featureCount Error "No paired-end reads were detected in paired-end read library"
1
0
Entering edit mode
12 months ago
cook.675 ▴ 230

I created a combined mm39 and MHV-A59 (Viral) reference genome and aligned my paired end reads using STAR with the following input commands:

STAR 
--runMode alignReads   
--runThreadN 16   
--genomeDir /genomeDir   
--readFilesIn /FastqDir/1.fq.gz, /FastqDir/2.fq.gz      
--readFilesCommand gunzip   -c      
--outReadsUnmapped Fastx   
--outSAMtype BAM   SortedByCoordinate 

It seems that everything went fine. Here is a result from one of the alignments:

                                 Started job on |   Nov 14 20:08:30
                         Started mapping on |   Nov 14 20:09:03
                                Finished on |   Nov 14 20:15:12
   Mapping speed, Million of reads per hour |   808.26

                      Number of input reads |   82847062
                  Average input read length |   150
                                UNIQUE READS:
               Uniquely mapped reads number |   77656936
                    Uniquely mapped reads % |   93.74%
                      Average mapped length |   149.28
                   Number of splices: Total |   37645057
        Number of splices: Annotated (sjdb) |   37376062
                   Number of splices: GT/AG |   37313095
                   Number of splices: GC/AG |   265167
                   Number of splices: AT/AC |   28575
           Number of splices: Non-canonical |   38220
                  Mismatch rate per base, % |   0.26%
                     Deletion rate per base |   0.01%
                    Deletion average length |   1.82
                    Insertion rate per base |   0.01%
                   Insertion average length |   1.57
                         MULTI-MAPPING READS:
    Number of reads mapped to multiple loci |   3072281
         % of reads mapped to multiple loci |   3.71%
    Number of reads mapped to too many loci |   98073
         % of reads mapped to too many loci |   0.12%
                              UNMAPPED READS:
   % of reads unmapped: too many mismatches |   0.00%
             % of reads unmapped: too short |   2.37%
                 % of reads unmapped: other |   0.07%
                              CHIMERIC READS:
                   Number of chimeric reads |   0
                        % of chimeric reads |   0.00%

Now I take this BAM file and run it through featureCount with the following parameters, where combined gtf is my mm39 and MHV-A59 gtf file I used for making the index:

featureCounts(files="/Users/BamFile.bam",
                          annot.ext = "/Users/combined.gtf", 
                          isGTFAnnotationFile = TRUE,
                          isPairedEnd=TRUE, 
                          requireBothEndsMapped = TRUE,
                          countReadPairs = TRUE,
                          strandSpecific = 2)

And I get the following error: ERROR: No paired-end reads were detected in paired-end read library

I feel like this must be a result of the combined mouse and viral reference but I cant quite figure out what it wrong. I checked and it looks like I have reads mapped to the viral genome so I think everything went smoothly on the mapping side. Any advice would be greatly appreciated!!!

Subread RNAseq featureCount • 1.0k views
ADD COMMENT
0
Entering edit mode
12 months ago

The R1 and R2 reads should be space separated for paired end alignment. If you comma separate them they get concatenated and treated as one file.

ADD COMMENT
0
Entering edit mode

beautiful thank you so much!

ADD REPLY

Login before adding your answer.

Traffic: 1661 users visited in the last hour
Help About
FAQ
Access RSS
API
Stats

Use of this site constitutes acceptance of our User Agreement and Privacy Policy.

Powered by the version 2.3.6