Login or Register to Ask a Question and Join Our Community

Sponsored Content
Full Discussion: Parsing a fasta sequence with start and end coordinates
Top Forums Shell Programming and Scripting Parsing a fasta sequence with start and end coordinates Post 302514157 by empyrean on Friday 15th of April 2011 01:47:10 AM
Old 04-15-2011
Thanks for the reply.. i am pretty new to awk programming.. so i have chromosome 1 in a fasta file format and where should i give it as input?
 

10 More Discussions You Might Find Interesting

1. UNIX for Dummies Questions & Answers

Help Parsing Sequence File

Hi Everyone, I am new in the world of UNIX and Shell scripting. I am working with a sequence file that looks like this: >contig00001 length=128 numreads=2 aTGTGCTGGgTGGGTGCCTGTTgCCccATGCTCCAGTtCAGGATTtCAGGCAttCTCATG TCCAGCATTTCTATTTAATCCTGCTGCTGGACTTGGGTGGtCTCAGTCtGGGAAGTGAGC tGTCTGTG... (8 Replies)
Discussion started by: Fahmida
8 Replies

2. UNIX for Dummies Questions & Answers

How to change sequence name in along fasta file?

Hi I have an alignment file (.fasta) with ~80 sequences. They look like this- >JV101.contig00066(+):25302-42404|sequence_index=0|block_index=4|species=JV101|JV101_4_0 GAGGTTAATTATCGATAACGTTTAATTAAAGTGTTTAGGTGTCATAATTT TAAATGACGATTTCTCATTACCATACACCTAAATTATCATCAATCTGAAT... (2 Replies)
Discussion started by: baika
2 Replies

3. Shell Programming and Scripting

Remove lines between the start string and end string including start and end string Python

Hi, I am trying to remove lines once a string is found till another string is found including the start string and end string. I want to basically grab all the lines starting with color (closing bracket). PS: The line after the closing bracket for color could be anything (currently 'more').... (1 Reply)
Discussion started by: Dabheeruz
1 Replies

4. UNIX for Dummies Questions & Answers

Change sequence names in fasta file

I have fasta files with multiple sequences in each. I need to change the sequence name headers from: >accD:_59176-60699 ATGGAAAAGTGGAGGATTTATTCGTTTCAGAAGGAGTTCGAACGCA >atpA_(reverse_strand):_showing_revcomp_of_10525-12048 ATGGTAACCATTCAAGCCGACGAAATTAGTAATCTTATCCGGGAAC... (2 Replies)
Discussion started by: tyrianthinae
2 Replies

5. Shell Programming and Scripting

Extract sequence from fasta file

Hi, I want to match the sequence id (sub-string of line starting with '>' and extract the information upto next '>' line ). Please help . input > fefrwefrwef X900 AGAGGGAATTGG AGGGGCCTGGAG GGTTCTCTTC > fefrwefrwef X932 AGAGGGAATTGG AGGAGGTGGAG GGTTCTCTTC > fefrwefrwef X937... (2 Replies)
Discussion started by: ritakadm
2 Replies

6. Shell Programming and Scripting

Count and search by sequence in multiple fasta file

Hello, I have 10 fasta files with sequenced reads information with read sizes from 15 - 35 . I have combined the reads and collapsed in to unique reads and filtered for sizes 18 - 26 bp long unique reads. Now i wanted to count each unique read appearance in all the fasta files and make a table... (5 Replies)
Discussion started by: empyrean
5 Replies

7. Shell Programming and Scripting

Parsing and masking regions from a single fasta file with subsequence

HI, I have a Complete genome fasta file and I have list of sub sequence regions in the format as : 4353..5633 6795..9354 1034..14456 I want a script which can mask these region in a single complete genome fasta file with the alphabet N kindly help (2 Replies)
Discussion started by: margarita
2 Replies

8. Shell Programming and Scripting

Command Line Perl for parsing fasta file

I would like to take a fasta file formated like >0001 agttcgaggtcagaatt >0002 agttcgag >0003 ggtaacctga and use command line perl to move the all sample gt 8 in length to a new file. the result would be >0001 agttcgaggtcagaatt >0003 ggtaacctga cat ${sample}.fasta | perl -lane... (2 Replies)
Discussion started by: jdilts
2 Replies

9. UNIX for Beginners Questions & Answers

How to find a specific sequence pattern in a fasta file?

I have to mine the following sequence pattern from a large fasta file namely gene.fasta (contains multiple fasta sequences) along with the flanking sequences of 5 bases at starting position and ending position, AAGCZ-N16-AAGCZ Z represents A, C or G (Except T) N16 represents any of the four... (3 Replies)
Discussion started by: dineshkumarsrk
3 Replies

10. UNIX for Beginners Questions & Answers

Splitting week start date and end date based on custom period start dates

Below are my custom period start and end dates based on a calender, these dates are placed in a file, for each period i need to split into three weeks for each period row, example is given below. Could you please help out to achieve solution through shell script.. File content: ... (2 Replies)
Discussion started by: nani2019
2 Replies

LEARN ABOUT DEBIAN

bio::seqio::tab

Bio::SeqIO::tab(3pm)					User Contributed Perl Documentation				      Bio::SeqIO::tab(3pm)

NAME

       Bio::SeqIO::tab - nearly raw sequence file input/output stream. Reads/writes id"	"sequence"
"

SYNOPSIS

       Do not use this module directly.  Use it via the Bio::SeqIO class.

DESCRIPTION

       This object can transform Bio::Seq objects to and from tabbed flat file databases.

       It is very useful when doing large scale stuff using the Unix command line utilities (grep, sort, awk, sed, split, you name it). Imagine
       that you have a format converter 'seqconvert' along the following lines:

	 my $in  = Bio::SeqIO->newFh(-fh => *STDIN , '-format' => $from);
	 my $out = Bio::SeqIO->newFh(-fh=> *STDOUT, '-format' => $to);
	 print $out $_ while <$in>;

       then you can very easily filter sequence files for duplicates as:

	 $ seqconvert < foo.fa -from fasta -to tab | sort -u |
	      seqconvert -from tab -to fasta > foo-unique.fa

       Or grep [-v] for certain sequences with:

	 $ seqconvert < foo.fa -from fasta -to tab | grep -v '^S[a-z]*control' |
	      seqconvert -from tab -to fasta > foo-without-controls.fa

       Or chop up a huge file with sequences into smaller chunks with:

	 $ seqconvert < all.fa -from fasta -to tab | split -l 10 - chunk-
	 $ for i in chunk-*; do seqconvert -from tab -to fasta < $i > $i.fa; done
	 # (this creates files chunk-aa.fa, chunk-ab.fa, ..., each containing 10
	 # sequences)

FEEDBACK

   Mailing Lists
       User feedback is an integral part of the evolution of this and other Bioperl modules. Send your comments and suggestions preferably to one
       of the Bioperl mailing lists.  Your participation is much appreciated.

	 bioperl-l@bioperl.org			- General discussion
	 http://bioperl.org/wiki/Mailing_lists	- About the mailing lists

   Support
       Please direct usage questions or support issues to the mailing list:

       bioperl-l@bioperl.org

       rather than to the module maintainer directly. Many experienced and reponsive experts will be able look at the problem and quickly address
       it. Please include a thorough description of the problem with code and data examples if at all possible.

   Reporting Bugs
       Report bugs to the Bioperl bug tracking system to help us keep track the bugs and their resolution.  Bug reports can be submitted via the
       web:

	 https://redmine.open-bio.org/projects/bioperl/

AUTHORS

       Philip Lijnzaad, p.lijnzaad@med.uu.nl

APPENDIX

       The rest of the documentation details each of the object methods.  Internal methods are usually preceded with a _

   next_seq
	Title	: next_seq
	Usage	: $seq = $stream->next_seq()
	Function: returns the next sequence in the stream
	Returns : Bio::Seq object
	Args	:

   write_seq
	Title	: write_seq
	Usage	: $stream->write_seq($seq)
	Function: writes the $seq object into the stream
	Returns : 1 for success and 0 for error
	Args	: Bio::Seq object

perl v5.14.2							    2012-03-02						      Bio::SeqIO::tab(3pm)
All times are GMT -4. The time now is 07:18 PM.
Unix & Linux Forums Content Copyright 1993-2022. All Rights Reserved.
Privacy Policy