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Addressing the challenges of symbiont-mediated RNAi in aphids

Because aphids are global agricultural pests and models for bacterial endosymbiosis, there is a need for reliable methods to study and control their gene function. However, current methods available for aphid gene knockout and knockdown of gene expression are often unreliable and time consuming. Tec...

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Autores principales: Elston, Katherine M., Maeda, Gerald P., Perreau, Julie, Barrick, Jeffrey E.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: PeerJ Inc. 2023
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9983426/
https://www.ncbi.nlm.nih.gov/pubmed/36874963
http://dx.doi.org/10.7717/peerj.14961
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author Elston, Katherine M.
Maeda, Gerald P.
Perreau, Julie
Barrick, Jeffrey E.
author_facet Elston, Katherine M.
Maeda, Gerald P.
Perreau, Julie
Barrick, Jeffrey E.
author_sort Elston, Katherine M.
collection PubMed
description Because aphids are global agricultural pests and models for bacterial endosymbiosis, there is a need for reliable methods to study and control their gene function. However, current methods available for aphid gene knockout and knockdown of gene expression are often unreliable and time consuming. Techniques like CRISPR-Cas genome editing can take several months to achieve a single gene knockout because they rely on aphids going through a cycle of sexual reproduction, and aphids often lack strong, consistent levels of knockdown when fed or injected with molecules that induce an RNA interference (RNAi) response. In the hopes of addressing these challenges, we attempted to adapt a new method called symbiont-mediated RNAi (smRNAi) for use in aphids. smRNAi involves engineering a bacterial symbiont of the insect to continuously supply double-stranded RNA (dsRNA) inside the insect body. This approach has been successful in thrips, kissing bugs, and honeybees. We engineered the laboratory Escherichia coli strain HT115 and the native aphid symbiont Serratia symbiotica CWBI-2.3(T) to produce dsRNA inside the gut of the pea aphid (Acyrthosiphon pisum) targeting salivary effector protein (C002) or ecdysone receptor genes. For C002 assays, we also tested co-knockdown with an aphid nuclease (Nuc1) to reduce RNA degradation. However, we found that smRNAi was not a reliable method for aphid gene knockdown under our conditions. We were unable to consistently achieve the expected phenotypic changes with either target. However, we did see indications that elements of the RNAi pathway were modestly upregulated, and expression of some targeted genes appeared to be somewhat reduced in some trials. We conclude with a discussion of the possible avenues through which smRNAi, and aphid RNAi in general, could be improved in the future.
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spelling pubmed-99834262023-03-04 Addressing the challenges of symbiont-mediated RNAi in aphids Elston, Katherine M. Maeda, Gerald P. Perreau, Julie Barrick, Jeffrey E. PeerJ Agricultural Science Because aphids are global agricultural pests and models for bacterial endosymbiosis, there is a need for reliable methods to study and control their gene function. However, current methods available for aphid gene knockout and knockdown of gene expression are often unreliable and time consuming. Techniques like CRISPR-Cas genome editing can take several months to achieve a single gene knockout because they rely on aphids going through a cycle of sexual reproduction, and aphids often lack strong, consistent levels of knockdown when fed or injected with molecules that induce an RNA interference (RNAi) response. In the hopes of addressing these challenges, we attempted to adapt a new method called symbiont-mediated RNAi (smRNAi) for use in aphids. smRNAi involves engineering a bacterial symbiont of the insect to continuously supply double-stranded RNA (dsRNA) inside the insect body. This approach has been successful in thrips, kissing bugs, and honeybees. We engineered the laboratory Escherichia coli strain HT115 and the native aphid symbiont Serratia symbiotica CWBI-2.3(T) to produce dsRNA inside the gut of the pea aphid (Acyrthosiphon pisum) targeting salivary effector protein (C002) or ecdysone receptor genes. For C002 assays, we also tested co-knockdown with an aphid nuclease (Nuc1) to reduce RNA degradation. However, we found that smRNAi was not a reliable method for aphid gene knockdown under our conditions. We were unable to consistently achieve the expected phenotypic changes with either target. However, we did see indications that elements of the RNAi pathway were modestly upregulated, and expression of some targeted genes appeared to be somewhat reduced in some trials. We conclude with a discussion of the possible avenues through which smRNAi, and aphid RNAi in general, could be improved in the future. PeerJ Inc. 2023-02-28 /pmc/articles/PMC9983426/ /pubmed/36874963 http://dx.doi.org/10.7717/peerj.14961 Text en © 2023 Elston et al. https://creativecommons.org/licenses/by/4.0/This is an open access article distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, reproduction and adaptation in any medium and for any purpose provided that it is properly attributed. For attribution, the original author(s), title, publication source (PeerJ) and either DOI or URL of the article must be cited.
spellingShingle Agricultural Science
Elston, Katherine M.
Maeda, Gerald P.
Perreau, Julie
Barrick, Jeffrey E.
Addressing the challenges of symbiont-mediated RNAi in aphids
title Addressing the challenges of symbiont-mediated RNAi in aphids
title_full Addressing the challenges of symbiont-mediated RNAi in aphids
title_fullStr Addressing the challenges of symbiont-mediated RNAi in aphids
title_full_unstemmed Addressing the challenges of symbiont-mediated RNAi in aphids
title_short Addressing the challenges of symbiont-mediated RNAi in aphids
title_sort addressing the challenges of symbiont-mediated rnai in aphids
topic Agricultural Science
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9983426/
https://www.ncbi.nlm.nih.gov/pubmed/36874963
http://dx.doi.org/10.7717/peerj.14961
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