I have encountered some bugs in transcriptome analysis using STAR and RSEM.
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7 weeks ago
Pallondyle • 0

I'm trying to analyze a set of RNA-seq data, and a subset of my data hasn't generated the results. The code I use:

for i in {KO1_1,KO1_2,KO1_3,KO2_1,KO2_2,KO2_3,KO_Ctrl_1,KO_Ctrl_2,KO_Ctrl_3,OE1_1,OE1_2,OE1_3,OE_NC_1,OE_NC_2,OE_NC_3};
do
## STAR alignment
STAR --twopassMode Basic \
    --quantMode TranscriptomeSAM GeneCounts \
    --runThreadN 6 \
    --genomeDir index/STAR_index_hg38+V41 \
    --alignIntronMin 20 \
    --alignIntronMax 50000 \
    --outSAMtype BAM SortedByCoordinate \
    --sjdbOverhang 149 \
    --outSAMattrRGline ID:sample SM:sample PL:ILLUMINA \
    --outFilterMismatchNmax 2 \
    --outSJfilterReads Unique \
    --outSAMmultNmax 1 \
    --outFileNamePrefix ${i} \
    --outSAMmapqUnique 60 \
    --readFilesCommand gunzip -c \
    --readFilesIn rawdata/Bianlab_RNA_seq/${i}_1.fq.gz rawdata/Bianlab_RNA_seq/${i}_2.fq.gz

## RSEM count
rsem-calculate-expression --paired-end --no-bam-output \
--alignments -p 15 \
--bam ${i}Aligned.toTranscriptome.out.bam \
index/RSEM_index_hg38+V41/RSEM_index_hg38+V41 \
intermediate_data/${i}_

done

I tried to rerun the groups that did not generate results, and encountered following error:

rsem-calculate-expression --paired-end --no-bam-output \
> --alignments -p 15 \
> --bam OE1_2Aligned.toTranscriptome.out.bam \
> index/RSEM_index_hg38+V41/RSEM_index_hg38+V41 \
> intermediate_data/OE1_2_
rsem-parse-alignments index/RSEM_index_hg38+V41/RSEM_index_hg38+V41 intermediate_data/OE1_2_.temp/OE1_2_ intermediate_data/OE1_2_.stat/OE1_2_ OE1_2Aligned.toTranscriptome.out.bam 3 -tag XM
[samopen] no @SQ lines in the header.
The SAM/BAM file declares less than one reference sequence!
"rsem-parse-alignments index/RSEM_index_hg38+V41/RSEM_index_hg38+V41 intermediate_data/OE1_2_.temp/OE1_2_ intermediate_data/OE1_2_.stat/OE1_2_ OE1_2Aligned.toTranscriptome.out.bam 3 -tag XM" failed! Plase check if you provide correct parameters/options for the pipeline!

I tried to check the bam file, however, the result is as:

samtools view OE1_2Aligned.toTranscriptome.out.bam
[main_samview] fail to read the header from "OE1_2Aligned.toTranscriptome.out.bam".

I am currently confused about which step's parameters have been called incorrectly, preventing me from obtaining the results.

STAR RSEM • 985 views
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what is the output of

file *.out.bam

?

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oops

file *.out.bam
KO1_2Aligned.sortedByCoord.out.bam:       gzip compressed data, extra field
KO1_2Aligned.toTranscriptome.out.bam:     gzip compressed data, extra field
KO1_3Aligned.sortedByCoord.out.bam:       gzip compressed data, extra field
KO1_3Aligned.toTranscriptome.out.bam:     gzip compressed data, extra field
KO2_1Aligned.sortedByCoord.out.bam:       gzip compressed data, extra field
KO2_1Aligned.toTranscriptome.out.bam:     gzip compressed data, extra field
KO2_2Aligned.sortedByCoord.out.bam:       gzip compressed data, extra field
KO2_2Aligned.toTranscriptome.out.bam:     gzip compressed data, extra field
KO2_3Aligned.sortedByCoord.out.bam:       gzip compressed data, extra field
KO2_3Aligned.toTranscriptome.out.bam:     gzip compressed data, extra field
KO_Ctrl_1Aligned.sortedByCoord.out.bam:   gzip compressed data, extra field
KO_Ctrl_1Aligned.toTranscriptome.out.bam: gzip compressed data, extra field
KO_Ctrl_2Aligned.sortedByCoord.out.bam:   gzip compressed data, extra field
KO_Ctrl_2Aligned.toTranscriptome.out.bam: gzip compressed data, extra field
KO_Ctrl_3Aligned.sortedByCoord.out.bam:   gzip compressed data, extra field
KO_Ctrl_3Aligned.toTranscriptome.out.bam: gzip compressed data, extra field
OE1_1Aligned.sortedByCoord.out.bam:       gzip compressed data, extra field
OE1_1Aligned.toTranscriptome.out.bam:     gzip compressed data, extra field
OE1_2Aligned.sortedByCoord.out.bam:       empty
OE1_2Aligned.toTranscriptome.out.bam:     empty
OE1_3Aligned.sortedByCoord.out.bam:       empty
OE1_3Aligned.toTranscriptome.out.bam:     empty
OE_NC_1Aligned.sortedByCoord.out.bam:     empty
OE_NC_1Aligned.toTranscriptome.out.bam:   empty
OE_NC_2Aligned.sortedByCoord.out.bam:     gzip compressed data, extra field
OE_NC_2Aligned.toTranscriptome.out.bam:   gzip compressed data, extra field
OE_NC_3Aligned.sortedByCoord.out.bam:     gzip compressed data, extra field
OE_NC_3Aligned.toTranscriptome.out.bam:   gzip compressed data, extra field
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However, OE1_2 and OE1_3 are not the only groups experiencing problems. I tried another non-empty file, and:

