<![CDATA[BOL: Related items]]> https://bioinformaticsonline.com/related/36897?offset=30 https://bioinformaticsonline.com/bookmarks/view/43057/hapsolo-an-optimization-approach-for-removing-secondary-haplotigs-during-diploid-genome-assembly-and-scaffolding Sat, 08 May 2021 21:25:00 -0500 https://bioinformaticsonline.com/bookmarks/view/43057/hapsolo-an-optimization-approach-for-removing-secondary-haplotigs-during-diploid-genome-assembly-and-scaffolding <![CDATA[HapSolo: An optimization approach for removing secondary haplotigs during diploid genome assembly and scaffolding]]> HapSolo, that identifies secondary contigs and defines a primary assembly based on multiple pairwise contig alignment metrics. HapSolo evaluates candidate primary assemblies using BUSCO scores and then distinguishes among candidate assemblies using a cost function. The cost function can be defined by the user but by default considers the number of missing, duplicated and single BUSCO genes within the assembly. HapSolo performs hill climbing to minimize cost over thousands of candidate assemblies. 

Address of the bookmark: https://github.com/esolares/HapSolo

]]> Jit https://bioinformaticsonline.com/blog/view/43634/illumina-based-assembly-pipeline-steps Fri, 10 Dec 2021 06:22:54 -0600 https://bioinformaticsonline.com/blog/view/43634/illumina-based-assembly-pipeline-steps <![CDATA[Illumina based assembly pipeline steps !]]> Illumina
  1. Merge re-sequenced FastQ files (cat)
  2. Read QC (FastQC)
  3. Adapter trimming (fastp)
  4. Removal of host reads (Kraken 2; optional)
  5. Variant calling
    1. Read alignment (Bowtie 2)
    2. Sort and index alignments (SAMtools)
    3. Primer sequence removal (iVar; amplicon data only)
    4. Duplicate read marking (picard; optional)
    5. Alignment-level QC (picard, SAMtools)
    6. Genome-wide and amplicon coverage QC plots (mosdepth)
    7. Choice of multiple variant calling and consensus sequence generation routes (iVar variants and consensus; default for amplicon data || BCFTools, BEDTools; default for metagenomics data)
      • Variant annotation (SnpEff, SnpSift)
      • Consensus assessment report (QUAST)
      • Lineage analysis (Pangolin)
      • Clade assignment, mutation calling and sequence quality checks (Nextclade)
      • Individual variant screenshots with annotation tracks (ASCIIGenome)
    8. Intersect variants across callers (BCFTools)
  6. De novo assembly
    1. Primer trimming (Cutadapt; amplicon data only)
    2. Choice of multiple assembly tools (SPAdes || Unicycler || minia)
  7. Present QC and visualisation for raw read, alignment, assembly and variant calling results (MultiQC)
]]> Surabhi Chaudhary https://bioinformaticsonline.com/bookmarks/view/44373/mitohifi-a-python-pipeline-for-mitochondrial-genome-assembly-from-pacbio-high-fidelity-reads Tue, 05 Sep 2023 07:31:35 -0500 https://bioinformaticsonline.com/bookmarks/view/44373/mitohifi-a-python-pipeline-for-mitochondrial-genome-assembly-from-pacbio-high-fidelity-reads <![CDATA[MitoHiFi: a python pipeline for mitochondrial genome assembly from PacBio high fidelity reads]]> MitoHiFi v3.2 is a python pipeline distributed under MIT License !

MitoHiFi was first developed to assemble the mitogenomes for a wide range of species in the Darwin Tree of Life Project (DToL)

https://bmcbioinformatics.biomedcentral.com/articles/10.1186/s12859-023-05385-y 

Address of the bookmark: https://github.com/marcelauliano/MitoHiFi

]]> Abhi https://bioinformaticsonline.com/bookmarks/view/26306/busco Sun, 07 Feb 2016 16:02:39 -0600 https://bioinformaticsonline.com/bookmarks/view/26306/busco <![CDATA[BUSCO]]> Assessing genome assembly and annotation completeness with Benchmarking Universal Single-Copy Orthologs

More at http://busco.ezlab.org/

Address of the bookmark: http://busco.ezlab.org/

]]> Jitendra Narayan https://bioinformaticsonline.com/bookmarks/view/31100/vaguevelvet-assembler-graphical-front-end Fri, 24 Feb 2017 08:56:49 -0600 https://bioinformaticsonline.com/bookmarks/view/31100/vaguevelvet-assembler-graphical-front-end <![CDATA[VAGUE:Velvet Assembler Graphical Front End]]> VAGUE is a vague acronym for "Velvet Assembler Graphical Front End", which means it is a GUI for the Velvet de novo assembler. The command line version of Velvet can be complicated for beginners to use, but VAGUE makes it clear and simple

