samtools(1)                  Bioinformatics tools                  samtools(1)



NAME
       samtools - Utilities for the Sequence Alignment/Map (SAM) format

SYNOPSIS
       samtools view -bt ref_list.txt -o aln.bam aln.sam.gz

       samtools sort aln.bam aln.sorted

       samtools index aln.sorted.bam

       samtools idxstats aln.sorted.bam

       samtools view aln.sorted.bam chr2:20,100,000-20,200,000

       samtools merge out.bam in1.bam in2.bam in3.bam

       samtools faidx ref.fasta

       samtools pileup -vcf ref.fasta aln.sorted.bam

       samtools mpileup -C50 -gf ref.fasta -r chr3:1,000-2,000 in1.bam in2.bam

       samtools tview aln.sorted.bam ref.fasta


DESCRIPTION
       Samtools is a set of utilities that manipulate alignments  in  the  BAM
       format. It imports from and exports to the SAM (Sequence Alignment/Map)
       format, does sorting, merging and  indexing,  and  allows  to  retrieve
       reads in any regions swiftly.

       Samtools  is designed to work on a stream. It regards an input file `-'
       as the standard input (stdin) and an output file `-'  as  the  standard
       output (stdout). Several commands can thus be combined with Unix pipes.
       Samtools always output warning and error messages to the standard error
       output (stderr).

       Samtools  is  also able to open a BAM (not SAM) file on a remote FTP or
       HTTP server if the BAM file name starts  with  `ftp://'  or  `http://'.
       Samtools  checks  the  current working directory for the index file and
       will download the index upon absence. Samtools does  not  retrieve  the
       entire alignment file unless it is asked to do so.


COMMANDS AND OPTIONS
       view      samtools  view  [-bchuHS]  [-t  in.refList]  [-o  output] [-f
                 reqFlag] [-F skipFlag] [-q minMapQ] [-l  library]  [-r  read-
                 Group] [-R rgFile] <in.bam>|<in.sam> [region1 [...]]

                 Extract/print  all or sub alignments in SAM or BAM format. If
                 no region is specified, all the alignments will  be  printed;
                 otherwise  only  alignments overlapping the specified regions
                 will be output. An alignment may be given multiple  times  if
                 it is overlapping several regions. A region can be presented,
                 for example, in  the  following  format:  `chr2'  (the  whole
                 chr2),  `chr2:1000000'  (region starting from 1,000,000bp) or
                 `chr2:1,000,000-2,000,000'  (region  between  1,000,000   and
                 2,000,000bp  including  the  end  points).  The coordinate is
                 1-based.

                 OPTIONS:

                 -b      Output in the BAM format.

                 -f INT  Only output alignments with all bits in  INT  present
                         in the FLAG field. INT can be in hex in the format of
                         /^0x[0-9A-F]+/ [0]

                 -F INT  Skip alignments with bits present in INT [0]

                 -h      Include the header in the output.

                 -H      Output the header only.

                 -l STR  Only output reads in library STR [null]

                 -o FILE Output file [stdout]

                 -q INT  Skip alignments with MAPQ smaller than INT [0]

                 -r STR  Only output reads in read group STR [null]

                 -R FILE Output reads in read groups listed in FILE [null]

                 -S      Input is in SAM. If @SQ header lines are absent,  the
                         `-t' option is required.

                 -c      Instead  of  printing the alignments, only count them
                         and print the total number. All filter options,  such
                         as `-f', `-F' and `-q' , are taken into account.

                 -t FILE This  file  is  TAB-delimited. Each line must contain
                         the reference name and the length of  the  reference,
                         one  line  for  each  distinct  reference; additional
                         fields are ignored. This file also defines the  order
                         of  the  reference  sequences  in sorting. If you run
                         `samtools faidx <ref.fa>', the resultant  index  file
                         <ref.fa>.fai  can be used as this <in.ref_list> file.

                 -u      Output uncompressed BAM. This option saves time spent
                         on  compression/decomprssion  and  is  thus preferred
                         when the output is piped to another samtools command.


       tview     samtools tview <in.sorted.bam> [ref.fasta]

                 Text  alignment viewer (based on the ncurses library). In the
                 viewer, press `?' for help and press `g' to check the  align-
                 ment    start    from   a   region   in   the   format   like
                 `chr10:10,000,000' or `=10,000,000'  when  viewing  the  same
                 reference sequence.


       mpileup   samtools mpileup [-Bug] [-C capQcoef] [-r reg] [-f in.fa] [-l
                 list] [-M capMapQ] [-Q minBaseQ] [-q minMapQ] in.bam [in2.bam
                 [...]]

