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Name Modified Size InfoDownloads / Week
Parent folder
reference.fasta1.pac 2014-11-18 251.0 kB
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reference.fasta1.rbwt 2014-11-18 376.5 kB
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reference.fasta1.rpac 2014-11-18 251.0 kB
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reference.fasta1.rsa 2014-11-18 125.5 kB
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reference.fasta2 2014-11-18 1.0 MB
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reference.fasta2.amb 2014-11-18 12 Bytes
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reference.fasta2.ann 2014-11-18 36 Bytes
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reference.fasta2.bwt 2014-11-18 376.5 kB
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reference.fasta2.pac 2014-11-18 251.0 kB
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reference.fasta2.rbwt 2014-11-18 376.5 kB
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reference.fasta2.rpac 2014-11-18 251.0 kB
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reference.fasta2.rsa 2014-11-18 125.5 kB
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reference.fasta2.sa 2014-11-18 125.5 kB
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reference.fasta3 2014-11-18 1.0 MB
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reference.fasta3.bwt 2014-11-18 376.5 kB
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reference.fasta3.pac 2014-11-18 251.0 kB
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reference.fasta3.rbwt 2014-11-18 376.5 kB
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reference.fasta3.rpac 2014-11-18 251.0 kB
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reference.fasta3.rsa 2014-11-18 125.5 kB
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reference.fasta3.sa 2014-11-18 125.5 kB
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reference.fasta4 2014-11-18 1.0 MB
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reference.fasta4.bwt 2014-11-18 376.5 kB
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reference.fasta4.pac 2014-11-18 251.0 kB
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reference.fasta4.rbwt 2014-11-18 376.5 kB
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reference.fasta4.rpac 2014-11-18 251.0 kB
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reference.fasta4.rsa 2014-11-18 125.5 kB
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reference.fasta4.sa 2014-11-18 125.5 kB
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reference.fasta5.bwt 2014-11-18 375.7 kB
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reference.fasta5.pac 2014-11-18 250.4 kB
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reference.fasta5.rbwt 2014-11-18 375.7 kB
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reference.fasta5.rpac 2014-11-18 250.4 kB
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reference.fasta5.rsa 2014-11-18 125.3 kB
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reference.fasta5.sa 2014-11-18 125.3 kB
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reference.fasta1.bwt 2014-11-18 376.5 kB
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reference.fasta1.ann 2014-11-18 36 Bytes
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reference.fasta1.amb 2014-11-18 12 Bytes
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reference.fasta0.sa 2014-11-18 125.3 kB
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reference.fasta0.rsa 2014-11-18 125.3 kB
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reference.fasta0.rpac 2014-11-18 250.5 kB
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reference.fasta0.rbwt 2014-11-18 375.8 kB
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reference.fasta0.pac 2014-11-18 250.5 kB
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reference.fasta0.bwt 2014-11-18 375.8 kB
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reference.fasta0.ann 2014-11-18 36 Bytes
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reference.fasta0.amb 2014-11-18 12 Bytes
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reference.fasta0 2014-11-18 1.0 MB
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reference.fasta.sa 2014-11-18 750.0 kB
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reference.fasta.rsa 2014-11-18 750.0 kB
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reference.fasta.rpac 2014-11-18 1.5 MB
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reference.fasta.rbwt 2014-11-18 2.2 MB
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reference.fasta.pac 2014-11-18 1.5 MB
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reference.fasta.bwt 2014-11-18 2.2 MB
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reference.fasta.ann 2014-11-18 127 Bytes
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reference.fasta.amb 2014-11-18 28 Bytes
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reference.fasta1 2014-11-18 1.0 MB
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reference.fasta 2014-11-18 6.1 MB
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split.txt 2014-11-18 1.7 MB
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picture.txt 2014-11-18 7.2 kB
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indi2.split.txt 2014-11-18 809.8 kB
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indi1.split.txt 2014-11-18 868.7 kB
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called_indi1_chr1.txt 2014-11-18 1.6 kB
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called_combine.txt 2014-11-18 2.8 kB
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Totals: 69 Items   33.5 MB 0 
SVseq is a tool to call deletions with exact break points. 

To learn how to use the program:
1 copy the proper program from executable/ to demo/
2 follow demo/demo.txt
3 compare the results with /demo/result/

Samtools is needed for the caller utility.

The input files are of 3 categories:
(1) anchor.
With the format: chromosome\tleft_position\tstrand\n
0 for forward strand, 1 for reverse strand.
(2) fastq.
The unmapped reads. 
(3) BAM files. That contains pair with both ends mapped.

Note: 
This version set a threshold >=50 on deletion length. 
Currently only works with paired-end reads.
For the fastq file: If a read is from BAM files, make sure it is not the reverse complement.
The insert size is defined as the left point to left point of a pair in this version.


Contact

Jin Zhang
jinzhang@engr.uconn.edu 
http://www.engr.uconn.edu/~jiz08001
Source: README.txt, updated 2014-11-18