<![CDATA[BOL: Related items]]> https://bioinformaticsonline.com/related/31278?offset=100 https://bioinformaticsonline.com/bookmarks/view/30074/minia Thu, 08 Dec 2016 05:07:00 -0600 https://bioinformaticsonline.com/bookmarks/view/30074/minia <![CDATA[Minia]]> Minia is a short-read assembler based on a de Bruijn graph, capable of assembling a human genome on a desktop computer in a day. The output of Minia is a set of contigs. Minia produces results of similar contiguity and accuracy to other de Bruijn assemblers (e.g. Velvet).

Download

Minia 2.0.7 Linux 64-bits binaries (Source code(Legacy codebase)

For the impatient

A typical Minia command line looks like:

./minia -in reads.fa -kmer-size 31 -abundance-min 3 -out output_prefix

Type

./minia

for a quick explanation of the parameters.

For more information, refer to the manual.

KmerGenie can be used to determine the best k-mer size, minimum abundance of correct k-mers, and genome size estimation for your dataset.

 

Address of the bookmark: http://minia.genouest.org/

]]> Jit https://bioinformaticsonline.com/bookmarks/view/30093/velvet-tutorial Fri, 09 Dec 2016 04:19:07 -0600 https://bioinformaticsonline.com/bookmarks/view/30093/velvet-tutorial <![CDATA[Velvet tutorial]]> The objective of this activity is to help you understand how to run Velvet in general, how to accurately estimate the insert size of a paired-end library through the use of Bowtie, the primary parameters of velvet, and the process involved in producing a de novo assembly from Illumina reads.

http://evomics.org/learning/assembly-and-alignment/velvet/

Address of the bookmark: http://evomics.org/learning/assembly-and-alignment/velvet/

]]> Poonam Mahapatra https://bioinformaticsonline.com/bookmarks/view/30153/e-mem-efficient-computation-of-maximal-exact-matches Thu, 15 Dec 2016 09:30:43 -0600 https://bioinformaticsonline.com/bookmarks/view/30153/e-mem-efficient-computation-of-maximal-exact-matches <![CDATA[E-MEM: Efficient computation of Maximal Exact Matches]]> E-MEM is a C++/OpenMP program designed to efficiently compute MEMs between large genomes. See the README file for instructions on how to use E-MEM. 

E-MEM source code

The source code can be downloaded here

If you use E-MEM, please cite:

  • N. Khiste, L. Ilie, E-MEM: Efficient computation of Maximal Exact Matches for very large genomes, Bioinformatics 31(4) (2015) 509 -- 514.

For any questions, please contact Lucian Ilie: ilie@uwo.ca 

Address of the bookmark: http://www.csd.uwo.ca/~ilie/E-MEM/

]]> Jit https://bioinformaticsonline.com/bookmarks/view/30212/pear Mon, 19 Dec 2016 09:28:30 -0600 https://bioinformaticsonline.com/bookmarks/view/30212/pear <![CDATA[PEAR]]> PEAR is an ultrafast, memory-efficient and highly accurate pair-end read merger. It is fully parallelized and can run with as low as just a few kilobytes of memory.

PEAR evaluates all possible paired-end read overlaps and without requiring the target fragment size as input. In addition, it implements a statistical test for minimizing false-positive results. Together with a highly optimized implementation, it can merge millions of paired end reads within a couple of minutes on a standard desktop computer.

Address of the bookmark: http://sco.h-its.org/exelixis/web/software/pear/doc.html

]]> Jit https://bioinformaticsonline.com/bookmarks/view/30304/mcscan Thu, 22 Dec 2016 03:53:58 -0600 https://bioinformaticsonline.com/bookmarks/view/30304/mcscan <![CDATA[MCscan]]> MCscan is a computer program that can simultaneously scan multiple genomes to identify homologous chromosomal regions and subsequently align these regions using genes as anchors. This is the toolset for generating the synteny correspondences in Plant Genome Duplication Database. It is intended as an easy-to-use and quick way to identify conserved gene arrays both within the same genome and across different genomes.

More at http://chibba.agtec.uga.edu/duplication/mcscan/

Address of the bookmark: http://chibba.agtec.uga.edu/duplication/mcscan/

]]> Bulbul https://bioinformaticsonline.com/bookmarks/view/30538/gkno Tue, 17 Jan 2017 03:35:34 -0600 https://bioinformaticsonline.com/bookmarks/view/30538/gkno <![CDATA[GKNO]]> gkno opens the world of complex bioinformatic analysis to people of all level of computational expertise. This site contains documentation, tutorials and information on all the tools that comprise gkno.

