ANGSD: Analysis of next generation Sequencing Data

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Available from version 0.559+.
Available from version 0.559+.
 
<pre>
Newer githubversions will limit the output to the chrs with data. Earlier versions was printout 'N"
</pre>
This option creates a fasta.gz file from a sequencing data file (BAM file). The function uses genome information in the BAM header to determine the length and chromosome names. For the sites without data an "N" is written.  
This option creates a fasta.gz file from a sequencing data file (BAM file). The function uses genome information in the BAM header to determine the length and chromosome names. For the sites without data an "N" is written.  



Revision as of 09:59, 2 November 2014

Available from version 0.559+.

Newer githubversions will limit the output to the chrs with data. Earlier versions was printout 'N"

This option creates a fasta.gz file from a sequencing data file (BAM file). The function uses genome information in the BAM header to determine the length and chromosome names. For the sites without data an "N" is written.

<classdiagram type="dir:LR">

[Single BAM file{bg:orange}]->[Sequence data|Random base (-doFasta 1);Consensus base (-doFasta 2);Highest EBD (-doFasta 3)]

[sequence data]->doFasta[fasta file{bg:blue}]

</classdiagram>

This can be used as input for the ANGSD analysis:

  1. Error estimation
  2. ABBA-BABA


Brief Overview

> ./angsd -doFasta
--------------
analysisFasta.cpp:
	-doFasta	0
	1: use a random base
	2: use the most common base (needs -doCounts 1)
	3: use the base with highest ebd (under development) 
	-minQ		13	(remove bases with qscore<minQ)
	-basesPerLine	50	(Number of bases perline in output file)

This function will dump a fasta file, the full header information from the SAM/BAM file will be used. This means that a fasta will be generated for ALL entries in the header even if '-r/-rf -sites' is used.

The EBD is the effective base depth, as defined by [1]:


For four bases we have 4 different EBD, each EBD is the product of the mapping quality and scores for the base under consideration.

Options

-doFasta 1
sample a random base at each position.
-doFasta 2
use the most common base. In the case of ties a random base is chosen among the bases with the same maximum counts. The "-doCounts 1" options for allele counts is needed in order to determine the most common base.

For filters see Filters

Output

Output is a fasta file, a normal looking fast file. Nothing special about this. For -doFasta 1, sometimes its big letters sometime small letters. This is due to the results being copied directly from the sequencing data. So small/big letters correspond to which strand for the original data. For the consensus fasta all letters are capital letters.

Example

Create a fasta file bases from a random samples of bases.

./angsd -i bams/smallNA07056.mapped.ILLUMINA.bwa.CEU.low_coverage.20111114.bam -doFasta 1