A complete bacterial genome assembled de novo using only nanopore sequencing data

A method for de novo assembly of data from the Oxford Nanopore MinION instrument is presented which is able to reconstruct the sequence of an entire bacterial chromosome in a single contig. Initially, overlaps between nanopore reads are detected. Reads are then subjected to one or more rounds of error correction by a multiple alignment process employing partial order graphs. After correction, reads are assembled using the Celera assembler. Finally, the assembly is polished using signal-level data from the nanopore employing a novel hidden Markov model. We show that this method is able to assemble nanopore reads from Escherichia coli K-12 MG1655 into a single contig of length 4.6Mb permitting a full reconstruction of gene order. The resulting draft assembly has 98.4% nucleotide identity compared to the finished reference genome. After polishing the assembly with our signal-level HMM, the nucleotide identity is improved to 99.4%. We show that MinION sequencing data can be used to reconstruct genomes without the need for a reference sequence or data from other sequencing platforms.

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Evaluation of hybrid and non-hybrid methods for de novo assembly of nanopore reads

10.1101/030437 ◽

2015 ◽

Cited By ~ 3

Author(s):

Ivan Sovic ◽

Kresimir Krizanovic ◽

Karolj Skala ◽

Mile Sikic

Keyword(s):

De Novo Assembly ◽

De Novo ◽

Hybrid Methods ◽

Bacterial Genome ◽

Error Rates ◽

Sequencing Data ◽

E Coli ◽

Recent Emergence ◽

K 12

Recent emergence of nanopore sequencing technology set a challenge for the established assembly methods not optimized for the combination of read lengths and high error rates of nanopore reads. In this work we assessed how existing de novo assembly methods perform on these reads. We benchmarked three non-hybrid (in terms of both error correction and scaffolding) assembly pipelines as well as two hybrid assemblers which use third generation sequencing data to scaffold Illumina assemblies. Tests were performed on several publicly available MinION and Illumina datasets of E. coli K-12, using several sequencing coverages of nanopore data (20x, 30x, 40x and 50x). We attempted to assess the quality of assembly at each of these coverages, to estimate the requirements for closed bacterial genome assembly. Results show that hybrid methods are highly dependent on the quality of NGS data, but much less on the quality and coverage of nanopore data and perform relatively well on lower nanopore coverages. Furthermore, when coverage is above 40x, all non-hybrid methods correctly assemble the E. coli genome, even a non-hybrid method tailored for Pacific Bioscience reads. While it requires higher coverage compared to a method designed particularly for nanopore reads, its running time is significantly lower.

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A complete bacterial genome assembled de novo using only nanopore sequencing data

Nature Methods ◽

10.1038/nmeth.3444 ◽

2015 ◽

Vol 12 (8) ◽

pp. 733-735 ◽

Cited By ~ 592

Author(s):

Nicholas J Loman ◽

Joshua Quick ◽

Jared T Simpson

Keyword(s):

De Novo ◽

Bacterial Genome ◽

Nanopore Sequencing ◽

Sequencing Data ◽

Complete Bacterial Genome

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Implications of Genetic Distance to Reference and De Novo Genome Assembly for Clinical Genomics in Africans

10.1101/2020.09.25.20201780 ◽

2020 ◽

Author(s):

Daniel Shriner ◽

Adebowale Adeyemo ◽

Charles Rotimi

Keyword(s):

Genetic Distance ◽

De Novo ◽

Reference Sequence ◽

Sequencing Data ◽

Single Nucleotide Variants ◽

De Novo Genome Assembly ◽

Single Nucleotide ◽

Clinical Genomics ◽

Advantages And Disadvantages ◽

False Discovery

In clinical genomics, variant calling from short-read sequencing data typically relies on a pan-genomic, universal human reference sequence. A major limitation of this approach is that the number of reads that incorrectly map or fail to map increase as the reads diverge from the reference sequence. In the context of genome sequencing of genetically diverse Africans, we investigate the advantages and disadvantages of using a de novo assembly of the read data as the reference sequence in single sample calling. Conditional on sufficient read depth, the alignment-based and assembly-based approaches yielded comparable sensitivity and false discovery rates for single nucleotide variants when benchmarked against a gold standard call set. The alignment-based approach yielded coverage of an additional 270.8 Mb over which sensitivity was lower and the false discovery rate was higher. Although both approaches detected and missed clinically relevant variants, the assembly-based approach identified more such variants than the alignment-based approach. Of particular relevance to individuals of African descent, the assembly-based approach identified four heterozygous genotypes containing the sickle allele whereas the alignment-based approach identified no occurrences of the sickle allele. Variant annotation using dbSNP and gnomAD identified systematic biases in these databases due to underrepresentation of Africans. Using the counts of homozygous alternate genotypes from the alignment-based approach as a measure of genetic distance to the reference sequence GRCh38.p12, we found that the numbers of misassemblies, total variant sites, potentially novel single nucleotide variants (SNVs), and certain variant classes (e.g., splice acceptor variants, stop loss variants, missense variants, synonymous variants, and variants absent from gnomAD) were significantly correlated with genetic distance. In contrast, genomic coverage and other variant classes (e.g., ClinVar pathogenic or likely pathogenic variants, start loss variants, stop gain variants, splice donor variants, incomplete terminal codons, variants with CADD score ≥20) were not correlated with genetic distance. With improvement in coverage, the assembly-based approach can offer a viable alternative to the alignment-based approach, with the advantage that it can obviate the need to generate diverse human reference sequences or collections of alternate scaffolds.

