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Currently, I am trying to use the PERL script of GFusion [https://github.com/xiaofengsong/GFusion].
In half of the execution, it throws an error because bowtie executed unrecognized option '--reorder' (an option of bowtie2). When I try to use bowtie2 indexes, tophat doesn't recognize them because it is searching bowtie indexes only. The script doesn't have any '--reorder' and it is implemented for bowtie 1. Do you know what could be the problem?
Then, an error appeared because Bow tie didn't recognize the option --reorder:
[Tue Dec 4 18:57:08 2018]
[2018-12-04 18:57:08] Beginning TopHat run (v2.1.0)
-----------------------------------------------
[2018-12-04 18:57:08] Checking for Bowtie
Bowtie version: 1.1.2.0
[2018-12-04 18:57:10] Checking for Bowtie index files (genome)..
[2018-12-04 18:57:10] Checking for reference FASTA file
[2018-12-04 18:57:10] Generating SAM header for /mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/BowtieIndex/genome
[2018-12-04 18:57:31] Preparing reads
left reads: min. length=50, max. length=50, 84131 kept reads (113 discarded)
right reads: min. length=50, max. length=50, 83725 kept reads (519 discarded)
[2018-12-04 18:57:33] Mapping left_kept_reads to genome genome with Bowtie
[FAILED]
Error running bowtie:
bowtie: unrecognized option '--reorder'
Usage:
bowtie [options]* <ebwt> {-1 <m1> -2 <m2> | --12 <r> | <s>} [<hit>]
<m1> Comma-separated list of files containing upstream mates (or the
sequences themselves, if -c is set) paired with mates in <m2>
<m2> Comma-separated list of files containing downstream mates (or the
sequences themselves if -c is set) paired with mates in <m1>
<r> Comma-separated list of files containing Crossbow-style reads. Can be
a mixture of paired and unpaired. Specify "-" for stdin.
<s> Comma-separated list of files containing unpaired reads, or the
sequences themselves, if -c is set. Specify "-" for stdin.
<hit> File to write hits to (default: stdout)
Input:
-q query input files are FASTQ .fq/.fastq (default)
-f query input files are (multi-)FASTA .fa/.mfa
-r query input files are raw one-sequence-per-line
-c query sequences given on cmd line (as <mates>, <singles>)
-C reads and index are in colorspace
-Q/--quals <file> QV file(s) corresponding to CSFASTA inputs; use with -f -C
--Q1/--Q2 <file> same as -Q, but for mate files 1 and 2 respectively
-s/--skip <int> skip the first <int> reads/pairs in the input
-u/--qupto <int> stop after first <int> reads/pairs (excl. skipped reads)
-5/--trim5 <int> trim <int> bases from 5' (left) end of reads
-3/--trim3 <int> trim <int> bases from 3' (right) end of reads
--phred33-quals input quals are Phred+33 (default)
--phred64-quals input quals are Phred+64 (same as --solexa1.3-quals)
--solexa-quals input quals are from GA Pipeline ver. < 1.3
--solexa1.3-quals input quals are from GA Pipeline ver. >= 1.3
--integer-quals qualities are given as space-separated integers (not ASCII)
--large-index force usage of a 'large' index, even if a small one is present
Alignment:
-v <int> report end-to-end hits w/ <=v mismatches; ignore qualities
or
-n/--seedmms <int> max mismatches in seed (can be 0-3, default: -n 2)
-e/--maqerr <int> max sum of mismatch quals across alignment for -n (def: 70)
-l/--seedlen <int> seed length for -n (default: 28)
--nomaqround disable Maq-like quality rounding for -n (nearest 10 <= 30)
-I/--minins <int> minimum insert size for paired-end alignment (default: 0)
-X/--maxins <int> maximum insert size for paired-end alignment (default: 250)
--fr/--rf/--ff -1, -2 mates align fw/rev, rev/fw, fw/fw (default: --fr)
--nofw/--norc do not align to forward/reverse-complement reference strand
