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A universal method for the rapid isolation of all known classes of functional silencing small RNAs

Diverse classes of silencing small (s)RNAs operate via ARGONAUTE-family proteins within RNA-induced-silencing-complexes (RISCs). Here, we have streamlined various embodiments of a Q-sepharose-based RISC-purification method that relies on conserved biochemical properties of all ARGONAUTEs. We show, i...

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Autores principales: Grentzinger, Thomas, Oberlin, Stefan, Schott, Gregory, Handler, Dominik, Svozil, Julia, Barragan-Borrero, Veronica, Humbert, Adeline, Duharcourt, Sandra, Brennecke, Julius, Voinnet, Olivier
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Oxford University Press 2020
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7641303/
https://www.ncbi.nlm.nih.gov/pubmed/32496553
http://dx.doi.org/10.1093/nar/gkaa472
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author Grentzinger, Thomas
Oberlin, Stefan
Schott, Gregory
Handler, Dominik
Svozil, Julia
Barragan-Borrero, Veronica
Humbert, Adeline
Duharcourt, Sandra
Brennecke, Julius
Voinnet, Olivier
author_facet Grentzinger, Thomas
Oberlin, Stefan
Schott, Gregory
Handler, Dominik
Svozil, Julia
Barragan-Borrero, Veronica
Humbert, Adeline
Duharcourt, Sandra
Brennecke, Julius
Voinnet, Olivier
author_sort Grentzinger, Thomas
collection PubMed
description Diverse classes of silencing small (s)RNAs operate via ARGONAUTE-family proteins within RNA-induced-silencing-complexes (RISCs). Here, we have streamlined various embodiments of a Q-sepharose-based RISC-purification method that relies on conserved biochemical properties of all ARGONAUTEs. We show, in multiple benchmarking assays, that the resulting 15-min benchtop extraction procedure allows simultaneous purification of all known classes of RISC-associated sRNAs without prior knowledge of the samples-intrinsic ARGONAUTE repertoires. Optimized under a user-friendly format, the method – coined ‘TraPR’ for Trans-kingdom, rapid, affordable Purification of RISCs – operates irrespectively of the organism, tissue, cell type or bio-fluid of interest, and scales to minute amounts of input material. The method is highly suited for direct profiling of silencing sRNAs, with TraPR-generated sequencing libraries outperforming those obtained via gold-standard procedures that require immunoprecipitations and/or lengthy polyacrylamide gel-selection. TraPR considerably improves the quality and consistency of silencing sRNA sample preparation including from notoriously difficult-to-handle tissues/bio-fluids such as starchy storage roots or mammalian plasma, and regardless of RNA contaminants or RNA degradation status of samples.
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spelling pubmed-76413032020-11-10 A universal method for the rapid isolation of all known classes of functional silencing small RNAs Grentzinger, Thomas Oberlin, Stefan Schott, Gregory Handler, Dominik Svozil, Julia Barragan-Borrero, Veronica Humbert, Adeline Duharcourt, Sandra Brennecke, Julius Voinnet, Olivier Nucleic Acids Res Methods Online Diverse classes of silencing small (s)RNAs operate via ARGONAUTE-family proteins within RNA-induced-silencing-complexes (RISCs). Here, we have streamlined various embodiments of a Q-sepharose-based RISC-purification method that relies on conserved biochemical properties of all ARGONAUTEs. We show, in multiple benchmarking assays, that the resulting 15-min benchtop extraction procedure allows simultaneous purification of all known classes of RISC-associated sRNAs without prior knowledge of the samples-intrinsic ARGONAUTE repertoires. Optimized under a user-friendly format, the method – coined ‘TraPR’ for Trans-kingdom, rapid, affordable Purification of RISCs – operates irrespectively of the organism, tissue, cell type or bio-fluid of interest, and scales to minute amounts of input material. The method is highly suited for direct profiling of silencing sRNAs, with TraPR-generated sequencing libraries outperforming those obtained via gold-standard procedures that require immunoprecipitations and/or lengthy polyacrylamide gel-selection. TraPR considerably improves the quality and consistency of silencing sRNA sample preparation including from notoriously difficult-to-handle tissues/bio-fluids such as starchy storage roots or mammalian plasma, and regardless of RNA contaminants or RNA degradation status of samples. Oxford University Press 2020-06-04 /pmc/articles/PMC7641303/ /pubmed/32496553 http://dx.doi.org/10.1093/nar/gkaa472 Text en © The Author(s) 2020. Published by Oxford University Press on behalf of Nucleic Acids Research. http://creativecommons.org/licenses/by-nc/4.0/ This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/4.0/), which permits non-commercial re-use, distribution, and reproduction in any medium, provided the original work is properly cited. For commercial re-use, please contact journals.permissions@oup.com
spellingShingle Methods Online
Grentzinger, Thomas
Oberlin, Stefan
Schott, Gregory
Handler, Dominik
Svozil, Julia
Barragan-Borrero, Veronica
Humbert, Adeline
Duharcourt, Sandra
Brennecke, Julius
Voinnet, Olivier
A universal method for the rapid isolation of all known classes of functional silencing small RNAs
title A universal method for the rapid isolation of all known classes of functional silencing small RNAs
title_full A universal method for the rapid isolation of all known classes of functional silencing small RNAs
title_fullStr A universal method for the rapid isolation of all known classes of functional silencing small RNAs
title_full_unstemmed A universal method for the rapid isolation of all known classes of functional silencing small RNAs
title_short A universal method for the rapid isolation of all known classes of functional silencing small RNAs
title_sort universal method for the rapid isolation of all known classes of functional silencing small rnas
topic Methods Online
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7641303/
https://www.ncbi.nlm.nih.gov/pubmed/32496553
http://dx.doi.org/10.1093/nar/gkaa472
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