you the result later.

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it empty again: samtools sort -@ 15 -n accepted_hits.bam -o accepted_hits_sort.bam htseq-count -f bam -m union -s no accepted_hits_sort.bam $GTF > union.out

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even the orignal file, it empty again

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What is empty? Could you be more specific? Earlier you were talking about that error message, but now it's something else?

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Yes, the same error message. I try to search the answer, and maybe caused by the original bam file from tophat2 which mixed with paired and single reads, and then i do the seperation.(that before even mixed, i never met this error.) J00142:73:HGKWTBBXX:2:1101:1215:7679 65 chr5 156482411 50 55M chr16 3454521 0 GCCATTTTGGCATGTGAATAGAGAACATGAGCCTCTATTCCAGCACATTGATGTG FJAFJFFJJF<jffjjjjjj7afjfjfjjf-f-aj<jjjjjj7f<a7f<fajjj&lt; as:i:-4="" xn:i:0="" xm:i:1="" xo:i:0="" xg:i:0="" nm:i:1="" md:z:48g6="" yt:z:uu="" xs:a:-="" nh:i:1="" j00142:73:hgkwtbbxx:2:2227:1215:43796="" 0="" chrmt="" 10806="" 50="" 42m="" *="" 0="" 0="" gactttccaaaaaacacataatttgaatcaacacaaccaccc="" fjj<affjfjjjjjjjjjff<jjjfffjjjajjjffjjjjjj="" as:i:0="" xn:i:0="" xm:i:0="" xo:i:0="" xg:i:0="" nm:i:0="" md:z:42="" yt:z:uu="" xs:a:+="" nh:i:1<="" p="">

HTseq-count successed, but the tough thing is the bam file i would used for macs2 callpeak, and mixed one seems does not work. again, i am so happy for your reply.

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dear michael.ante: thank you for your kind suggestion, it was running now. well ,cause the bam file i would use next in another software, and it report error, even the accepted_hits.bam, and after that i used the bed file in success days ago. but till yesterday, i started to think about what's wrong with bamfile and do HT-seq again, then post it.

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I'm not sure what's wrong, but htseq-count can take bam files so there is no need to convert to sam. See the -f flag in the manual

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thanks a lot, i will do try later, but question is still there.

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finally, i find what's wrong, cause on the processing of clean_data, i use the single-end way, which cause the unpaired reads. thank you for your precious time.

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