DOKK / manpages / debian 10 / tracetuner / ttuner.1.en
TTUNER(1) User Commands TTUNER(1)

ttuner - interpretation of DNA Sanger sequencing data

(Help) This message
(Quiet) Turn off status messages
(Verbose) Output more status messages
Disable base recalling and just use the original called bases read from the input sample file
Disable adding bases to or deleting from the original called sequence. Only recall Ns
Call call hetezygotes
Call mixed bases
Override the default threshold ratio of heights of
Set the trimming window size for averaging quality to the specified value. The default is 10.

-trim_threshold <qv> Set the average quality value used in trimming to

Specify the name of the FASTA file which contains the consensus sequence
Start base recalling from the ABI's edited bases
Use specified lookup table. This option overrides the default (automatic choice of the lookup table) as well as the options -3700pop5, -3700pop6, -3100, and -mbace. To get a message showing which table was used, specify -V option
-3730
Use the built-in ABI 3730-pop7 lookup table
-3700pop5
Use the built-in ABI 3700-pop5 lookup table
-3700pop6
Use the built-in ABI 3700-pop6 lookup table
-3100
Use the built-in ABI 3100-pop6 lookup table
Use the built-in MegaBACE lookup table
Output SCF file(s), in the current directory
Output SCF file(s), in the specified directory
Use version 3 for output SCF file. Default is version 2.
Output multi-fasta files of bases (tt.seq), their locations (tt.pos), quality values (tt.qual) and status reports (tt.status) to directory <dir>
Output .phd.1 file(s), in the current directory
Output .phd.1 file(s), in the specified directory
Output .qual file(s), in the current directory
Append .qual file(s) to <file>
Output .qual file(s), in the specified directory
Output .seq file(s) in FASTA format, in the current directory
Append .seq file(s) in FASTA format to <file>
Output .seq file(s) in FASTA format, in the specified directory
Output a quality report that gives data for a histogram on the number of reads with quality values >= 20, to the specified file
Read the input sample filenames from the specified file
Read the input sample files from specified directory
Call heterozygotes or mixed bases and output .tab file(s) in the current directory
Call mixed bases and output .tab file(s), in the specified directory
Output .tal file(s),in the current directory
Output .tal file(s),in the specified directory
Output a homopolymer runs file in current directory
Output a homopolymer runs file(s),in the specified directory
Output .poly file(s),in the current directory
<dir> Output .poly file(s),in the specified directory
Input the original bases and peak locations from a .phd file in the specified directory.

This manpage was written by Andreas Tille for the Debian distribution and can be used for any other usage of the program.

October 2018 ttuner 3.0.6~beta