rsem-calculate-expression --paired-end --no-bam-output \
> --alignments -p 15 \
> --bam OE_NC_2Aligned.toTranscriptome.out.bam \
> index/RSEM_index_hg38+V41/RSEM_index_hg38+V41 \
> intermediate_data/OE_NC_2_
rsem-parse-alignments index/RSEM_index_hg38+V41/RSEM_index_hg38+V41 intermediate_data/OE_NC_2_.temp/OE_NC_2_ intermediate_data/OE_NC_2_.stat/OE_NC_2_ OE_NC_2Aligned.toTranscriptome.out.bam 3 -tag XM
Done!

rsem-build-read-index 32 1 0 intermediate_data/OE_NC_2_.temp/OE_NC_2__alignable_1.fq intermediate_data/OE_NC_2_.temp/OE_NC_2__alignable_2.fq
Cannot open intermediate_data/OE_NC_2_.temp/OE_NC_2__alignable_1.fq! It may not exist.
"rsem-build-read-index 32 1 0 intermediate_data/OE_NC_2_.temp/OE_NC_2__alignable_1.fq intermediate_data/OE_NC_2_.temp/OE_NC_2__alignable_2.fq" failed! Plase check if you provide correct parameters/options for the pipeline!
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The most torturous thing is that some groups did indeed generate results.

ls intermediate_data
KO1_1_.stat              KO1_3_.isoforms.results  KO2_2_.isoforms.results   KO_Ctrl_1_.isoforms.results  KO_Ctrl_3_.isoforms.results  OE1_2_.temp    OE_NC_2_.temp
KO1_1_.temp              KO1_3_.stat              KO2_2_.stat               KO_Ctrl_1_.stat              KO_Ctrl_3_.stat              OE1_3_.stat    OE_NC_3_.stat
KO1_2_.genes.results     KO2_1_.genes.results     KO2_3_.genes.results      KO_Ctrl_2_.genes.results     OE1_1_.genes.results         OE1_3_.temp    OE_NC_3_.temp
KO1_2_.isoforms.results  KO2_1_.isoforms.results  KO2_3_.isoforms.results   KO_Ctrl_2_.isoforms.results  OE1_1_.isoforms.results      OE_NC_1_.stat
KO1_2_.stat              KO2_1_.stat              KO2_3_.stat               KO_Ctrl_2_.stat              OE1_1_.stat                  OE_NC_1_.temp
KO1_3_.genes.results     KO2_2_.genes.results     KO_Ctrl_1_.genes.results  KO_Ctrl_3_.genes.results     OE1_2_.stat                  OE_NC_2_.stat

I'm so confused...

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Cannot open intermediate_data/OE_NC_2_.temp/OE_NC_2__alignable_1.fq! It may not exist.

Looks like you are missing some files.

BTW this is not a bugsince those are generally problems associated with programs themselves. This seems to be an issue with your execution and/or data.

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Their .fq files all look similar, should I rerun these programs?

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Since we don't have access to your data we can't comment. Check the integrity of your input data files. Validate the files if you are not sure about their contents.

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It seems that the files that generated the results also have significant issues. Except for one sample, all other samples only have over 200 transcripts with non-zero counts.

> table(df$intermediate_data.KO1_2_.genes.results==0)

FALSE  TRUE 
  295 20934
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One of them looks okay, but I don't quite believe it.

> table(df$`intermediate_data.OE1_1_.genes.results`==0)

FALSE  TRUE 
21200    29
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Pallondyle : Use ADD REPLY/ADD COMMENT to add additional information to existing threads. ADD YOUR ANSWER is meant for adding new answers to the original question.

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Can you check using featureCounts to make sure things look reasonable with alignments? You could also use salmon to do transcript quantitation instead of rsem.

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Thx. I found out that I used the wrong reference genome. I have a set of data from mice and a set from humans. I processed the human data using the mouse reference genome and the mouse data using the human reference genome.

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7 weeks ago
Michael 55k

Something went wrong during star alignments of samples OE1_2, OE1_3, and OE_NC_1. The obvious place to look for the reason is in the Star logs.

Try cat OE1_2*Log*. This should point you to the root cause of the problem.

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Thx. It turns out that the file was damaged during transmission.

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Ok, that's quite common but can cause a lot of fuzz (if you notice it, even more if it goes unnoticed). Try to check the md5 sums generated by the sequencing facility and do a round of fastp->multiqc before each analysis run.

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