<![CDATA[BOL: Related items]]> https://bioinformaticsonline.com/related/26306?offset=1330 https://bioinformaticsonline.com/bookmarks/view/37674/qualimap2-evaluating-next-generation-sequencing-alignment-data Tue, 11 Sep 2018 04:44:29 -0500 https://bioinformaticsonline.com/bookmarks/view/37674/qualimap2-evaluating-next-generation-sequencing-alignment-data <![CDATA[Qualimap2: Evaluating next generation sequencing alignment data]]> Qualimap 2 is a platform-independent application written in Java and R that provides both a Graphical User Inteface (GUI) and a command-line interface to facilitate the quality control of alignment sequencing data and its derivatives like feature counts. 

Supported types of experiments include:

  • Whole-genome sequencing
  • Whole-exome sequencing
  • RNA-seq (speical mode available)
  • ChIP-seq

Address of the bookmark: http://qualimap.bioinfo.cipf.es/

]]> Jit https://bioinformaticsonline.com/bookmarks/view/39726/jackalope-a-swift-versatile-phylogenomic-and-high-throughput-sequencing-simulator Fri, 26 Jul 2019 00:58:12 -0500 https://bioinformaticsonline.com/bookmarks/view/39726/jackalope-a-swift-versatile-phylogenomic-and-high-throughput-sequencing-simulator <![CDATA[jackalope: A swift, versatile phylogenomic and high-throughput sequencing simulator]]> jackalope simply and efficiently simulates (i) variants from reference genomes and (ii) reads from both Illumina and Pacific Biosciences (PacBio) platforms. It can either read reference genomes from FASTA files or simulate new ones. Genomic variants can be simulated using summary statistics, phylogenies, Variant Call Format (VCF) files, and coalescent simulations—the latter of which can include selection, recombination, and demographic fluctuations. jackalope can simulate single, paired-end, or mate-pair Illumina reads, as well as reads from Pacific Biosciences These simulations include sequencing errors, mapping qualities, multiplexing, and optical/PCR duplicates. All outputs can be written to standard file formats.

A swift, versatile phylogenomic and high-throughput sequencing simulator https://jackalope.lucasnell.com

Address of the bookmark: https://github.com/lucasnell/jackalope

]]> Abhimanyu Singh https://bioinformaticsonline.com/bookmarks/view/41009/genomics-public-data-links Thu, 13 Feb 2020 00:20:00 -0600 https://bioinformaticsonline.com/bookmarks/view/41009/genomics-public-data-links <![CDATA[genomics public data links !]]> List of publically available databases on google server.

More at https://software.broadinstitute.org/gatk/download/bundle

ftp://ftp.ncbi.nlm.nih.gov/snp/organisms/human_9606/VCF/GATK/.

ftp://ftp.broadinstitute.org/bundle/hg38/hg38bundle/

Address of the bookmark: https://console.cloud.google.com/storage/browser/genomics-public-data/resources/broad/hg38/v0?pli=1

]]> Jit https://bioinformaticsonline.com/blog/view/43550/basic-structure-of-snakemake-pipeline-run Thu, 14 Oct 2021 07:01:38 -0500 https://bioinformaticsonline.com/blog/view/43550/basic-structure-of-snakemake-pipeline-run <![CDATA[Basic Structure of Snakemake Pipeline Run !]]> /user/snakemake-demo$ ls
config.json data envs scripts slurm-240702.out Snakefile
  • data = mock data for the snakefile to use
  • Snakefile = name of the snakemake “formula” file
    • Note: The default file that snakemake looks for in the current working directory is the Snakefile. If you would like to override that you can specify it following the -s
      • snakemake -s snakefile.py
  • envs = directory for storing the conda environments that the workflow will use.
  • scripts = directory for storing python scripts called by the snakemake formula.
  • config.json = json format file with extra parameters for our snakemake file to use.
  • cluster.json = json format file with specification for running on the HPC
  • samples.txt = file we will use later relating to the config.json file.

Run the snakemake file as a dry run (the example workflow shown above).

  • This will build a DAG of the jobs to be run without actually executing them.
  • snakemake --dry-run

User can execute rules of interest.

  • snakemake --dry-run all VS. snakemake --dry-run call VS. snakemake --dry-run bwa

Run the snakemake file in order to produce an image of the DAG of jobs to be run.

  • snakemake --dag | dot -Tsvg > dag.svg OR snakemake --dag | dot -Tsvg > dag.svg

Run the snakemake (this time not as a dry run)

  1. snakemake --use-conda
]]> Abhi https://bioinformaticsonline.com/bookmarks/view/44675/variant-calling-pipeline Sat, 19 Oct 2024 12:23:40 -0500 https://bioinformaticsonline.com/bookmarks/view/44675/variant-calling-pipeline <![CDATA[Variant Calling Pipeline]]> The variantcalling.nf nextflow script will take any number of samples with paired-end reads in FASTQ format, map reads using Bowtie2, process BAM files, and finally call variants using BCFtools v1.21 and/or Freebayes v1.3.6. If part of the pipeline is unsuccessful for a sample then these errors are ignored.