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NanoGalaxy: Nanopore long-read sequencing data analysis in Galaxy

GigaScience ◽

10.1093/gigascience/giaa105 ◽

2020 ◽

Vol 9 (10) ◽

Cited By ~ 1

Author(s):

Willem de Koning ◽

Milad Miladi ◽

Saskia Hiltemann ◽

Astrid Heikema ◽

John P Hays ◽

...

Keyword(s):

Genome Assembly ◽

Bioinformatics Analysis ◽

De Novo ◽

Sequence Data ◽

Ease Of Use ◽

Easy Access ◽

Complex Data ◽

Sequencing Data ◽

Long Read ◽

Sequencing Platforms

Abstract Background Long-read sequencing can be applied to generate very long contigs and even completely assembled genomes at relatively low cost and with minimal sample preparation. As a result, long-read sequencing platforms are becoming more popular. In this respect, the Oxford Nanopore Technologies–based long-read sequencing “nanopore" platform is becoming a widely used tool with a broad range of applications and end-users. However, the need to explore and manipulate the complex data generated by long-read sequencing platforms necessitates accompanying specialized bioinformatics platforms and tools to process the long-read data correctly. Importantly, such tools should additionally help democratize bioinformatics analysis by enabling easy access and ease-of-use solutions for researchers. Results The Galaxy platform provides a user-friendly interface to computational command line–based tools, handles the software dependencies, and provides refined workflows. The users do not have to possess programming experience or extended computer skills. The interface enables researchers to perform powerful bioinformatics analysis, including the assembly and analysis of short- or long-read sequence data. The newly developed “NanoGalaxy" is a Galaxy-based toolkit for analysing long-read sequencing data, which is suitable for diverse applications, including de novo genome assembly from genomic, metagenomic, and plasmid sequence reads. Conclusions A range of best-practice tools and workflows for long-read sequence genome assembly has been integrated into a NanoGalaxy platform to facilitate easy access and use of bioinformatics tools for researchers. NanoGalaxy is freely available at the European Galaxy server https://nanopore.usegalaxy.eu with supporting self-learning training material available at https://training.galaxyproject.org.

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Toward Complete Bacterial Genome Sequencing Through the Combined Use of Multiple Next-Generation Sequencing Platforms

Journal of Microbiology and Biotechnology ◽

10.4014/jmb.1507.07055 ◽

2016 ◽

Vol 26 (1) ◽

pp. 207-212 ◽

Cited By ~ 6

Author(s):

Haeyoung Jeong ◽

Dae-Hee Lee ◽

Choong-Min Ryu ◽

Seung-Hwan Park

Keyword(s):

Next Generation Sequencing ◽

Genome Sequencing ◽

Bacterial Genome ◽

Next Generation ◽

Combined Use ◽

Complete Bacterial Genome ◽

Sequencing Platforms ◽

Bacterial Genome Sequencing ◽

Generation Sequencing

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A reference bacterial genome dataset generated on the MinION™ portable single-molecule nanopore sequencer

10.1101/009613 ◽

2014 ◽

Author(s):

Josh Quick ◽

Aaron Quinlan ◽

Nicholas Loman

Keyword(s):

Single Molecule ◽

De Novo ◽

Sequence Data ◽

Bacterial Genome ◽

Model Organism ◽

Variant Calling ◽

Laptop Computer ◽

Early Access ◽

Dna Strands ◽

K 12

Background: The MinION™ is a new, portable single-molecule sequencer developed by Oxford Nanopore Technologies. It measures four inches in length and is powered from the USB 3.0 port of a laptop computer. By measuring the change in current produced when DNA strands translocate through and interact with a charged protein nanopore the device is able to deduce the underlying nucleotide sequence. Findings: We present a read dataset from whole-genome shotgun sequencing of the model organism Escherichia coli K-12 substr. MG1655 generated on a MinION™ device during the early-access MinION Access Program (MAP). Sequencing runs of the MinION™ are presented, one generated using R7 chemistry (released in July 2014) and one using R7.3 (released in September 2014). Conclusions: Base-called sequence data are provided to demonstrate the nature of data produced by the MinION™ platform and to encourage the development of customised methods for alignment, consensus and variant calling, de novo assembly and scaffolding. FAST5 files containing event data within the HDF5 container format are provided to assist with the development of improved base-calling methods. Datasets are provided through the GigaDB database at http://gigadb.org/dataset/100102

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gapFinisher: a reliable gap filling pipeline for SSPACE-LongRead scaffolder output

10.7287/peerj.preprints.3467 ◽

2017 ◽

Author(s):

Juhana I Kammonen ◽

Olli-Pekka Smolander ◽

Lars Paulin ◽

Pedro AB Pereira ◽

Pia Laine ◽

...

