TFASTX
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Table of Contents
FUNCTION
DESCRIPTION
EXAMPLE
OUTPUT
INPUT
FILES
RELATED
PROGRAMS
RESTRICTIONS
ALGORITHM
CONSIDERATIONS
SUGGESTIONS
COMMAND-LINE
SUMMARY
LOCAL
DATA FILES
PARAMETER
REFERENCE
FUNCTION
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TFastX does a Pearson and Lipman search for
similarity between a protein query sequence and any group of nucleotide
sequences, taking frameshifts into account. It is designed to be a replacement
for TFastA, and like TFastA, it is designed to answer
the question, "What implied protein sequences in a nucleotide sequence
database are similar to my protein sequence?"
DESCRIPTION
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TFastX uses the method of Pearson and Lipman
(Proc. Natl. Acad. Sci. USA 85; 2444-2448 (1988)) to search
for similarities between a query protein sequence and any group of nucleotide
sequences.
TFastX can be considered to be an enhanced
version of TFastA. TFastA
treats each of the six reading frames of a nucleotide sequence as a separate
sequence, resulting in three separate alignments for each strand. TFastX, on
the other hand, compares the protein query sequence to only one translated
protein per strand of the nucleotide sequence, resulting in one alignment per
strand. It calculates a similarity score for alignments that takes frameshifts
into account, allowing it to "join" short regions separated by
frameshifts into a single long alignment. TFastX may alert you to more
meaningful hits than TFastA does when the nucleotide
sequences contain frameshift errors.
TFastX can also be used in situations where FrameSearch is used. TFastX is faster, but FrameSearch is more sensitive.
In the first step of this search, the comparison
can be viewed as a set of dot plots, with the query as the vertical sequence
and the group of sequences to which the query is being compared as the
different horizontal sequences. This first step finds the registers of
comparison (diagonals) having the largest number of short perfect
matches (words) for each comparison. In the second step, these
"best" regions are rescored using a scoring matrix that allows
conservative replacements, ambiguity symbols, and runs of identities shorter
than the size of a word. In the third step, the program checks to see if some
of these initial highest-scoring diagonals can be joined together. Finally, the
search set sequences with the highest scores are aligned to the query sequence
for display.
What is a Word?
A word is any short sequence (n-mer or k-tuple)
where you have set n to some small integer less than or equal to six. The word
GGATGG is one of the 4,096 possible words of length six that can be created
from an alphabet consisting of the four letters G, A, T, and C. The word QL is
one of the 400 possible words of length two that you can make with the 20
letters of the amino acid alphabet.
EXAMPLE
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Here is a session using TFastX to identify
sequences in a collection of nucleotide sequences that may contain translated
regions similar to a human globin protein:
% tfastx
TFASTX with what query sequence ? ggamma.pep
Removing terminal * from query sequence...
Begin (* 1 *) ?
End (* 147 *) ?
Search for query in what sequence(s) (* GenBank:* *) ? fragments.rsf{*}
What word size (* 2 *) ?
Don't show scores whose E() value exceeds: (* 10.0 *):
What should I call the output file (* ggamma.tfastx *) ?
1 Sequences 400 nt searched Fragments.Rsf{Aa004794}
/////////////////////////////////////////////////////////////
CPU time used:
Database scan: 0:00: 0.6
Post-scan processing: 0:00: 1.4
Total CPU time: 0:00: 2.1
Output file: ggamma.tfastx
%
OUTPUT
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The
output from TFastX is a list file, and is suitable for input to any GCG program
that allows indirect file specifications. (For information about indirect file
specification, see Section 2, Using Sequence Files and Databases of the User's
Guide.)
Here
is some of the output file:
!!SEQUENCE_LIST 1.0
(Peptide) TFASTX of: ggamma.pep from: 1 to: 147 October 14, 1998 13:11
TRANSLATE of: gamma.seq check: 6474 from: 2179 to: 2270
and of: gamma.seq check: 6474 from: 2393 to: 2615
and of: gamma.seq check: 6474 from: 3502 to: 3630
generated symbols 1 to: 148.
