SYNOPSIS
findknownsnps <options>
DESCRIPTION
findknownsnps is the main executable for the snpomatic software.
OPTIONS
These options control whether output is written to file(s), standard output, or directly to a man pager.
--genome=GENOME_FILE
- FASTA file with chromosomes (mandatory)
--fasta=FASTA_FILE
- FASTA file with Solexa reads (mandatory, except when --fastq or --index is used)
--fasta=FASTA_FILE
- FASTA file with Solexa reads (mandatory, except when --fastq or --index is used)
--fastq=FASTQ_FILE
- FASTQ file with Solexa reads (mandatory, except when --fasta or --index is used)
--fastq2=FASTQ_FILE2
- FASTQ file with Solexa reads (optional; read mate)
--nono=FILENAME
- File with list of read names (!) to ignore (optional)
--regions=REGION_FILE
- Region file for finding new SNPs (optional) [DEPRECATED]
--snps=SNP_FILE
- Simple SNP file (optional)
--gff=GFF_FILE
- GFF file with SNPs (optional)
--uniqueness=FILE
- Output a uniqueness data file for the reference; no Solexa reads needed; implies---noshortcuts` (optional)
--pileup=FILE
- Outputs complete pileup into that file (optional)
--cigar=FILE
- Outputs alignment in CIGAR format (optional)
--gffout=FILE
- Outputs reads in GFF format (optional)
--coverage=FILENAME
- Outputs (high depth) coverage data (optional)
--wobble=FILENAME
- Outputs a list of possible variations (optional; paired reads only) [UNDER CONSTRUCTION]
--fragmentplot=FILENAME
- Outputs a plot of fragment size distribution to a file (optional)
--snpsinreads=FILENAME
- Outputs a list of reads containing known SNPs to a file (optional)
--indelplot=FILENAME
- Outputs indel data to a file (optional)
--inversions=FILENAME
- For paired reads, writes read matches indicating inversions into a file (optional)
--faceaway=FILENAME
- For paired reads, writes read matches that "face away" from each other into a file (optional)
--sqlite=FILENAME
- Creates a sqlite text file with alignment data [EXPERIMENTAL] (optional)
--sam=FILENAME
- Creates a SAM alignment file (optional)
--spancontigs=FILENAME
- Outputs read pairs where "half" reads map uniquely to different contigs (optional)
--bins=FILE_PREFIX
- Outputs no-match, single-match and multi-match Solexa reads into prefixed files (optional)
--binmask=MASK
- Mask of 1s and 0s to turn off individual bins. Order: No match, single match, multi-match, IUPAC. Example: 0100 creates only single-match bin. (optional; default:1111)
--pair=NUMBER
- For paired reads, the length of the first part of the read (mandatory for paired reads)
--fragment=NUMBER
- For paired reads, the average fragment length (mandatory for paired reads)
--variance=NUMBER
- For paired reads, the variance of the fragment length to either side (optional; default: 1/4 of fragment size)
--wobblemax=NUMBER
- Maximum number of mismatches for wobble (optional; default 2; see --wobble)
--mspi=NUMBER
- Maximum number of SNPs per chromosomal index (optional; default:8)
--index=FILENAME
- Index filename (index will be created if it does not exist; optional)
--noshortcuts
- Will process all chrososomal regions, even those with lots'o'repeats (optional; no value)
--snpsonly
- Only lists found SNPs in the pileup (optional; no value)
--chromosome=NAME
- Discards all chromosomes but NAME prior to run (optional)
--index_from=NUMBER
- Starts indexing at this position on all chromosomes (optional)
--index_to=NUMBER
- Stops indexing at this position on all chromosomes (optional)
--chop=NUMBER
-
For paired reads, if one but not the other matches, shorten the other by NUMBER` bases (optional)
--index1=NUMBER`
- Length of internal index 1 (optional; default:10)
--index2=NUMBER
- Length of internal index 2 (optional; default:16)
--memory_save=NUMBER
- Indexes the genome every NUMBER of positions; saves memory and runtime, but can have strange side effects (optional)
--multimatch
- Puts a multiple-matching read to a random position (optional) [currently paired reads only]
--singlematch
- Only performs additional output functions for single matches (optional) [currently paired reads only]
--foum
- For paired reads, at least one read has to match uniquely in the genome (force one unique match) (optional)
--mismatch
- The number of mismatches allowed outside the index (index1+index2) (optional)
--rpa=FILENAME
- Writes all read pair alignments into a file (optional)