featureCounts output summary assigned value higher than uniquely mapped reads from HISAT2
1
0
Entering edit mode
6 months ago
Prawesh • 0

Hello all,

Data: Paired end, RNASeq data.

I had an issue with the featureCounts output Assigned reads are greater than the HISAT mapped on aligned concordantly exactly 1 time

From HISAT:
aligned concordantly exactly 1 time is 48335140 

From featureCounts summary:
Assigned: 64074047

Assigned value is 1.32 times greater than HISAT mapping results. It's weird that Assigned value is higher than mapped reads. how do I solve this issue?

I used bam file from hisat2 to extract only uniquely concordant mapped reads code to address the issue but still I get 1.3x greater than hisat. code below:

# Run HISAT2
.......

# extract header from bam and save to sam file
…..

#extract uniquely concordant reads
samtools view sample-sorted.bam | \
awk 'BEGIN{FS="\t";OFS="\t"}{if ($NF=="NH:i:1" && $(NF-2)=="YT:Z:CP"){print $0}}' > \
sample-for-subread.sam

# merge header and sam file above
….

# sam to bam
….

#sort bam for featureCounts
samtools sort -o sample-for-subread-with-header-sorted.bam \
sample-for-subread-with-header.bam

#run featureCounts
  featureCounts  -p -B -d 20 -D 500000 -C --ignoreDup --primary  -Q 1 -t CDS -a reference/canFam3.gtf  -o sample_one_overlap.txt sample-for-subread-with-header-sorted.bam

Output:

featureCounts output:

Assigned    64074047
Unassigned_Unmapped 0
Unassigned_Read_Type    0
Unassigned_Singleton    0
Unassigned_MappingQuality   0
Unassigned_Chimera  0
Unassigned_FragmentLength   0
Unassigned_Duplicate    0
Unassigned_MultiMapping 0
Unassigned_Secondary    0
Unassigned_NonSplit 0
Unassigned_NoFeatures   32309500
Unassigned_Overlapping_Length   0
Unassigned_Ambiguity    286733

HISAT2 Output:

61464086 reads; of these:
  61464086 (100.00%) were paired; of these:
    11848735 (19.28%) aligned concordantly 0 times
    **48335140 (78.64%) aligned concordantly exactly 1 time**
    1280211 (2.08%) aligned concordantly >1 times

Please help me to solve this.

RNA-seq featureCounts HISAT • 863 views
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It's featureCounts, not featureCount. I've edited your post and fixed all mentions of featureCounts.

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What is the output of samtools flagstat?

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6 months ago
Prawesh • 0

I figured out:

Since featureCounts counts fragments and not reads, we have pair-end data that means Assigned value from the output will be divided by 2. i.e 64074047/2 which is lesser than the HISAT alignment.

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You always need to add the following option when you are using -p to count paired-end reads.

--countReadPairs    If specified, fragments (or templates) will be counted
                      instead of reads. This option is only applicable for
                      paired-end reads. For single-end data, it is ignored.
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Please accept your own answer to mark the post as solved.

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