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How nanopore sequencing works

Oxford Nanopore has developed a new generation of DNA/RNA sequencing technology. It is the only sequencing technology that offers real-time analysis (for rapid insights), in fully scalable formats from pocket to population scale, that can analyse native DNA or RNA and sequence any length of fragment to achieve short to ultra-long read lengths.

Real-time

The only sequencing technology that offers real-time analysis

Fully scalable

From pocket to population-scale devices

Direct DNA/RNA sequencing

Call base modifications simultaneously with nucleotide sequence

Ultra-long reads

Improve assembly and characterise repetitive and difficult regions with ultra-long reads

Sequence anywhere

MinION is being used outside the traditional lab environment — taking the analysis to the sample.

Nanopores

All Oxford Nanopore sequencing devices use flow cells which contain an array of tiny holes — nanopores — embedded in an electro-resistant membrane. Each nanopore corresponds to its own electrode connected to a channel and sensor chip, which measures the electric current that flows through the nanopore. When a molecule passes through a nanopore, the current is disrupted to produce a characteristic ‘squiggle’. The squiggle is then decoded using basecalling algorithms to determine the DNA or RNA sequence in real time.

Learn more about flow cells and nanopores

   

Learn how basecalling works
Basecalling

You can think of the current as water flowing through a pipe. When an object enters the pipe, the flow of water is disrupted, just as DNA disrupts the current as it passes through the nanopore.

nanopore

DNA/RNA sequencing

A strand of DNA or RNA is made up of a sequence of different combinations of four nucleotide bases: A, T (or U for RNA), G and C. Each base that passes through the nanopore can be identified through the characteristic disruption it causes to the current in real-time. This makes nanopore sequencing unique, in that it is the only sequencing technology that enables direct, real-time analysis of short to ultra-long fragments of DNA/RNA, in fully scalable formats. Advantages of real-time sequencing include rapid access to time critical information (e.g. pathogen identification), the generation of early sample insights and more control over the sequencing experiment.

 

Learn more about the advantages of real-time sequencing

Why DNA / RNA?

DNA and RNA are molecules that are present in all living things. DNA is the genetic code of life, the instructions for building and operating an organism. RNA is primarily a messenger molecule, carrying instructions from the DNA code to control the synthesis of proteins — the building blocks of organisms. Sequencing can answer a range of biological questions, providing information on pathogen identity, genetic disease risk or how an organism has evolved.

 

Learn about the applications of nanopore sequencing
DNA Sequencing

You can think of sequencing DNA/RNA like reading music — the bases being the notes, which when played in the correct order, produces a recognisable the song. Nanopore sequencing is used to determine the sequence of DNA/RNA bases.

the power of long reads

You can think of this like trying to complete two jigsaws of the same photograph — one with significantly larger pieces than the other. A jigsaw with only 9 pieces is much easier to assemble than one with 900.

The power of long reads

Traditional methods are only able to sequence short lengths of DNA which must then be reassembled. It is therefore difficult to sequence repetitive regions for accurate genome assemblies without gaps, resolve large structural variations, or differentiate isoforms. Nanopore sequencing is limited only by the length of the DNA/RNA fragment presented to the pore and can therefore span entire repetitive regions, resolve structural variants, and differentiate between different isoforms. The ability to sequence native DNA and RNA without the requirement for amplification, eliminates PCR bias and allows for the identification of base modifications, such as methylation, alongside nucleotide sequence.

Learn more about the advantages of nanopore sequencing

Nanopore sequencing is fully scalable

Nanopore sequencing is the only sequencing technology to enable real-time analysis in fully scalable formats. From the pocket-sized MinION to the high-throughput, population-scale PromethION — scale nanopore sequencing to suit any experimental needs.

PromethION 48

PromethION 48

Flexible, population-scale sequencing using up to 48 independent, high-capacity flow cells — complete genomic and transcriptomic characterisation of large sample numbers.

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PromethION 24

PromethION 24

Combining up to 24 independently addressable, high-capacity flow cells with powerful, integrated compute, PromethION 24 delivers flexible, on-demand access to terabases of sequencing data — ideal for cost-effective, high-throughput sequencing.

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PromethION 2 & 2 Solo

PromethION 2 & 2 Solo

Flexible, high-yield nanopore sequencing for every lab. The PromethION 2 devices are designed to be compact and accessible, utilising 2 PromethION Flow Cells that can generate hundreds of gigabases of data each.

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GridION

GridION

From genome assembly to gene expression, run multiple experiments on-demand using 5 independent MinION flow cells.

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MinION

MinION

Integrated sequencing and analysis in a powerful handheld device — suitable for small animal genomes, targeted sequencing, and gene expression studies.

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Flongle

Flongle

Adapting MinION and GridION for smaller, routine tests and analyses. Low plex targeted sequencing, RNA isoform analysis, and quality control applications.

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VolTRAX

VolTRAX

Automated library preparation for nanopore sequencing.

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