Home

MIRA is a whole genome shotgun and EST sequence assembler for Sanger, 454, Solexa (Illumina), IonTorrent data and PacBio (the later at the moment only CCS and error-corrected CLR reads). It can be seen as a Swiss army knife of sequence assembly developed and used in the past 16 years to get assembly jobs done efficiently - and especially accurately. That is, without actually putting too much manual work into finishing the assembly.

The latest stable version is MIRA 4.0

---

Table of contents

• Quicklinks
• Documentation
• Short history
• Hybrid de-novo assemblies with Sanger, 454, Illumina / Solexa, IonTorrent and PacBio
• Automatic sequence editors
• SNP and mutations discovery for mapping assemblies
• Publications
  • Papers
  • Posters
• Sponsors

---

Quicklinks

• Visit the project page on SourceForge
• Download the latest release either as source or as binary for Linux or OSX
• See some interesting features of MIRA 4 explained in action
• Found a bug or have a feature request? File it here and also send a quick mail to the MIRA talk mailing list
• Need help? Want to discuss something with other users? There are mailing lists for MIRA

Documentation

The most up-to-date documentation is also always available in the binary distribution packages.

• Whole documentation, stable version as HTML, one file (800 KiB + 3 MiB images)
• Whole documentation, stable version: PDF (3.5 MiB)

Scaffolding:
* Scaffolding with Bambus Instructions for scaffolding MIRA contigs & paired-end data with BAMBUS. Written by Gregory Harhay, USDA.

Short history

MIRA started in 1997 as a PhD project at the German Cancer Research Centre in Heidelberg (Deutsches Krebsforschungszentrum Heidelberg). Binaries were always distributed publicly and over time, other labs and sequencing providers have found MIRA useful for assembly of extremely 'unfriendly' projects containing lots of repetitive sequences (as always, your mileage may vary).

In 2007 I (Bastien Chevreux) asked the DKFZ for the permission to put MIRA under an open source license ... and got it.

Hybrid de-novo assemblies with Sanger, 454, Illumina / Solexa, IonTorrent and PacBio

MIRA 4 is able to perform true hybrid de-novo assemblies using reads gathered through Sanger, 454, Solexa, IonTorrent or PacBio sequencing technologies. That is, it assembles reads instead of a mix of (eventually shredded) consensus sequence and reads. See an example on how it looks like for Sanger and 454 in the documentation introduction, but it also works with any other combination of sequencing technologies. Only restriction at the moment: reads must be <= 32 kilobases and for PacBio, MIRA must get CCS reads or error-corrected CLR data.

The combination currently preferred by the author is a mix of de-novo error-corrected PacBio reads and Illumina mapping assemblies: PacBio to get long contigs built, Illumina to get rid of the indels which even Quiver (PacBio software) cannot get rid of. Here's the recipe I use for sequencing a bacterium or lower eukaryote de-novo and almost perfectly for comparatively little money:

1. get your DNA sequenced at ~100x polymerase read coverage with PacBio
2. get the very same DNA sequenced at ~30-100x coverage with Illumina (100 or more base pairs)
3. get the error corrected sequences from the HGAP pipeline and assemble them with MIRA
4. map Illumina data to the assembly above with MIRA
5. add half a day or so for prettifying the resulting assembly and check remaining uncertainties (if you really want to) with gap4

Granted, there may be a few more steps ... but that's basically it.

Automatic sequence editors

MIRA contains integrated editors for all sequence technologies which iteratively remove many sequencing errors from the assembly project and improve the overal alignment quality.

SNP and mutations discovery for mapping assemblies

MIRA can also be used for mapping assemblies and automatic tagging of difference site (SNPs, insertions or deletions) of mutant strains against a reference sequence.

For organisms where annotated files in GFF3 format are available (or for GenBank files without intron/exon structures), MIRA can generate tables which are ready to use for biologists as they show exactly which genes are hit and give a first estimate whether the function of the protein is attained by the change.

Publications

Papers

• Chevreux et al. (1999) Genome Sequence Assembly Using Trace Signals and Additional Sequence Information Computer Science and Biology: Proceedings of the German Conference on Bioinformatics (GCB) 99, pp. 45-56. There are also slides for the talk held at the conference, get them here.
• Chevreux et al. (2004) Using the miraEST Assembler for Reliable and Automated mRNA Transcript Assembly and SNP Detection in Sequenced ESTs Genome Research 2004. 14:1147-1159.

Posters

• Chevreux et al. (1998) Computer assisted editing of genomic sequences poster at the "Genome and Proteomics 98" in Heidelberg and the "German Conference on Bioinformatics" GCB 98 in Cologne (english)
• Chevreux et al. (1999) MIRA & EdIt poster presented at the ISMB 99 conference in Heidelberg and the "German Conference on Bioinformatics" GCB 99 in Hannover

Sponsors

• 1997 to 2000: Bundesministerium für Bildung, Wissenschaft, Forschung und Technologie by grant number 01 KW 9611

Project Members:

• Bastien Chevreux (admin)