--maxbts <int> max # backtracks for -n 2/3 (default: 125, 800 for --best)
--pairtries <int> max # attempts to find mate for anchor hit (default: 100)
-y/--tryhard try hard to find valid alignments, at the expense of speed
--chunkmbs <int> max megabytes of RAM for best-first search frames (def: 64)
Reporting:
-k <int> report up to <int> good alignments per read (default: 1)
-a/--all report all alignments per read (much slower than low -k)
-m <int> suppress all alignments if > <int> exist (def: no limit)
-M <int> like -m, but reports 1 random hit (MAPQ=0); requires --best
--best hits guaranteed best stratum; ties broken by quality
--strata hits in sub-optimal strata aren't reported (requires --best)
Output:
-t/--time print wall-clock time taken by search phases
-B/--offbase <int> leftmost ref offset = <int> in bowtie output (default: 0)
--quiet print nothing but the alignments
--refout write alignments to files refXXXXX.map, 1 map per reference
--refidx refer to ref. seqs by 0-based index rather than name
--al <fname> write aligned reads/pairs to file(s) <fname>
--un <fname> write unaligned reads/pairs to file(s) <fname>
--max <fname> write reads/pairs over -m limit to file(s) <fname>
--suppress <cols> suppresses given columns (comma-delim'ed) in default output
--fullref write entire ref name (default: only up to 1st space)
Colorspace:
--snpphred <int> Phred penalty for SNP when decoding colorspace (def: 30)
or
--snpfrac <dec> approx. fraction of SNP bases (e.g. 0.001); sets --snpphred
--col-cseq print aligned colorspace seqs as colors, not decoded bases
--col-cqual print original colorspace quals, not decoded quals
--col-keepends keep nucleotides at extreme ends of decoded alignment
SAM:
-S/--sam write hits in SAM format
--mapq <int> default mapping quality (MAPQ) to print for SAM alignments
--sam-nohead supppress header lines (starting with @) for SAM output
--sam-nosq supppress @SQ header lines for SAM output
--sam-RG <text> add <text> (usually "lab=value") to @RG line of SAM header
Performance:
-o/--offrate <int> override offrate of index; must be >= index's offrate
-p/--threads <int> number of alignment threads to launch (default: 1)
--mm use memory-mapped I/O for index; many 'bowtie's can share
--shmem use shared mem for index; many 'bowtie's can share
Other:
--seed <int> seed for random number generator
--verbose verbose output (for debugging)
--version print version information and quit
-h/--help print this usage message
Command: bowtie --wrapper basic-0 -v 2 -k 20 -m 20 -S -p 12 --reorder --sam-nohead --max /dev/null /mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/BowtieIndex/genome -
open: No such file or directory
[main_samview] fail to open "output1/accepted_hits.bam" for reading.
open: No such file or directory
[main_samview] fail to open "output1/unmapped.bam" for reading.
[Tue Dec 4 18:57:33 2018]
Warning: Could not find any reads in "output1/un.fastq"
# reads processed: 0
# reads with at least one reported alignment: 0 (0.00%)
# reads that failed to align: 0 (0.00%)
No alignments
[samopen] SAM header is present: 195 sequences.
[sam_read1] reference 'ID:Bowtie VN:1.1.2 CL:"bowtie --wrapper basic-0 -p 12 /mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/BowtieIndex/genome output1/un.fastq -S output1/fusion_out/un.sam"
r3 LN:198295559
@SQ SN:chr4 LN:190214555
@SQ SN:chr5 LN:181538259
@SQ !' is recognized as '*'.
[main_samview] truncated file.
[samopen] SAM header is present: 195 sequences.
[sam_read1] reference 'ID:Bowtie VN:1.1.2 CL:"bowtie --wrapper basic-0 -p 12 /mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/BowtieIndex/genome output1/un.fastq -S output1/fusion_out/un.sam"
hr3 LN:198295559
@SQ SN:chr4 LN:190214555
@SQ SN:chr5 LN:181538259
@SQ!' is recognized as '*'.