More at http://gkno.me/

Address of the bookmark: http://gkno.me/

]]> Jit https://bioinformaticsonline.com/bookmarks/view/30829/mercator Mon, 06 Feb 2017 04:20:36 -0600 https://bioinformaticsonline.com/bookmarks/view/30829/mercator <![CDATA[Mercator]]> Our basic strategy in building homology maps is to use exons that are orthologous in multiple genomes as map "anchors." Given K genomes, the steps in the map construction are as follows:

  • For each genome, obtain a set of exon annotations. These annotations can be a combination of both exon predictions (e.g. Genscan) and annotations that have been experimentally verified (e.g. RefSeq). Ideally, we would like to have these annotations be as sensitive as possible. Specificity is not a concern, as incorrect annotations are not likely not have significant alignments with other gene annotations.
  • Compare all exons against all exons in other genomes and record significant alignments between exons. Currently, we use BLAT to do this all-vs-all comparison with alignments being performed in protein space.
  • Construct a graph with each vertex corresponding to a exon and edges between vertices whose corresponding exons have significant alignments.
  • Identify cliques in this graph. These cliques are potential anchors to be used in the map.
  • Starting with the largest cliques (those that have exons in all or most of the genomes), join neighboring (adjacent in genomic coordinates, in each genome) cliques to form runs. Smaller cliques that are inconsistent with runs formed by larger cliques are filtered out. After the smallest cliques have been considered, cliques that are not part of a run are discarded.
  • The extents of each run in each genome are outputted as orthologous segments. The cliques from each run are used to output the exact genomic coordinates of anchors within each orthologous segment. These anchors can be used by genomic alignment programs (such as MAVID) to do a detailed alignment of each orthologous segment.

https://www.biostat.wisc.edu/~cdewey/mercator/

Address of the bookmark: https://www.biostat.wisc.edu/~cdewey/mercator/

]]> Jit https://bioinformaticsonline.com/bookmarks/view/30976/brig Thu, 16 Feb 2017 13:14:25 -0600 https://bioinformaticsonline.com/bookmarks/view/30976/brig <![CDATA[BRIG]]> BRIG is a free cross-platform (Windows/Mac/Unix) application that can display circular comparisons between a large number of genomes, with a focus on handling genome assembly data. The application is available at:http://sourceforge.net/projects/brig

If you have any questions or comments, post them on one of the trackers on BRIG’s SourceForge page:http://sourceforge.net/tracker/?group_id=328245.

Features:

  • Images show similarity between a central reference sequence and other sequences as concentric rings.
  • BRIG will perform all BLAST comparisons and file parsing automatically via a simple GUI.
  • Contig boundaries and read coverage can be displayed for draft genomes; customized graphs and annotations can be displayed.
  • Using a user-defined set of genes as input, BRIG can display gene presence, absence, truncation or sequence variation in a set of complete genomes, draft genomes or even raw, unassembled sequence data.
  • BRIG also accepts SAM-formatted read-mapping files enabling genomic regions present in unassembled sequence data from multiple samples to be compared simultaneously

 

Address of the bookmark: http://brig.sourceforge.net/

]]> Jit https://bioinformaticsonline.com/bookmarks/view/31139/pbsuite-software-for-long-read-sequencing-data-from-pacbio Mon, 27 Feb 2017 09:54:47 -0600 https://bioinformaticsonline.com/bookmarks/view/31139/pbsuite-software-for-long-read-sequencing-data-from-pacbio <![CDATA[PBSuite: Software for Long-Read Sequencing Data from PacBio]]> PBJelly - the genome upgrading tool. 
PBHoney - the structural variation discovery tool 

Both are contained within the PBSuite code found in downloads.

----- PBJelly -----
Read The Paper 
http://www.plosone.org/article/info%3Adoi%2F10.1371%2Fjournal.pone.0047768

PBJelly is a highly automated pipeline that aligns long sequencing reads (such as PacBio RS reads or long 454 reads in fasta format) to high-confidence draft assembles. PBJelly fills or reduces as many captured gaps as possible to produce upgraded draft genomes. 

----- PBHoney -----
Read The Paper
http://www.biomedcentral.com/1471-2105/15/180/abstract

PBHoney is an implementation of two variant-identification approaches designed to exploit the high mappability of long reads (i.e., greater than 10,000 bp). PBHoney considers both intra-read discordance and soft-clipped tails of long reads to identify structural variants.

Address of the bookmark: https://sourceforge.net/projects/pb-jelly/

]]> Jit https://bioinformaticsonline.com/bookmarks/view/32376/diamond Thu, 27 Apr 2017 04:21:54 -0500 https://bioinformaticsonline.com/bookmarks/view/32376/diamond <![CDATA[DIAMOND]]> DIAMOND is a sequence aligner for protein and translated DNA searches and functions as a drop-in replacement for the NCBI BLAST software tools. It is suitable for protein-protein search as well as DNA-protein search on short reads and longer sequences including contigs and assemblies, providing a speedup of BLAST ranging up to x20,000.

More at file:///home/urbe/Downloads/diamond_manual.pdf

http://www.nature.com/nmeth/journal/v12/n1/full/nmeth.3176.html

Address of the bookmark: https://github.com/bbuchfink/diamond

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