Tissue- and time-directed electroporation of CAS9 protein–gRNA complexes in vivo yields efficient multigene knockout for studying gene function in regeneration

A rapid method for temporally and spatially controlled CRISPR-mediated gene knockout in vertebrates will be an important tool to screen for genes involved in complex biological phenomena like regeneration. Here we show that in vivo injection of CAS9 protein–guide RNA (gRNA) complexes into the spinal...

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Autores principales: Fei, Ji-Feng, Knapp, Dunja, Schuez, Maritta, Murawala, Prayag, Zou, Yan, Pal Singh, Sumeet, Drechsel, David, Tanaka, Elly M
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Nature Publishing Group 2016
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Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5744710/
https://www.ncbi.nlm.nih.gov/pubmed/29302334
http://dx.doi.org/10.1038/npjregenmed.2016.2
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author Fei, Ji-Feng
Knapp, Dunja
Schuez, Maritta
Murawala, Prayag
Zou, Yan
Pal Singh, Sumeet
Drechsel, David
Tanaka, Elly M
author_facet Fei, Ji-Feng
Knapp, Dunja
Schuez, Maritta
Murawala, Prayag
Zou, Yan
Pal Singh, Sumeet
Drechsel, David
Tanaka, Elly M
author_sort Fei, Ji-Feng
collection PubMed
description A rapid method for temporally and spatially controlled CRISPR-mediated gene knockout in vertebrates will be an important tool to screen for genes involved in complex biological phenomena like regeneration. Here we show that in vivo injection of CAS9 protein–guide RNA (gRNA) complexes into the spinal cord lumen of the axolotl and subsequent electroporation leads to comprehensive knockout of Sox2 gene expression in SOX2(+) neural stem cells with corresponding functional phenotypes from the gene knockout. This is particularly surprising considering the known prevalence of RNase activity in cerebral spinal fluid, which apparently the CAS9 protein protects against. The penetrance/efficiency of gene knockout in the protein-based system is far higher than corresponding electroporation of plasmid-based CRISPR systems. We further show that simultaneous delivery of CAS9–gRNA complexes directed against Sox2 and GFP yields efficient knockout of both genes in GFP-reporter animals. Finally, we show that this method can also be applied to other tissues such as skin and limb mesenchyme. This efficient delivery method opens up the possibility for rapid in vivo genetic screens during axolotl regeneration and can in principle be applied to other vertebrate tissue systems.
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spelling pubmed-57447102018-01-04 Tissue- and time-directed electroporation of CAS9 protein–gRNA complexes in vivo yields efficient multigene knockout for studying gene function in regeneration Fei, Ji-Feng Knapp, Dunja Schuez, Maritta Murawala, Prayag Zou, Yan Pal Singh, Sumeet Drechsel, David Tanaka, Elly M NPJ Regen Med Article A rapid method for temporally and spatially controlled CRISPR-mediated gene knockout in vertebrates will be an important tool to screen for genes involved in complex biological phenomena like regeneration. Here we show that in vivo injection of CAS9 protein–guide RNA (gRNA) complexes into the spinal cord lumen of the axolotl and subsequent electroporation leads to comprehensive knockout of Sox2 gene expression in SOX2(+) neural stem cells with corresponding functional phenotypes from the gene knockout. This is particularly surprising considering the known prevalence of RNase activity in cerebral spinal fluid, which apparently the CAS9 protein protects against. The penetrance/efficiency of gene knockout in the protein-based system is far higher than corresponding electroporation of plasmid-based CRISPR systems. We further show that simultaneous delivery of CAS9–gRNA complexes directed against Sox2 and GFP yields efficient knockout of both genes in GFP-reporter animals. Finally, we show that this method can also be applied to other tissues such as skin and limb mesenchyme. This efficient delivery method opens up the possibility for rapid in vivo genetic screens during axolotl regeneration and can in principle be applied to other vertebrate tissue systems. Nature Publishing Group 2016-06-09 /pmc/articles/PMC5744710/ /pubmed/29302334 http://dx.doi.org/10.1038/npjregenmed.2016.2 Text en Copyright © 2016 Published in partnership with the Australian Regenerative Medicine Institute http://creativecommons.org/licenses/by-nc-nd/4.0/ This work is licensed under a Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International License. The images or other third party material in this article are included in the article’s Creative Commons license, unless indicated otherwise in the credit line; if the material is not included under the Creative Commons license, users will need to obtain permission from the license holder to reproduce the material. To view a copy of this license, visit http://creativecommons.org/licenses/by-nc-nd/4.0/
spellingShingle Article
Fei, Ji-Feng
Knapp, Dunja
Schuez, Maritta
Murawala, Prayag
Zou, Yan
Pal Singh, Sumeet
Drechsel, David
Tanaka, Elly M
Tissue- and time-directed electroporation of CAS9 protein–gRNA complexes in vivo yields efficient multigene knockout for studying gene function in regeneration
title Tissue- and time-directed electroporation of CAS9 protein–gRNA complexes in vivo yields efficient multigene knockout for studying gene function in regeneration
title_full Tissue- and time-directed electroporation of CAS9 protein–gRNA complexes in vivo yields efficient multigene knockout for studying gene function in regeneration
title_fullStr Tissue- and time-directed electroporation of CAS9 protein–gRNA complexes in vivo yields efficient multigene knockout for studying gene function in regeneration
title_full_unstemmed Tissue- and time-directed electroporation of CAS9 protein–gRNA complexes in vivo yields efficient multigene knockout for studying gene function in regeneration
title_short Tissue- and time-directed electroporation of CAS9 protein–gRNA complexes in vivo yields efficient multigene knockout for studying gene function in regeneration
title_sort tissue- and time-directed electroporation of cas9 protein–grna complexes in vivo yields efficient multigene knockout for studying gene function in regeneration
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5744710/
https://www.ncbi.nlm.nih.gov/pubmed/29302334
http://dx.doi.org/10.1038/npjregenmed.2016.2
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