Human fetal beta globins G and A gamma
from Shen, Slightom and Smithies, Cell 26; 191-203. . . .
TO: FRAGMENTS.RSF{*} Sequences: 31 Symbols: 12,095 Word Size: 2
Searching both strands.
Scoring matrix: GenRunData:Blosum50.Cmp
Variable pamfactor used
Gap creation penalty: 15 Gap extension penalty: 2 Frameshift penalty: 20
Histogram Key:
Each histogram symbol represents 1 search set sequences
z-scores computed from opt scores
z-score obs exp
(=) (*)
< 20 0 0:
22 0 0:
24 0 0:
26 0 0:
28 0 0:
30 0 0:
32 0 0:
34 0 0:
36 0 1:*
38 0 2: *
40 0 2: *
42 10 3:==*=======
44 6 3:==*===
46 3 3:==*
48 1 3:= *
50 1 3:= *
52 1 2:=*
54 2 2:=*
56 2 2:=*
58 1 1:*
60 0 1:*
62 0 1:*
64 0 1:*
66 1 1:*
68 0 0:
70 1 0:=
72 1 0:=
74 0 0:
76 0 0:
78 1 0:=
80 0 0:
82 0 0:
84 0 0:
86 0 0:
88 0 0:
90 0 0:
92 0 0:
94 0 0:
96 0 0:
98 0 0:
100 0 0:
102 0 0:
104 0 0:
106 0 0:
108 0 0:
110 0 0:
112 0 0:
114 0 0:
116 0 0:
118 0 0:
>120 0 0:
Joining threshold: 36, opt. threshold: 24, opt. width: 16, reg.-scaled
The best scores are: strand init1 initn opt z-sc E(31)..
FRAGMENTS.RSF{AA096098}! SAMPLE of: l7628.seq.F Fetal heart,...(f) 681 761 763 78.7 0.43
FRAGMENTS.RSF{AA038757}! SAMPLE of: mi94d08.r1 Soares mouse ...(f) 574 596 625 71.8 1
FRAGMENTS.RSF{AA063750}! SAMPLE of: mj79g09.r1 Soares mouse ...(f) 337 540 580 69.6 1.4
/////////////////////////////////////////////////////////////////////////////
\\End of List
ggamma.pep
FRAGMENTS.RSF{AA096098}
Description: SAMPLE of: l7628.seq.F Fetal heart, Lambda ZAP Express
Accession/ID:
SCORES Strand:(f) Init1: 681 Initn: 761 Opt: 763 z-score: 78.7 E(): 0.43
Smith-Waterman score: 763; 93.0% identity in 129 aa overlap
10 20 30 40 50 60
ggamma.pep MGHFTEEDKATITSLWGKVNVEDAGGETLGRLLVVYPWTQRFFDSFGNLSSASAIMGNPK
|||||||||||||||||||||||||||| |||||||||||||||||||||||||||||||
FRAGMENTS.RS MGHFTEEDKATITSLWGKVNVEDAGGETPGRLLVVYPWTQRFFDSFGNLSSASAIMGNPK
20 30 40 50 60 70
70 80 90 100 110 119
ggamma.pep VKAHGKKVLTSLGDAIKHLDDLKGTFAQLSELHCDKLHVDPEN-FKLLGNVLVTVLAIHF
||||||||||||||||||||||||||||||||||||||||||| :|||||||| ||||||
FRAGMENTS.RS VKAHGKKVLTSLGDAIKHLDDLKGTFAQLSELHCDKLHVDPEN/LKLLGNVLVPVLAIHF
80 90 100 110 120 130
120
ggamma.pep GKEFTPEVQ
||: | |:
FRAGMENTS.RS GKDS-PXVR
140
/////////////////////////////////////////////////////////////////////////
! Distributed over 1 thread.
! Start time: Wed Oct 14 13:11:29 1998
! Completion time: Wed Oct 14 13:11:44 1998
! CPU time used:
! Database scan: 0:00:00.6
! Post-scan processing: 0:00:01.4
! Total CPU time: 0:00:02.1
! Output File: ggamma.tfastx
What
is the Output?
