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Multiplexed long-read plasmid validation and analysis using OnRamp

Recombinant plasmid vectors are versatile tools that have facilitated discoveries in molecular biology, genetics, proteomics, and many other fields. As the enzymatic and bacterial processes used to create recombinant DNA can introduce errors, sequence validation is an essential step in plasmid assem...

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Detalles Bibliográficos
Autores principales: Mumm, Camille, Drexel, Melissa L., McDonald, Torrin L., Diehl, Adam G., Switzenberg, Jessica A., Boyle, Alan P.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Cold Spring Harbor Laboratory Press 2023
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10317119/
https://www.ncbi.nlm.nih.gov/pubmed/37156622
http://dx.doi.org/10.1101/gr.277369.122
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author Mumm, Camille
Drexel, Melissa L.
McDonald, Torrin L.
Diehl, Adam G.
Switzenberg, Jessica A.
Boyle, Alan P.
author_facet Mumm, Camille
Drexel, Melissa L.
McDonald, Torrin L.
Diehl, Adam G.
Switzenberg, Jessica A.
Boyle, Alan P.
author_sort Mumm, Camille
collection PubMed
description Recombinant plasmid vectors are versatile tools that have facilitated discoveries in molecular biology, genetics, proteomics, and many other fields. As the enzymatic and bacterial processes used to create recombinant DNA can introduce errors, sequence validation is an essential step in plasmid assembly. Sanger sequencing is the current standard for plasmid validation; however, this method is limited by an inability to sequence through complex secondary structure and lacks scalability when applied to full-plasmid sequencing of multiple plasmids owing to read-length limits. Although high-throughput sequencing does provide full-plasmid sequencing at scale, it is impractical and costly when used outside of library-scale validation. Here, we present Oxford nanopore-based rapid analysis of multiplexed plasmids (OnRamp), an alternative method for routine plasmid validation that combines the advantages of high-throughput sequencing's full-plasmid coverage and scalability with Sanger's affordability and accessibility by leveraging nanopore's long-read sequencing technology. We include customized wet-laboratory protocols for plasmid preparation along with a pipeline designed for analysis of read data obtained using these protocols. This analysis pipeline is deployed on the OnRamp web app, which generates alignments between actual and predicted plasmid sequences, quality scores, and read-level views. OnRamp is designed to be broadly accessible regardless of programming experience to facilitate more widespread adoption of long-read sequencing for routine plasmid validation. Here we describe the OnRamp protocols and pipeline and show our ability to obtain full sequences from pooled plasmids while detecting sequence variation even in regions of high secondary structure at less than half the cost of equivalent Sanger sequencing.
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spelling pubmed-103171192023-07-04 Multiplexed long-read plasmid validation and analysis using OnRamp Mumm, Camille Drexel, Melissa L. McDonald, Torrin L. Diehl, Adam G. Switzenberg, Jessica A. Boyle, Alan P. Genome Res Methods Recombinant plasmid vectors are versatile tools that have facilitated discoveries in molecular biology, genetics, proteomics, and many other fields. As the enzymatic and bacterial processes used to create recombinant DNA can introduce errors, sequence validation is an essential step in plasmid assembly. Sanger sequencing is the current standard for plasmid validation; however, this method is limited by an inability to sequence through complex secondary structure and lacks scalability when applied to full-plasmid sequencing of multiple plasmids owing to read-length limits. Although high-throughput sequencing does provide full-plasmid sequencing at scale, it is impractical and costly when used outside of library-scale validation. Here, we present Oxford nanopore-based rapid analysis of multiplexed plasmids (OnRamp), an alternative method for routine plasmid validation that combines the advantages of high-throughput sequencing's full-plasmid coverage and scalability with Sanger's affordability and accessibility by leveraging nanopore's long-read sequencing technology. We include customized wet-laboratory protocols for plasmid preparation along with a pipeline designed for analysis of read data obtained using these protocols. This analysis pipeline is deployed on the OnRamp web app, which generates alignments between actual and predicted plasmid sequences, quality scores, and read-level views. OnRamp is designed to be broadly accessible regardless of programming experience to facilitate more widespread adoption of long-read sequencing for routine plasmid validation. Here we describe the OnRamp protocols and pipeline and show our ability to obtain full sequences from pooled plasmids while detecting sequence variation even in regions of high secondary structure at less than half the cost of equivalent Sanger sequencing. Cold Spring Harbor Laboratory Press 2023-05 /pmc/articles/PMC10317119/ /pubmed/37156622 http://dx.doi.org/10.1101/gr.277369.122 Text en © 2023 Mumm et al.; Published by Cold Spring Harbor Laboratory Press https://creativecommons.org/licenses/by/4.0/This article, published in Genome Research, is available under a Creative Commons License (Attribution 4.0 International), as described at http://creativecommons.org/licenses/by/4.0/ (https://creativecommons.org/licenses/by/4.0/) .
spellingShingle Methods
Mumm, Camille
Drexel, Melissa L.
McDonald, Torrin L.
Diehl, Adam G.
Switzenberg, Jessica A.
Boyle, Alan P.
Multiplexed long-read plasmid validation and analysis using OnRamp
title Multiplexed long-read plasmid validation and analysis using OnRamp
title_full Multiplexed long-read plasmid validation and analysis using OnRamp
title_fullStr Multiplexed long-read plasmid validation and analysis using OnRamp
title_full_unstemmed Multiplexed long-read plasmid validation and analysis using OnRamp
title_short Multiplexed long-read plasmid validation and analysis using OnRamp
title_sort multiplexed long-read plasmid validation and analysis using onramp
topic Methods
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10317119/
https://www.ncbi.nlm.nih.gov/pubmed/37156622
http://dx.doi.org/10.1101/gr.277369.122
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