Pipeline flowchart:

 
 

Dependencies (version tested)

  • Nextflow (24.04.4)
  • Java (18.0.2.1)
  • Python (3.10)
  • Perl (5.32.1)
  • Bowtie2 (2.5.3)
  • SAMtools (1.19.2)
  • GATK4 (4.5)
  • BCFtools (1.21)
  • Freebayes (1.3.6)

Address of the bookmark: https://github.com/Tom-Jenkins/nextflow-pipelines/blob/main/docs/variant-calling.md

]]> LEGE https://bioinformaticsonline.com/bookmarks/view/35292/pgap-x-extension-on-pan-genome-analysis-pipeline Tue, 23 Jan 2018 11:41:43 -0600 https://bioinformaticsonline.com/bookmarks/view/35292/pgap-x-extension-on-pan-genome-analysis-pipeline <![CDATA[PGAP-X: Extension on pan-genome analysis pipeline]]> PGAP-X is a microbial comparative genomic analysis platform with graphic interface. Serials of algorithms and methodologies have been developed and integrated to analyze and visualize genomics structure variation, gene distribution with different conservative levels, and genetic variation from pan-genome sight. At the same time, analytical result data from many other programs, including genome alignment result and orthologs clusters, are also supported to be further analyzed or visualized in PGAP-X. The workflow and feature snapshot in PGAP-X were shown as Fig.1 and Fig.2.

image
 

 

Address of the bookmark: https://pgapx.ybzhao.com/

]]> Rahul Nayak https://bioinformaticsonline.com/bookmarks/view/38762/katuali-is-a-flexible-consensus-pipeline-implemented-in-snakemake-to-basecall-assemble-and-polish-oxford-nanopore-technologies-sequencing-data Tue, 22 Jan 2019 06:26:55 -0600 https://bioinformaticsonline.com/bookmarks/view/38762/katuali-is-a-flexible-consensus-pipeline-implemented-in-snakemake-to-basecall-assemble-and-polish-oxford-nanopore-technologies-sequencing-data <![CDATA[Katuali is a flexible consensus pipeline implemented in Snakemake to basecall, assemble, and polish Oxford Nanopore Technologies' sequencing data]]>
  • Run a pipeline processing fast5s to a consensus in a single command.
  • Recommended fixed "standard" and "fast" pipelines.
  • Interchange basecaller, assembler, and consensus components of the pipelines simply by changing the target filepath.
  • Seemless distribution of tasks over local or distributed compute.
  • Highly configurable.
  • Open source (Mozilla Public License 2.0).

    • Documentation can be found at https://nanoporetech.github.io/katuali/.

    Address of the bookmark: https://github.com/nanoporetech/katuali

    ]]>     Jit     https://bioinformaticsonline.com/bookmarks/view/41030/slr-superscaffolder-a-scaffold-assemble-pipeline-for-stlfr-reads Fri, 14 Feb 2020 14:23:30 -0600 https://bioinformaticsonline.com/bookmarks/view/41030/slr-superscaffolder-a-scaffold-assemble-pipeline-for-stlfr-reads <![CDATA[SLR-superscaffolder: A scaffold assemble pipeline for stLFR reads.]]> This is a scaffold assembler designed for stLFR reads[1]. It uses the link-reads information from stLFR reads to assemble contigs to scaffolds.

    Here is an illustration of this pipeline:

     image

    Address of the bookmark: https://github.com/BGI-Qingdao/SLR-superscaffolder

    ]]>     Jit     https://bioinformaticsonline.com/bookmarks/view/42038/pyparanoid-a-pipeline-for-rapid-identification-of-homologous-gene-families-in-a-set-of-genomes Thu, 13 Aug 2020 10:06:19 -0500 https://bioinformaticsonline.com/bookmarks/view/42038/pyparanoid-a-pipeline-for-rapid-identification-of-homologous-gene-families-in-a-set-of-genomes <![CDATA[PyParanoid: a pipeline for rapid identification of homologous gene families in a set of genomes]]> PyParanoid is a pipeline for rapid identification of homologous gene families in a set of genomes - a central task of any comparative genomics analysis. The "gold standard" for identifying homologs is to use reciprocal best hits (RBHs) which depends on performing a all-vs-all sequence comparison, usually using BLAST, to determine homology. However, these methods are computationally expensive, requiring O(n2) resources to identify RBHs. This is problematic, as the modern deluge of sequencing data means that comparative genomics analyses could be performed on datasets of thousands of strains.

    Address of the bookmark: https://github.com/ryanmelnyk/PyParanoid

    ]]>     BioStar     https://bioinformaticsonline.com/bookmarks/view/43353/judi-just-do-it Mon, 06 Sep 2021 02:44:35 -0500 https://bioinformaticsonline.com/bookmarks/view/43353/judi-just-do-it <![CDATA[JUDI: Just Do It]]> judi comes from the idea of bringing the power and efficiency of doit to execute any kind of task under many combinations of parameter settings.

    https://github.com/ncbi/JUDI

    Address of the bookmark: https://github.com/ncbi/JUDI

    ]]>     Jit