The
first part of the output file contains a histogram showing the distribution of
the z-scores between the query and search set sequences. (See the
ALGORITHM topic for an explanation of z-score.) The histogram is
composed of bins of size 2 that are labeled according to the higher score for
that bin (the leftmost column of the histogram). For example, the bin labeled
24 stores the number of sequence pairs that had scores of 23 or 24.
The
next two columns of the histogram list the number of z-scores that
fell within each bin. The second column lists the number of z-scores
observed in the search and the third column lists the number of z-scores
that were expected.
The
body of the histogram displays a graphical representation of the score
distributions. Equal signs (=) indicate the number of scores of that magnitude
that were observed during the search, while asterisks (*) plot the number of
scores of that magnitude that were expected.
At
the bottom of the histogram is a list of some of the parameters pertaining to
the search.
Below
the histogram, TFastX displays a listing of the best scores. This listing
includes the strand (f or r) of the original nucleotide sequence from which the
reported translated sequence is derived.
Following
the list of best scores, TFastX displays the alignments of the regions of best
overlap between the query and search sequences. In these alignments, stop
codons are represented by the letter X.
This
program displays only the region of overlap between the two aligned sequences
(plus some residues on either side of the region to provide context for the
alignment) unless you use -SHOWall.
The display of identities and conservative replacements between the aligned
sequences depends on the value of -MARKx. By default ( -MARKx=3),
the pipe character (|) is used to denote identities and the colon (:) to denote
conservative replacements.
INPUT
FILES
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TFastX
accepts a single protein sequence as the query sequence. The search set is
either a single nucleic acid sequence or multiple nucleic acid sequences. You
can specify multiple sequences in a number of ways: by using a list file, for
example @project.list; by
using an MSF or RSF file, for example
project.msf{*}; or by using a sequence specification with an
asterisk (*) wildcard, for
example GenBank:*. If TFastX
rejects your protein sequence, turn to Appendix VI
to see how to change or set the type of a sequence.
RELATED PROGRAMS
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TFastX+ does a Pearson and Lipman search for similarity
between a protein query sequence and any group of nucleotide sequences, taking
frameshifts into account. It is designed to be a replacement for TFastA+, and
like TFastA+, it is designed to answer the question,
"What implied protein sequences in a nucleotide sequence database are
similar to my protein sequence?"
FastA does a Pearson and Lipman search for similarity
between a query sequence and a group of sequences of the same type (nucleic
acid or protein). For nucleotide searches, FastA may
be more sensitive than BLAST.
BLAST searches one or more nucleic acid or protein
databases for sequences similar to one or more query sequences of any type. BLAST can produce gapped alignments for the matches it
finds. NetBLAST searches for sequences similar to a query sequence. The query
and the database searched can be either peptide or nucleic acid in any
combination. NetBLAST can search only databases
maintained at the National Center
for Biotechnology Information (NCBI) in Bethesda,
Maryland, USA.
SSearch does a rigorous Smith-Waterman search for
similarity between a query sequence and a group of sequences of the same type
(nucleic acid or protein). This may be the most sensitive method available for
similarity searches. Compared to BLAST and FastA, it can be very slow.
TFastA does a Pearson and Lipman search for similarity
between a protein query sequence and any group of nucleotide sequences. TFastA translates the nucleotide sequences in all six
reading frames before performing the comparison. It is designed to answer the
question, "What implied protein sequences in a nucleotide sequence database
are similar to my protein sequence?"
FastX does a Pearson and Lipman search for similarity
between a nucleotide query sequence and a group of protein sequences, taking
frameshifts into account. FastX translates both
strands of the nucleic sequence before performing the comparison. It is
designed to answer the question, "What implied protein sequences in my
nucleic acid sequence are similar to sequences in a protein database?"
FrameSearch searches a group of protein sequences
for similarity to one or more nucleotide query sequences, or searches a group
of nucleotide sequences for similarity to one or more protein query sequences.
For each sequence comparison, the program finds an optimal alignment between
the protein sequence and all possible codons on each strand of the nucleotide
sequence. Optimal alignments may include reading frame shifts.