[main_samview] truncated file.
open: No such file or directory
[main_samview] fail to open "output1/accepted_hits.bam" for reading.
open: No such file or directory
[main_samview] fail to open "output1/accepted_hits.bam" for reading.
[samopen] no @SQ lines in the header.
[sam_read1] missing header? Abort!
[bam_header_read] EOF marker is absent. The input is probably truncated.
[Tue Dec 4 18:57:37 2018]
Result: No Fusion Genes! The time elapsed: about 0 hours.
[Tue Dec 4 19:01:33 2018]
[2018-12-04 19:01:33] Beginning TopHat run (v2.1.0)
-----------------------------------------------
[2018-12-04 19:01:33] Checking for Bowtie
Bowtie version: 1.1.2.0
[2018-12-04 19:01:33] Checking for Bowtie index files (genome)..
Error: Could not find Bowtie index files (/mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/Bowtie2Index/genome.*.ebwt)
open: No such file or directory
[main_samview] fail to open "output1/accepted_hits.bam" for reading.
open: No such file or directory
[main_samview] fail to open "output1/unmapped.bam" for reading.
[Tue Dec 4 19:01:33 2018]
Could not locate a Bowtie index corresponding to basename "/mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/Bowtie2Index/genome"
Command: bowtie --wrapper basic-0 -p 12 -S /mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/Bowtie2Index/genome output1/un.fastq output1/fusion_out/un.sam
[samopen] SAM header is present: 195 sequences.
[sam_read1] reference 'ID:Bowtie VN:1.1.2 CL:"bowtie --wrapper basic-0 -p 12 /mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/BowtieIndex/genome output1/un.fastq -S output1/fusion_out/un.sam"
r3 LN:198295559
@SQ SN:chr4 LN:190214555
@SQ SN:chr5 LN:181538259
@SQ !' is recognized as '*'.
[main_samview] truncated file.
[samopen] SAM header is present: 195 sequences.
[sam_read1] reference 'ID:Bowtie VN:1.1.2 CL:"bowtie --wrapper basic-0 -p 12 /mnt/home/soft/human/data/hg38_illumina/Homo_sapiens/NCBI/GRCh38/Sequence/BowtieIndex/genome output1/un.fastq -S output1/fusion_out/un.sam"
hr3 LN:198295559
@SQ SN:chr4 LN:190214555
@SQ SN:chr5 LN:181538259
@SQ!' is recognized as '*'.
[main_samview] truncated file.
open: No such file or directory
[main_samview] fail to open "output1/accepted_hits.bam" for reading.
open: No such file or directory
[main_samview] fail to open "output1/accepted_hits.bam" for reading.
[samopen] no @SQ lines in the header.
[sam_read1] missing header? Abort!
[bam_header_read] EOF marker is absent. The input is probably truncated.
[Tue Dec 4 19:01:35 2018]
Result: No Fusion Genes! The time elapsed: about 0 hours.
I don't know how to solve this situation exactly. It looks like it works with hg19 but that shouldn't be the problem. Thanks in advance.
The text was updated successfully, but these errors were encountered:
Damtagor
changed the title
What bowtie is it using?
What's wrong with bowtie?
Dec 12, 2018
Damtagor
changed the title
What's wrong with bowtie?
What's wrong with bowtie? (--reorder option with bowtie1)
Dec 12, 2018
Currently, I am trying to use the PERL script of GFusion [https://github.com/xiaofengsong/GFusion].
In half of the execution, it throws an error because bowtie executed unrecognized option '--reorder' (an option of bowtie2). When I try to use bowtie2 indexes, tophat doesn't recognize them because it is searching bowtie indexes only. The script doesn't have any '--reorder' and it is implemented for bowtie 1. Do you know what could be the problem?
I used this command:
Then, an error appeared because Bow tie didn't recognize the option --reorder:
After this, I used Bowtie2 indexes:
But the script doesn't use that type of indexes:
I don't know how to solve this situation exactly. It looks like it works with hg19 but that shouldn't be the problem. Thanks in advance.
The text was updated successfully, but these errors were encountered: