Sam file not create it killed #14
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Hello, I ran into the same issue and can't seem to resolve it: bin/Linux-x64/graphmap2 align -x rnaseq -r /home/alex/Desktop/Zbf_adult_polyA/Zbf_adult/mapping/Danio_rerio.GRCz11.dna.primary_assembly.fa -d /home/alex/Desktop/Zbf_adult_polyA/Zbf_adult/fastq_trimmed/trimmed_10_50_reads.fastq -o alignments.sam AW |
/home/aclab/apps/graphmap2/bin/Linux-x64/graphmap2 align -r Homo_sapiens.fa -i /Drive4/graphmap2/Homo_sapiens.fa.gmidx -d combined_T.fastq -o homo.sam
e313594bd264 runi...[19:21:34 BuildIndexes] Loading reference sequences.
[19:28:18 SetupIndex_] Loading index from file: '/Drive4/graphmap2/Homo_sapiens.fa.gmidx'.
[19:40:42 Index] Memory consumption: [currentRSS = 156693 MB, peakRSS = 217297 MB]
[19:40:42 Run] Hits will be thresholded at the percentil value (percentil: 99.000000%, frequency: 1496).
[19:40:42 Run] Minimizers will be used. Minimizer window length: 5
[19:40:42 Run] Automatically setting the maximum allowed number of regions: max. 5101, attempt to reduce after 0
[19:40:42 Run] Reference genome is assumed to be linear.
[19:40:42 Run] Only one alignment will be reported per mapped read.
[19:40:42 ProcessReads] Reads will be loaded in batches of up to 1024 MB in size.
[19:40:47 ProcessReads] Batch of 482940 reads (1024 MiB) loaded in 4.71 sec. (93960397030528 bases)
[19:40:47 ProcessReads] Memory consumption: [currentRSS = 157878 MB, peakRSS = 217297 MB]
[19:40:47 ProcessReads] Using 24 threads.
[19:40:47 ProcessReads] [CPU time: 4.72 sec, RSS: 157878 MB] Read: 10/482940 (0.00%) [m: 0, u: 0], length = 229, qname: bed425b1-097a-4528-a5a0-8e9c41d99ffb run...
After than it killed.
I have memory 500gb so its not a problem i think but it killed always i tried many times. Can you please help me what is the problem.
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