WordSearch identifies sequences in the database that
share large numbers of common words in the same register of comparison with
your query sequence. The output of WordSearch can
be displayed with Segments.
ProfileSearch and MotifSearch
use a profile (derived from a set of aligned sequences) instead of a
query sequence to search a collection of sequences. FindPatterns
uses a pattern described by a regular expression to search a
collection of sequences.
StringSearch, LookUp,
and Names identify sequences by searching the annotation (non-sequence)
portions of seqence files or sequence databases.
FastA+ does a Pearson and Lipman search for similarity
between a query sequence and a group of sequences of the same type (nucleic
acid or protein). For nucleotide searches, FastA+ may be more sensitive than
BLAST+.
BLAST+ searches one or more nucleic acid or protein
databases for sequences similar to one or more query sequences of any type.
BLAST+ can produce gapped alignments for the matches it finds. NetBLAST+
searches for sequences similar to a query sequence. The query and the database
searched can be either peptide or nucleic acid in any combination. NetBLAST+
can search only databases maintained at the National
Center for Biotechnology
Information (NCBI) in Bethesda, Maryland,
USA.
SSearch+ does a rigorous Smith-Waterman search for
similarity between a query sequence and a group of sequences of the same type
(nucleic acid or protein). This may be the most sensitive method available for
similarity searches. Compared to BLAST and FastA, it can be very slow.
TFastA+ does a Pearson and Lipman search for similarity
between a protein query sequence and any group of nucleotide sequences. TFastA+
translates the nucleotide sequences in all six reading frames before performing
the comparison. It is designed to answer the question, "What implied
protein sequences in a nucleotide sequence database are similar to my protein
sequence?"
FastX+ does a Pearson and Lipman search for similarity
between a nucleotide query sequence and a group of protein sequences, taking
frameshifts into account. FastX translates both strands of the nucleic sequence
before performing the comparison. It is designed to answer the question,
"What implied protein sequences in my nucleic acid sequence are similar to
sequences in a protein database?"
RESTRICTIONS
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The
query sequence may not be longer than 32,000 symbols. You cannot select a list
size of more than 1,000 best scores nor view more than 1,000 alignments. The
word size must be either 1 or 2.
For
the estimates of statistical significance to be valid, the search set must
contain a large sample of unrelated sequences. The statistical estimates will
not be calculated at all if there are fewer than 10 sequences in the search set
(20 sequences when both strands are searched).
With -NOOPTall, the estimates of statistical
significance will not be accurate.
ALGORITHM
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For
a description of the algorithm, see the FastA program
documentation. TFastX always uses an unrestricted Smith-Waterman algorithm for
the final alignment, so this step may take a long time.
CONSIDERATIONS
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TFastX
translates stop codons in search set sequences to the sequence symbol X.
The
E() scores are affected by similarities in sequence composition between the
query sequence and the search set sequence. Unrelated sequences may have
"significant" scores because of composition bias.
If
there is a database entry that overlaps your query in several places, but there
are large gaps between the matching regions, only the best overlap appears in
the alignment display.
There
are two ways to control the size of the list of best scores. By default, scores
are listed until a specific E() value is reached. You may set the value in
response to the program prompt or by using -EXPect; otherwise the program uses 10.0 for protein searches,
2.0 for nucleic acid searches. (If you are running the program interactively,
it will show no more than 40 scores initially, and ask if you want to see more
scores if there are any more that are less than the E() value.)
If
you use -LIStsize, the E() value is ignored, and the
program will list the number of scores you requested.
You
can control the number of alignments using -NOALIgn and -ALIgn.
The program behaves differently depending on whether it is being run
noninteractively (in batch or with -Default
on the command line) or interactively. In the noninteractive case, the program
displays the number of alignments set by -ALIgn. (If this is not present, it shows 40 alignments or the
number of scores that were listed, whichever is smaller.) If you run the
program interactively, it displays the list of best scores, then asks you how
many alignments you want to see. (This prompt does not appear if you use -NOALIgn or -ALIgn.)