                 Generate  BCF or pileup for one or multiple BAM files. Align-
                 ment records are grouped by sample identifiers in @RG  header
                 lines.  If  sample identifiers are absent, each input file is
                 regarded as one sample.

                 OPTIONS:

                 -B      Disable probabilistic realignment for the computation
                         of  base  alignment  quality (BAQ). BAQ is the Phred-
                         scaled probability of a read base  being  misaligned.
                         Applying  this  option  greatly helps to reduce false
                         SNPs caused by misalignments.

                 -C INT  Coefficient for downgrading mapping quality for reads
                         containing  excessive mismatches. Given a read with a
                         phred-scaled probability q of  being  generated  from
                         the mapped position, the new mapping quality is about
                         sqrt((INT-q)/INT)*INT. A  zero  value  disables  this
                         functionality;  if enabled, the recommended value for
                         BWA is 50. [0]

                 -e INT  Phred-scaled gap extension sequencing error probabil-
                         ity. Reducing INT leads to longer indels. [20]

                 -f FILE The reference file [null]

                 -g      Compute  genotype  likelihoods and output them in the
                         binary call format (BCF).

                 -h INT  Coefficient for modeling homopolymer errors. Given an
                         l-long  homopolymer  run,  the sequencing error of an
                         indel of size s is modeled as INT*s/l.  [100]

                 -l FILE File containing a list of sites where pileup  or  BCF
                         is outputted [null]

                 -o INT  Phred-scaled  gap  open sequencing error probability.
                         Reducing INT leads to more indel calls. [40]

                 -P STR  Comma dilimited list of platforms (determined by @RG-
                         PL)  from  which indel candidates are obtained. It is
                         recommended to collect indel candidates from sequenc-
                         ing  technologies that have low indel error rate such
                         as ILLUMINA. [all]

                 -q INT  Minimum mapping quality for an alignment to  be  used
                         [0]

                 -Q INT  Minimum base quality for a base to be considered [13]

                 -r STR  Only generate pileup in region STR [all sites]

                 -u      Similar to -g except that the output is  uncompressed
                         BCF, which is preferred for piping.


       reheader  samtools reheader <in.header.sam> <in.bam>

                 Replace   the   header   in   in.bam   with   the  header  in
                 in.header.sam.  This command is much  faster  than  replacing
                 the header with a BAM->SAM->BAM conversion.


       sort      samtools sort [-no] [-m maxMem] <in.bam> <out.prefix>

                 Sort  alignments  by  leftmost  coordinates.  File  <out.pre-
                 fix>.bam will be created. This command may also create tempo-
                 rary  files <out.prefix>.%d.bam when the whole alignment can-
                 not be fitted into memory (controlled by option -m).

                 OPTIONS:

                 -o      Output the final alignment to the standard output.

                 -n      Sort by read names rather than by chromosomal coordi-
                         nates

                 -m INT  Approximately    the    maximum    required   memory.
                         [500000000]


       merge     samtools  merge  [-nur]  [-h  inh.sam]  [-R  reg]   <out.bam>
                 <in1.bam> <in2.bam> [...]

                 Merge multiple sorted alignments.  The header reference lists
                 of all the input BAM files, and the @SQ headers  of  inh.sam,
                 if  any,  must  all  refer  to  the  same  set  of  reference
                 sequences.  The header reference list and (unless  overridden
                 by  -h) `@' headers of in1.bam will be copied to out.bam, and
                 the headers of other files will be ignored.

                 OPTIONS:

                 -h FILE Use the lines of FILE as `@' headers to be copied  to
                         out.bam, replacing any header lines that would other-
                         wise be copied from in1.bam.  (FILE  is  actually  in
                         SAM  format, though any alignment records it may con-
                         tain are ignored.)

                 -R STR  Merge files in the specified region indicated by STR

                 -r      Attach an RG tag to each alignment. The tag value  is
                         inferred from file names.

                 -n      The  input alignments are sorted by read names rather
                         than by chromosomal coordinates

                 -u      Uncompressed BAM output


       index     samtools index <aln.bam>

                 Index sorted alignment for fast  random  access.  Index  file
                 <aln.bam>.bai will be created.


       idxstats  samtools idxstats <aln.bam>

                 Retrieve and print stats in the index file. The output is TAB
                 delimited with each line  consisting  of  reference  sequence
                 name, sequence length, # mapped reads and # unmapped reads.


       faidx     samtools faidx <ref.fasta> [region1 [...]]