Keyword(s):

De Novo ◽

Draft Genome ◽

Sequence Information ◽

Sequencing Data ◽

Gap Filling ◽

Third Generation Sequencing ◽

Long Reads ◽

Unix Command ◽

Sequencing Platforms ◽

Scaffolding Software

Unknown sequences, or gaps, are largely present in most published genomes across public databases. Gap filling is an important finishing step in de novo genome assembly, especially in large genomes. The gap filling problem is nontrivial and while many computational tools exist partially solving the problem, several have shortcomings as to the reliability and correctness of the output, i.e. the gap filled draft genome. SSPACE-LongRead is a scaffolding software that utilizes long reads from multiple third-generation sequencing platforms in finding links between contigs and combining them. The long reads potentially contain sequence information to fill the gaps, but SSPACE-LongRead currently lacks this functionality. We present an automated pipeline called gapFinisher to process SSPACE-LongRead output to fill gaps after the actual scaffolding. gapFinisher is based on controlled use of a gap filling tool called FGAP and works on all standard Linux/UNIX command lines. We conclude that performing the workflows of SSPACE-LongRead and gapFinisher enables users to fill gaps reliably. There is no need for further scrutiny of the existing sequencing data after performing the analysis.

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NxRepair: Error correction in de novo sequence assembly using Nextera mate pairs

10.7287/peerj.preprints.747v1 ◽

2014 ◽

Author(s):

Rebecca R Murphy ◽

Jared M O'Connell ◽

Anthony J Cox ◽

Ole B Schulz-Trieglaff

Keyword(s):

Error Correction ◽

Large Scale ◽

De Novo ◽

Reference Sequence ◽

De Bruijn Graph ◽

Sequencing Data ◽

Additional Information ◽

Mate Pair ◽

De Bruijn ◽

De Novo Sequence Assembly

Scaffolding errors and incorrect traversals of the de Bruijn graph during de novo assembly can result in large scale misassemblies in draft genomes. Nextera mate pair sequencing data provide additional information to resolve assembly ambiguities during scaffolding. Here, we introduce NxRepair, an open source toolkit for error correction in de novo assemblies that uses Nextera mate pair libraries to identify and correct large-scale errors. We show that NxRepair can identify and correct large scaffolding errors, without use of a reference sequence, resulting in quantitative improvements in the assembly quality. NxRepair can be downloaded from GitHub; a tutorial and user documentation are also available.

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Assembly methods for nanopore-based metagenomic sequencing: a comparative study

10.1101/722405 ◽

2019 ◽

Cited By ~ 1

Author(s):

Adriel Latorre-Pérez ◽

Pascual Villalba-Bermell ◽

Javier Pascual ◽

Manuel Porcar ◽

Cristina Vilanova

Keyword(s):

Bacterial Genome ◽

Gene Clusters ◽

Systematic Evaluation ◽

Metagenomic Sequencing ◽

Sequencing Data ◽

Short Reads ◽

Sequencing Technologies ◽

Long Reads ◽

Oxford Nanopore ◽

Sequencing Platforms

ABSTRACTBackgroundMetagenomic sequencing has lead to the recovery of previously unexplored microbial genomes. In this sense, short-reads sequencing platforms often result in highly fragmented metagenomes, thus complicating downstream analyses. Third generation sequencing technologies, such as MinION, could lead to more contiguous assemblies due to their ability to generate long reads. Nevertheless, there is a lack of studies evaluating the suitability of the available assembly tools for this new type of data.FindingsWe benchmarked the ability of different short-reads and long-reads tools to assembly two different commercially available mock communities, and observed remarkable differences in the resulting assemblies depending on the software of choice. Short-reads metagenomic assemblers proved unsuitable for MinION data. Among the long-reads assemblers tested, Flye and Canu were the only ones performing well in all the datasets. These tools were able to retrieve complete individual genomes directly from the metagenome, and assembled a bacterial genome in only two contigs in the best scenario. Despite the intrinsic high error of long-reads technologies, Canu and Flye lead to high accurate assemblies (~99.4-99.8 % of accuracy). However, errors still had an impact on the prediction of biosynthetic gene clusters.ConclusionsMinION metagenomic sequencing data proved sufficient for assembling low-complex microbial communities, leading to the recovery of highly complete and contiguous individual genomes. This work is the first systematic evaluation of the performance of different assembly tools on MinION data, and may help other researchers willing to use this technology to choose the most appropriate software depending on their goals. Future work is still needed in order to assess the performance of Oxford Nanopore MinION data on more complex microbiomes.

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