Increasing
Sensitivity By Adjusting Word Size
By
default, TFastX uses a word size of 2. If it finds few or no matches,
especially if your query sequence is short, rerun the search using -WORdsize=1 to increase the sensitivity. Note
that this will dramatically increase the amount of CPU time required to run the
program.
Adjusting
Gap Creation, Gap Extension, and Frameshift Penalties
Unlike
other GCG programs, TFastX does not read the default gap creation, gap
extension, and frameshift penalties from the scoring matrix file. It uses
default penalties that were empirically determined to be appropriate for the
BLOSUM50 scoring matrix. If you select a different scoring matrix with -MATRix, you may need to change the gap
penalties. The histogram display gives a qualitative view of the quality of fit
between the actual distribution of scores and the expected distribution of
scores. This information may indicate whether or not suitable gap creation and
extension penalties were used for the search. When the histogram shows poor
agreement between the actual distribution and the theoretical distribution, you
might consider using -GAPweight and/or -LENgthweight to specify higher gap creation
and extension penalties, respectively. For example, you might increase the gap
creation penalty from 15 to 20 and the gap extension penalty from 2 to 6. You
may also need to use
-FRAMEweight
to adjust the frameshift penalty.
Differences
in Applying Gap Extension Penalties
There
are two different philosophies on how to penalize gaps in an alignment. One way
is to penalize a gap by the gap creation penalty plus the extension penalty
times the length of the gap (gapweight +
(lengthweight x gap length)). The other way is to use the gap
creation penalty plus the extension penalty times the gap length excluding
the first residue in the gap (gapweight
+ (lengthweight x (gap length - 1)).
"Native"
GCG programs, such as Framesearch and Bestfit, handle gap extension penalties
the first way, while the FastA-family programs use the second way. Therefore a
value for -LENgthweight that gives good results with
one of the FastA-family programs may not give equivalent results with a native
GCG program, and vice versa.
Increasing
Program Speed Using Multithreading
This
program is multithreaded. It has the potential to run faster on a machine
equipped with multiple processors because different parts of the analysis can
be run in parallel on different processors. By default, the program assumes you
have one processor, so the analysis is performed using one thread. You can use -PROCessors to increase the number of threads
up to the number of physical processors on the computer.
Under
ideal conditions, the increase in speed is roughly linear with the number of
processors used. But conditions are rarely ideal. If your computer is heavily
used, competition for the processors can reduce the program's performance. In
such an environment, try to run multithreaded programs during times when the
load on the system is light.
As
the number of threads increases, the amount of memory required increases
substantially. You may need to ask your system administrator to increase the
memory quota for your account if you want to use more than two threads.
Never
use -PROCessors to set the number of threads
higher than the number of physical processors that the machine has -- it does
not increase program performance, but instead uses up a lot of memory
needlessly and makes it harder for other users on the system to get processor
time. Ask your system administrator how many processors your computer has if
you aren't sure.
SUGGESTIONS
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Identifying
the Search Set
If
you want to search a single database division instead of an entire database,
see the "Using Database Sequences" topic of Section 2, Using Sequence
Files and Databases of the User's Guide for a list of the logical names used
for the databases and the divisions of each database. The search set can also
consist of a group of sequence files that are not in a database. Use a multiple
sequence specification to name these. For information about naming groups of
sequences for the search set, see the topics "Specifying Files" and
"Using Wildcards" in Section 1, Getting Started, and "Using
Database Sequences," "Using Multiple Sequence Format (MSF)
Files", "Using Rich Sequence Format (RSF) Files", and
"Using List Files" in Section 2, Using Sequence Files and Databases
of the User's Guide.
Batch
Queue
TFastX
is one of the few programs in Accelrys GCG (GCG) that can take more
than a few minutes to run. Most comparisons should probably be run in the batch
queue. You can specify that this program run at a later time in the batch queue
by using -BATch. Run this way, the program prompts you
for all the required parameters and then automatically submits itself to the
batch or at queue. For more information, see "Using
the Batch Queue" in Section 3, Using Programs in the User's Guide.
Very large comparisons may exceed the CPU limit set by some systems.