                 Index  reference sequence in the FASTA format or extract sub-
                 sequence from indexed reference sequence.  If  no  region  is
                 specified,   faidx   will   index   the   file   and   create
                 <ref.fasta>.fai on the disk. If regions are speficified,  the
                 subsequences  will  be retrieved and printed to stdout in the
                 FASTA format. The input file can be compressed  in  the  RAZF
                 format.


       fixmate   samtools fixmate <in.nameSrt.bam> <out.bam>

                 Fill in mate coordinates, ISIZE and mate related flags from a
                 name-sorted alignment.


       rmdup     samtools rmdup [-sS] <input.srt.bam> <out.bam>

                 Remove potential PCR duplicates: if multiple read pairs  have
                 identical  external  coordinates,  only  retain the pair with
                 highest mapping quality.  In the paired-end mode,  this  com-
                 mand  ONLY  works  with  FR orientation and requires ISIZE is
                 correctly set. It does not work for unpaired reads (e.g.  two
                 ends mapped to different chromosomes or orphan reads).

                 OPTIONS:

                 -s      Remove  duplicate  for  single-end reads. By default,
                         the command works for paired-end reads only.

                 -S      Treat paired-end reads and single-end reads.


       calmd     samtools calmd [-eubSr] [-C capQcoef] <aln.bam> <ref.fasta>

                 Generate the MD tag. If the MD tag is already  present,  this
                 command  will  give a warning if the MD tag generated is dif-
                 ferent from the existing tag. Output SAM by default.

                 OPTIONS:

                 -A      When used jointly with -r this option overwrites  the
                         original base quality.

                 -e      Convert  a  the  read base to = if it is identical to
                         the aligned reference base.  Indel  caller  does  not
                         support the = bases at the moment.

                 -u      Output uncompressed BAM

                 -b      Output compressed BAM

                 -S      The input is SAM with header lines

                 -C INT  Coefficient  to  cap mapping quality of poorly mapped
                         reads. See the pileup command for details. [0]

                 -r      Compute the BQ tag without changing the base quality.


       pileup    samtools pileup [-2sSBicv] [-f in.ref.fasta] [-t in.ref_list]
                 [-l in.site_list] [-C capMapQ] [-M maxMapQ]  [-T  theta]  [-N
                 nHap]  [-r  pairDiffRate]  [-m  mask]  [-d maxIndelDepth] [-G
                 indelPrior] <in.bam>|<in.sam>

                 Print the alignment in the pileup format. In the pileup  for-
                 mat,  each  line represents a genomic position, consisting of
                 chromosome name, coordinate, reference base, read bases, read
                 qualities  and  alignment  mapping  qualities. Information on
                 match, mismatch, indel, strand, mapping quality and start and
                 end  of  a  read  are all encoded at the read base column. At
                 this column, a dot stands for a match to the  reference  base
                 on  the  forward  strand,  a comma for a match on the reverse
                 strand, a '>' or '<' for a reference skip, `ACGTN' for a mis-
                 match on the forward strand and `acgtn' for a mismatch on the
                 reverse strand. A pattern  `\+[0-9]+[ACGTNacgtn]+'  indicates
                 there is an insertion between this reference position and the
                 next reference position. The length of the insertion is given
                 by  the  integer  in  the  pattern,  followed by the inserted
                 sequence. Similarly, a pattern `-[0-9]+[ACGTNacgtn]+'  repre-
                 sents  a  deletion from the reference. The deleted bases will
                 be presented as `*' in the following lines. Also at the  read
                 base  column,  a  symbol  `^'  marks the start of a read. The
                 ASCII of the character following `^' minus 33 gives the  map-
                 ping quality. A symbol `$' marks the end of a read segment.

                 If  option  -c  is  applied, the consensus base, Phred-scaled
                 consensus quality, SNP quality (i.e. the Phred-scaled  proba-
                 bility of the consensus being identical to the reference) and
                 root mean square (RMS) mapping quality of the reads  covering
                 the  site  will  be inserted between the `reference base' and
                 the `read bases' columns. An  indel  occupies  an  additional
                 line.  Each  indel  line consists of chromosome name, coordi-
                 nate, a star, the genotype, consensus quality,  SNP  quality,
                 RMS mapping quality, # covering reads, the first alllele, the
                 second allele, # reads supporting the first allele,  #  reads
                 supporting  the  second  allele and # reads containing indels
                 different from the top two alleles.