More at http://www.vicbioinformatics.com/software.vague.shtml

Address of the bookmark: http://www.vicbioinformatics.com/software.vague.shtml

]]> Jit https://bioinformaticsonline.com/bookmarks/view/31105/understanding-pacbio Fri, 24 Feb 2017 10:17:36 -0600 https://bioinformaticsonline.com/bookmarks/view/31105/understanding-pacbio <![CDATA[Understanding PacBio]]> This tutorial includes resources for learning more about PacBio data and bioinformatics analysis, and includes content suitable for both beginners and experts. Below are links to training modules (webinars and PowerPoint presentations) to help you get started with your data processing, as well as information for specialized applications.

Training Resources:

Specialized Applications:

Address of the bookmark: https://github.com/PacificBiosciences/Bioinformatics-Training/wiki

]]> Jitendra Narayan 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/30205/garmgenome-assembly-reconciliation-and-merging Mon, 19 Dec 2016 06:03:02 -0600 https://bioinformaticsonline.com/bookmarks/view/30205/garmgenome-assembly-reconciliation-and-merging <![CDATA[GARM:Genome Assembly, Reconciliation and Merging]]> The pipeline is based mainly implemented using Perl scripts and modules and third-party open source software like the AMOS (Myers et al., 2000) and MUMmer (Kurtz et al., 2004) packages. The pipeline was tested on Debian, Ubuntu, Fedora and BioLinux distributions. The method merges contigs or scaffolds from different assemblers using the same or different sequencing technologies. When scaffolds are provided, a process of finding probable compressions or extensions (CE) problems in the assemblies can be per-formed; contigs are joined back into scaffolds after gap recalculation

Address of the bookmark: http://garm-meta-assem.sourceforge.net/

]]> Jit https://bioinformaticsonline.com/bookmarks/view/30216/quickmerge-a-simple-and-fast-metassembler-and-assembly-gap-filler-designed-for-long-molecule-based-assemblies Mon, 19 Dec 2016 10:23:36 -0600 https://bioinformaticsonline.com/bookmarks/view/30216/quickmerge-a-simple-and-fast-metassembler-and-assembly-gap-filler-designed-for-long-molecule-based-assemblies <![CDATA[quickmerge: A simple and fast metassembler and assembly gap filler designed for long molecule based assemblies.]]> quickmerge uses a simple concept to improve contiguity of genome assemblies based on long molecule sequences, often with dramatic outcomes. The program uses information from assemblies made with illumina short reads and PacBio long reads to improve contiguities of an assembly generated with PacBio long reads alone. This is counterintuitive because illumina short reads are not typically considered to cover genomic regions which PacBio long reads cannot. Although we have not evaluated this program for assemblies generated with Oxford nanopore sequences, the program should work with ONP-assemblies too. 

Address of the bookmark: https://github.com/mahulchak/quickmerge

]]> Jit https://bioinformaticsonline.com/bookmarks/view/31343/metabat-an-efficient-tool-for-accurately-reconstructing-single-genomes-from-complex-microbial-communities Mon, 06 Mar 2017 03:44:34 -0600 https://bioinformaticsonline.com/bookmarks/view/31343/metabat-an-efficient-tool-for-accurately-reconstructing-single-genomes-from-complex-microbial-communities <![CDATA[MetaBAT: An Efficient Tool for Accurately Reconstructing Single Genomes from Complex Microbial Communities]]> MetaBAT, An Efficient Tool for Accurately Reconstructing Single Genomes from Complex Microbial Communities

Grouping large genomic fragments assembled from shotgun metagenomic sequences to deconvolute complex microbial communities, or metagenome binning, enables the study of individual organisms and their interactions. Here we developed an automated metagenome binning software, called MetaBAT, which integrates empirical probabilistic distances of genome abundance and tetranucleotide frequency. Tested on both synthetic and real metagenome datasets, MetaBAT outperforms alternative methods in both accuracy and computational efficiency. Applying MetaBAT to an assembly from 1,704 human gut samples formed 1,634 genome bins (>200kb) in 3 hours, where 621 genome bins are >50% complete with <5% contamination from other species. Further analysis shows that the quality of these genome bins approaches manually curated genomes.

Address of the bookmark: https://bitbucket.org/berkeleylab/metabat

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