Interrupting
a Search: <Ctrl>C
You
can type <Ctrl>C to interrupt a search and see the results from the part
of the search that has already been completed. Because the program is
multithreaded, the search may not be interrupted immediately, but will continue
until one of the threads finishes processing its data and returns for more
data.
COMMAND-LINE
SUMMARY
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All
parameters for this program may be added to the command line. Use -CHEck to view the summary below and to
specify parameters before the program executes. In the summary below, the
capitalized letters in the parameter names are the letters that you must
type in order to use the parameter. Square brackets ([ and ]) enclose parameter
values that are optional.
Minimal Syntax: % tfastx [-INfile1=]ggamma.pep -Default
Prompted Parameters:
[-INfile2=]GenBank:* specifies search set
[-OUTfile=]ggamma.tfastx names the output file
-BEGin=1 -END=148 sets the range of interest
-WORdsize=2 sets the word size
-EXPect=2.0 lists scores until E() value reaches 2.0
Local Data Files:
-MATRix=blosum50.cmp assigns the scoring matrix for proteins
Optional Parameters:
-PROCessors=2 sets the number of threads devoted to the analysis
on a multiprocessor computer
-MINLength=1000 searches only sequences of 1000 or more residues
-MAXLength=5000 searches only sequences of 5000 or fewer residues
-SINce=6.90 limits search to sequences dated on or after June 1990
-DBTOPstrand translates and searches only the top (forward) strand of
the search set sequences
-DBBOTtomstrand translates and searches only the reverse complement strand
of the search set sequences
-NOPAMfactor uses a constant factor to calculate initial diagonal scores
-GAPweight=15 sets the gap creation penalty
-LENgthweight=2 sets the gap extension penalty
-FRAmeweight=20 sets the frame shift penalty
-OPTall=20 computes opt score when the initn score is 20
or higher; sorts on opt score
-NOOPTall doesn't compute opt score during search; sorts on initn
-LIStsize=40 shows the best 40 scores (overrides EXPect)
-ALIgn=20 shows the best 20 alignments
-NOALIgn suppresses sequence alignments
-SHOWall shows complete sequences in alignment, not just overlaps
-MARKx=3 sets the alignment display mode
-NOHIStogram suppresses printing the histogram
-LINEsize=60 sets number of sequence symbols per line of the alignment
-NODOCLines suppresses sequence documentation in the alignment
-BATch submits the program to run in the batch queue
-NOMONitor suppresses the screen trace for each search set sequence
LOCAL
DATA FILES
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The
files described below supply auxiliary data to this program. The program
automatically reads them from a public data directory unless you either 1) have
a data file with exactly the same name in your current working directory; or 2)
name a file on the command line with an expression like -DATa1=myfile.dat. For more information
see Section 4, Using Data Files in the User's Guide.
Local
Scoring Matrices
This
program reads one or more scoring matrices for the comparison of sequence
characters. The program automatically reads the program's default scoring
matrix in a public data directory unless you either 1) have a data file with
exactly the same name as the program default scoring matrix in your current
working directory; or 2) have a data file with exactly the same name as the
program default scoring matrix in the directory with the logical name MyData;
or 3) name a file on the command line with an expression like -MATRix=mymatrix.cmp. If you don't include
a directory specification when you name a file with -MATRix, the program searches for the file
first in your local directory, then in the directory with the logical name
MyData, then in the public data directory with the logical name GenMoreData,
and finally in the public data directory with the logical name GenRunData. For
more information see "Using a Special Kind of Data File: A Scoring
Matrix" in Section 4, Using Data Files in the User's Guide.
TFastX
reads a scoring matrix containing the values for every possible match from your
working directory or the public database. The default matrix is blosum50.cmp,
which is a BLOSUM50 matrix. You can use the Fetch
program to obtain a copy of this file if you need to modify it for your own
needs.
PARAMETER REFERENCE
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You
can set the parameters listed below from the command line.
-WORdsize=2
Sets
the size of the word (k-tuple) to use for the hashing step.