                 NOTE: Since 0.1.10, the `pileup'  command  is  deprecated  by
                 `mpileup'.

                 OPTIONS:

                 -B        Disable  the  BAQ computation. See the mpileup com-
                           mand for details.

                 -c        Call the consensus sequence. Options -T, -N, -I and
                           -r are only effective when -c or -g is in use.

                 -C INT    Coefficient  for downgrading the mapping quality of
                           poorly mapped reads. See the  mpileup  command  for
                           details. [0]

                 -d INT    Use  the  first  NUM  reads in the pileup for indel
                           calling for speed up. Zero for unlimited. [1024]

                 -f FILE   The reference sequence in the FASTA  format.  Index
                           file FILE.fai will be created if absent.

                 -g        Generate  genotype  likelihood  in the binary GLFv3
                           format. This option suppresses -c, -i and -s.  This
                           option is deprecated by the mpileup command.

                 -i        Only output pileup lines containing indels.

                 -I INT    Phred  probability  of an indel in sequencing/prep.
                           [40]

                 -l FILE   List of sites at which pileup is output. This  file
                           is  space  delimited.  The  first  two  columns are
                           required to be chromosome and  1-based  coordinate.
                           Additional  columns  are ignored. It is recommended
                           to use option

                 -m INT    Filter reads  with  flag  containing  bits  in  INT
                           [1796]

                 -M INT    Cap mapping quality at INT [60]

                 -N INT    Number of haplotypes in the sample (>=2) [2]

                 -r FLOAT  Expected  fraction of differences between a pair of
                           haplotypes [0.001]

                 -s        Print the mapping quality as the last column.  This
                           option  makes  the output easier to parse, although
                           this format is not space efficient.

                 -S        The input file is in SAM.

                 -t FILE   List of reference names ane  sequence  lengths,  in
                           the  format  described  for  the import command. If
                           this option is present, samtools assumes the  input
                           <in.alignment>  is  in  SAM  format;  otherwise  it
                           assumes in BAM format.  -s together with -l  as  in
                           the  default  format  we  may  not know the mapping
                           quality.

                 -T FLOAT  The theta parameter (error dependency  coefficient)
                           in the maq consensus calling model [0.85]


SAM FORMAT
       SAM  is  TAB-delimited.  Apart from the header lines, which are started
       with the `@' symbol, each alignment line consists of:


       +----+-------+----------------------------------------------------------+
       |Col | Field |                       Description                        |
       +----+-------+----------------------------------------------------------+
       | 1  | QNAME | Query (pair) NAME                                        |
       | 2  | FLAG  | bitwise FLAG                                             |
       | 3  | RNAME | Reference sequence NAME                                  |
       | 4  | POS   | 1-based leftmost POSition/coordinate of clipped sequence |
       | 5  | MAPQ  | MAPping Quality (Phred-scaled)                           |
       | 6  | CIAGR | extended CIGAR string                                    |
       | 7  | MRNM  | Mate Reference sequence NaMe (`=' if same as RNAME)      |
       | 8  | MPOS  | 1-based Mate POSistion                                   |
       | 9  | ISIZE | Inferred insert SIZE                                     |
       |10  | SEQ   | query SEQuence on the same strand as the reference       |
       |11  | QUAL  | query QUALity (ASCII-33 gives the Phred base quality)    |
       |12  | OPT   | variable OPTional fields in the format TAG:VTYPE:VALUE   |
       +----+-------+----------------------------------------------------------+

       Each bit in the FLAG field is defined as:


          +-------+-----+--------------------------------------------------+
          | Flag  | Chr |                   Description                    |
          +-------+-----+--------------------------------------------------+
          |0x0001 |  p  | the read is paired in sequencing                 |
          |0x0002 |  P  | the read is mapped in a proper pair              |
          |0x0004 |  u  | the query sequence itself is unmapped            |
          |0x0008 |  U  | the mate is unmapped                             |
          |0x0010 |  r  | strand of the query (1 for reverse)              |
          |0x0020 |  R  | strand of the mate                               |
          |0x0040 |  1  | the read is the first read in a pair             |
          |0x0080 |  2  | the read is the second read in a pair            |
          |0x0100 |  s  | the alignment is not primary                     |
          |0x0200 |  f  | the read fails platform/vendor quality checks    |
          |0x0400 |  d  | the read is either a PCR or an optical duplicate |
          +-------+-----+--------------------------------------------------+

