How to build ribosomal interval files to use in CollectRnaSeqMetrics for hg38.p14
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Entering edit mode
7 months ago
naaj • 0

Hi,

I have been following this post to build my own ribosomal intervals for hg38.p14

Referenc Genome: GRCh38.p5 Ensembl release 84
#
# 
# 1. Prepare chromosome sizes file  from fasta sequence if needed.
#
#     ftp://ftp.ensembl.org/pub/release-84/fasta/homo_sapiens/dna/Homo_sapiens.GRCh38.dna.primary_assembly.fa.gz
#     samtools faidx Homo_sapiens.GRCh38.dna.primary_assembly.fa
#     cut -f1,2 Homo_sapiens.GRCh38.dna.primary_assembly.fa.fai > sizes.genome
#
# 2. Make an interval_list file suitable for CollectRnaSeqMetrics.jar.
#
# Ensembl genes:
#
#   ftp://ftp.ensembl.org/pub/release-84/gtf/homo_sapiens/Homo_sapiens.GRCh38.84.gtf.gz
#
#
#
# Picard Tools CollectRnaSeqMetrics.jar:
#
#   https://broadinstitute.github.io/picard/command-line-overview.html#CollectRnaSeqMetrics

chrom_sizes=sizes.genome

# rRNA interval_list file -------------------------------------------------

# Genes from Ensembl.

genes=/home/dell/Documents/Arindam/Work/ReferenceGenome/Human_84/Annotation/gtf/Homo_sapiens.GRCh38.84.gtf


# Output file suitable for Picard CollectRnaSeqMetrics.jar.

rRNA=GRCh38.p5.rRNA.interval_list

# Sequence names and lengths. (Must be tab-delimited.)
perl -lane 'print "\@SQ\tSN:$F[0]\tLN:$F[1]\tAS:GRCh38"' $chrom_sizes | \
    grep -v _ \ >> "$rRNA"

# Intervals for rRNA transcripts.
grep 'gene_biotype "rRNA"' $genes | \
    awk '$3 == "gene"' | \
    cut -f1,4,5,7,9 | \
    perl -lane '
        /gene_id "([^"]+)"/ or die "no gene_id on $.";
        print join "\t", (@F[0,1,2,3], $1)
    ' | \
    sort -k1V -k2n -k3n \ >> "$rRNA"

But, when I ran the command, I received an error message telling that 'GRCh38.p14.rRNA.interval_list does not contain intervals', what should I do?

I really stuck right now, really clueless what to do next. Any help and guidance are highly appreciated.

hg38.p14 ribosomal-intervals • 937 views
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Entering edit mode
7 months ago
noodle ▴ 590

Edited

IMO if you want to use rRNA intervals for QC you should just stick with something published, like this;

Look for the file GRCh38_rRNA.bed from RSeQC: An RNA-seq Quality Control Package

And then create the interval list using picard (assumes you've already created the dictionary for the genome);

picard BedToIntervalList -I GRCh38_rRNA.bed -O GRCh38_rRNA.bed.intervalList.txt --SEQUENCE_DICTIONARY GRCh38.dict

BUT

If you want the specific files you reference above to work you can try the below (depends on ucsctools);

wget ftp://ftp.ensembl.org/pub/release-84/gtf/homo_sapiens/Homo_sapiens.GRCh38.84.gtf.gz 
wget ftp://ftp.ensembl.org/pub/release-84/fasta/homo_sapiens/dna/Homo_sapiens.GRCh38.dna.primary_assembly.fa.gz
gunzip *
picard CreateSequenceDictionary R=Homo_sapiens.GRCh38.dna.primary_assembly.fa O=Homo_sapiens.GRCh38.dna.primary_assembly.fa.dict
grep 'rRNA' Homo_sapiens.GRCh38.84.gtf  > Homo_sapiens.GRCh38.84.rRNA.gtf 
gtfToGenePred -genePredExt -geneNameAsName2 Homo_sapiens.GRCh38.84.rRNA.gtf Homo_sapiens.GRCh38.84.rRNA.gtf.genePred
awk 'BEGIN{OFS="\t"} {print $2, $4, $5, $3, $12}' Homo_sapiens.GRCh38.84.rRNA.gtf.genePred > Homo_sapiens.GRCh38.84.rRNA.gtf.genePred.shortlist
cat Homo_sapiens.GRCh38.dna.primary_assembly.fa.dict Homo_sapiens.GRCh38.84.rRNA.gtf.genePred.shortlist > Homo_sapiens.GRCh38.84.rRNA.intervals.list
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Entering edit mode

Thank you for your help. I created the rRNA interval list using yours, however when I ran CollectRnaSeqMetrics using this command

java -jar $PICARD_JAR/picard.jar CollectRnaSeqMetrics \
      I=/mnt/iusers01/jw01/c02544na/training/dummy/AB1_gencode44_trimmed_TruSeq3_readcountAligned.sortedByCoord.out.bam \
      O=AB1_output.RNA_Metrics \
      REF_FLAT=/mnt/iusers01/jw01/c02544na/refFlat.txt \
      STRAND=SECOND_READ_TRANSCRIPTION_STRAND \
      RIBOSOMAL_INTERVALS=/mnt/iusers01/jw01/c02544na/training/dummy/psa_transcriptomic_training/Homo_sapiens.GRCh38.111.rRNA.intervals.list 

and, I received this error message

To get help, see http://broadinstitute.github.io/picard/index.html#GettingHelp
Exception in thread "main" htsjdk.tribble.TribbleException: Invalid interval record contains 1 fields: 1 9437668 9437778 - RNA5SP40
    at htsjdk.tribble.IntervalList.IntervalListCodec.parseIntervalString(IntervalListCodec.java:73)
    at htsjdk.tribble.IntervalList.IntervalListCodec.decode(IntervalListCodec.java:130)
    at htsjdk.samtools.util.IntervalList.fromReader(IntervalList.java:529)
    at htsjdk.samtools.util.IntervalList.fromPath(IntervalList.java:458)
    at htsjdk.samtools.util.IntervalList.fromFile(IntervalList.java:447)
    at picard.analysis.directed.RnaSeqMetricsCollector.makeOverlapDetector(RnaSeqMetricsCollector.java:79)
    at picard.analysis.CollectRnaSeqMetrics.setup(CollectRnaSeqMetrics.java:168)
    at picard.analysis.SinglePassSamProgram.makeItSo(SinglePassSamProgram.java:145)
    at picard.analysis.SinglePassSamProgram.doWork(SinglePassSamProgram.java:94)
    at picard.cmdline.CommandLineProgram.instanceMain(CommandLineProgram.java:280)
    at picard.cmdline.PicardCommandLine.instanceMain(PicardCommandLine.java:105)
    at picard.cmdline.PicardCommandLine.main(PicardCommandLine.java:115)

What should I do to fix this?

Many thanks

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Entering edit mode

Ah, I think the awk is printed space-separated instead of tab-separated. I updated my awk comment adding BEGIN{OFS="\t"}

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Entering edit mode

Thanks a lot. It works perfectly :)

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Entering edit mode

Just a final comment - it looks like the only rRNAs in the gtf are 5S and depending on how you do the library prep these might be lost during size selection. You should make sure that the larger rRNAs are included in this type of analysis, otherwise it won't be accurate.

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How to make sure the larger rRNAs are included?

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Find an annotation that contains them, or create it yourself.

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