-MATRix=mymatrix.cmp
Allows
you to specify a scoring matrix file name other than the program default. If
you don't include a directory specification when you name a file with -MATRix, the program searches for the file
first in your local directory, then in the directory with the logical name
MyData, then in the public data directory with the logical name GenMoreData,
and finally in the public data directory with the logical name GenRunData.
For
more information see the Local Scoring Matrices section.
-EXPect=2.0
Shows
all scores whose E() value is less than 2.0. Ignored if -LIStsize is used.
-PROCessors=2
Tells
the program to use 2 threads for the database search on a multiprocessor
computer.
-MINLength=1000
Restricts
the search to search set sequences that are equal to or longer than 1000
residues.
-MAXLength=5000
Restricts
the search to search set sequences that are equal to or shorter than 5000
residues.
-SINce=6.1990
Limits
the search to sequences that have been entered into the database or modified
since June 1990. As this is being written, only the EMBL, GenBank, and
SWISS-PROT databases support this parameter.
-DBTOPstrand
Translates
and searches only the top strand of search set sequences.
-DBBOTtomstrand
Translates
and searches only the reverse complement strand of search set sequences.
-NOPAMfactor
Uses
a constant factor for the calculation of initial diagonal scores, instead of
using the identical match scores from the scoring matrix.
-GAPweight=12
Specifies
the gap creation penalty that is subtracted from the alignment score whenever a
gap is created.
-LENgthweight=2
Specifies
the gap extension penalty that is subtracted from the alignment score for each residue
added to an existing gap.
-FRAMEweight=20
Specifies
the penalty that is subtracted from the alignment score whenever a frameshift
is inserted.
-OPTall=20
Immediately
performs an alignment and calculates the opt score when the initn score is greater
than or equal to 20. This parameter allows you to override the default
threshold calculated by the program. Scores are sorted and saved by opt score
during the search.
-NOOPTall
doesn't compute the opt score until the search is complete. In this case scores
are sorted and saved by initn score instead of by opt score.
-LIStsize=40
Shows
the best 40 scores. Overrides -EXPect.
-ALIgn=10
Limits
the number of alignments to display in the output file to the 10 best matches
in the list. Use the
-NOALIgn to
suppress the sequence alignments in the output file.
-SHOWall
Shows
entire sequences in the alignment display, instead of just the best region of
overlap and its surroundings.
-MARKx=3
Determines
the alignment display mode -- especially the symbols that identify matches and
mismatches. The default value, 3, uses a pipe character (|) to show identities
and a colon (:) to show conservative replacements. -MARKx=0 uses a colon to show identities
and a period (.) to show conservative replacements. -MARKx=1 will not mark identities;
instead, conservative replacements are connected with a lowercase x, and
non-conservative substitutions are connected with an uppercase X. If -MARKx=2, the residues in the second
sequence are shown only if they differ from the first sequence.
Use -MARKx=10 to get aligned sequences in the FastA "parsable" output format. A document
describing this format appears after FastA in the Program Manual.
-NOHIStogram
Suppresses
printing the histogram.
-LINesize=60
Lets
you set the number of sequence symbols in each line of the alignment to any
number between 60 and 200.
-NODOCLines
Suppresses
the documentation from the search set sequence accompanying the alignment in
the output file. Use
-DOCLines=5 to copy
only five non-blank lines of documentation.
-BATch
Submits
the program to the batch queue for processing after prompting you for all required
user inputs. Any information that would normally appear on the screen while the
program is running is written into a log file. Whether that log file is
deleted, printed, or saved to your current directory depends on how your system
manager has set up the command that submits this program to the batch queue.
All output files are written to your current directory, unless you direct the
output to another directory when you specify the output file.
-MONitor=500
Monitors
this program's progress on your screen. Use this parameter to see this same
monitor in the log file for a batch process. If the monitor is slowing down the
program because your terminal is connected to a slow modem, suppress it with -NOMONitor.
The
monitor is updated every time the program processes 500 sequences or files. You
can use a value after the parameter to set this monitoring interval to some
other number.
Printed:
May 27, 2005 14:55
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All other product names mentioned in this documentation
may be trademarks, and if so, are trademarks or registered trademarks of their
respective holders and are used in this documentation for identification
purposes only.
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