EXAMPLES
       o Import SAM to BAM when @SQ lines are present in the header:

           samtools view -bS aln.sam > aln.bam

         If @SQ lines are absent:

           samtools faidx ref.fa
           samtools view -bt ref.fa.fai aln.sam > aln.bam

         where ref.fa.fai is generated automatically by the faidx command.


       o Attach the RG tag while merging sorted alignments:

           perl      -e       'print       "@RG\tID:ga\tSM:hs\tLB:ga\tPL:Illu-
         mina\n@RG\tID:454\tSM:hs\tLB:454\tPL:454\n"' > rg.txt
           samtools merge -rh rg.txt merged.bam ga.bam 454.bam

         The value in a RG tag is determined by the file name the read is com-
         ing from. In this example, in the merged.bam, reads from ga.bam  will
         be  attached  RG:Z:ga,  while  reads  from  454.bam  will be attached
         RG:Z:454.


       o Call SNPs and short indels for one diploid individual:

           samtools mpileup -ugf ref.fa aln.bam |  bcftools  view  -bvcg  -  >
         var.raw.bcf
           bcftools   view  var.raw.bcf  |  vcfutils.pl  varFilter  -D  100  >
         var.flt.vcf

         The -D option of varFilter controls the  maximum  read  depth,  which
         should  be  adjusted  to about twice the average read depth.  One may
         consider to add -C50 to mpileup if mapping quality  is  overestimated
         for  reads containing excessive mismatches. Applying this option usu-
         ally helps BWA-short but may not other mappers.


       o Call SNPs and short indels for multiple diploid individuals:

           samtools mpileup -P ILLUMINA -ugf  ref.fa  *.bam  |  bcftools  view
         -bcvg - > var.raw.bcf
           bcftools  view  var.raw.bcf  |  vcfutils.pl  varFilter  -D  2000  >
         var.flt.vcf

         Individuals are identified from the SM tags in the @RG header  lines.
         Individuals  can  be pooled in one alignment file; one individual can
         also be separated into multiple files. The -P option  specifies  that
         indel  candidates  should be collected only from read groups with the
         @RG-PL tag set to ILLUMINA.  Collecting indel candidates  from  reads
         sequenced  by an indel-prone technology may affect the performance of
         indel calling.


       o Derive the allele frequency spectrum (AFS) on a list  of  sites  from
         multiple individuals:

           samtools mpileup -Igf ref.fa *.bam > all.bcf
           bcftools view -bl sites.list all.bcf > sites.bcf
           bcftools view -cGP cond2 sites.bcf > /dev/null 2> sites.1.afs
           bcftools view -cGP sites.1.afs sites.bcf > /dev/null 2> sites.2.afs
           bcftools view -cGP sites.2.afs sites.bcf > /dev/null 2> sites.3.afs
           ......

         where sites.list contains the list of sites with each line consisting
         of the reference sequence name and position. The  following  bcftools
         commands estimate AFS by EM.


       o Dump BAQ applied alignment for other SNP callers:

           samtools calmd -bAr aln.bam > aln.baq.bam

         It  adds  and corrects the NM and MD tags at the same time. The calmd
         command also comes with the -C option, the same as the one in  pileup
         and mpileup.  Apply if it helps.


LIMITATIONS
       o Unaligned   words  used  in  bam_import.c,  bam_endian.h,  bam.c  and
         bam_aux.c.

       o In merging, the input files are required to have the same  number  of
         reference  sequences.  The  requirement  can be relaxed. In addition,
         merging does not reconstruct the header  dictionaries  automatically.
         Endusers  have  to  provide  the  correct header. Picard is better at
         merging.

       o Samtools paired-end rmdup does not  work  for  unpaired  reads  (e.g.
         orphan  reads  or ends mapped to different chromosomes). If this is a
         concern, please use Picard's MarkDuplicate  which  correctly  handles
         these cases, although a little slower.


AUTHOR
       Heng  Li from the Sanger Institute wrote the C version of samtools. Bob
       Handsaker from the Broad Institute implemented the BGZF library and Jue
       Ruan  from Beijing Genomics Institute wrote the RAZF library. John Mar-
       shall and Petr Danecek contribute to the source code and various people
       from the 1000 Genomes Project have contributed to the SAM format speci-
       fication.


SEE ALSO
       Samtools website: <http://samtools.sourceforge.net>



samtools-0.1.10                15 November 2010                    samtools(1)
