Nicking loop™ / Technology
Circular sequencing by Geno1® technologies
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PCR-free DNA amplification
Nicking Loop™ enables direct linear amplification of circular ssDNA libraries, eliminating biases and pitfalls associated with PCR amplification.
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High-fidelity queries and copies
Nicking Loop™ transforms DNA libraries into structured databases, enabling efficient operations like data copying and advanced querying.
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Platform-agnostic sequencing
Circular Nicking Loop™ libraries are compatible with any sequencing platform. Libraries can be sequenced directly in their circular form or converted into linear libraries to fit seamlessly with any workflow.
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Designed for simplicity, evenness and uniformity
Nicking Loop™ provides a simple and robust process that minimizes errors while delivering highly even and uniform data for exceptional accuracy and consistency.
Nicking Loop™ copying – PCR-free DNA amplification
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Nicking Loop™ copying is a PCR-free amplification method for circular DNA, suited for high-fidelity information read-out and database-like operations.
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01
A loop-specific oligonucleotide is annealed with the Nicking Loop™-converted DNA.
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02
Rolling circle amplification is primed to create concatemeric copies of the circular DNA.
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03
The looped part of the concatemer is cleaved, resulting in monomerization of the concatemer.
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04
The monomers are self-circularized to result in amplified circular DNA.
Nicking Loop™ DNA conversion & indexing
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In Nicking Loop conversion, a looped index oligo complex is ligated to DNA molecules, enabling their circularization
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01
Y-adapters are ligated to end-repaired DNA.
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02
The looped index is brought into contact with the Y-adapted-ligated DNA using a supporting oligo.
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03
The supporting oligo is allowed to anneal to the Y-adapter ends.
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04
The looped index is ligated to the Y-adapter ends.
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05
The supporting oligo is removed, resulting in Nicking Loop™-converted DNA molecules.
NICKING LOOP™
How does it perform?
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Patents
Methods for accurate parallel detection and quantification of nucleic acids
Highly sensitive methods for accurate parallel quantification of nucleic acids
Methods for accurate parallel quantification of nucleic acids in dilute or non-purified samples
Accurate and massively parallel quantification of nucleic acid