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  Substantially improved gene transfer to interneurons with second-generation glutamate receptor-targeted DART-AAV vectors

Günther, D., Kovacs, R., Wildner, F., Salivara, A., Thalheimer, F., Fries, P., Geiger, J., & Buchholz, C. (2023). Substantially improved gene transfer to interneurons with second-generation glutamate receptor-targeted DART-AAV vectors. Journal of Neuroscience Methods, 399:. doi:10.1016/j.jneumeth.2023.109981.

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アイテムのパーマリンク: https://hdl.handle.net/21.11116/0000-000D-ECBE-4 版のパーマリンク: https://hdl.handle.net/21.11116/0000-000D-ECBF-3
資料種別: 学術論文

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Guenther_2023_SubstantiallyImproved.pdf (出版社版), 6MB
ファイルのパーマリンク:
https://hdl.handle.net/21.11116/0000-000D-ECC0-0
ファイル名:
Guenther_2023_SubstantiallyImproved.pdf
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Hybrid
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公開
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application/pdf / [MD5]
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著作権日付:
2023
著作権情報:
© 2023 The Authors. Published by Elsevier B.V. This is an open access article under the CC BY-NC-ND license

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作成者

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 作成者:
Günther, D.M.1, 2, 著者
Kovacs, R., 著者
Wildner, F., 著者
Salivara, A., 著者
Thalheimer, F.B., 著者
Fries, Pascal1, 2, 著者                 
Geiger, J.R.P., 著者
Buchholz, C.J., 著者
所属:
1Ernst Strüngmann Institute (ESI) for Neuroscience in Cooperation with Max Planck Society, Max Planck Society, ou_2074314              
2Fries Lab, Ernst Strüngmann Institute (ESI) for Neuroscience in Cooperation with Max Planck Society, Max Planck Society, Deutschordenstraße 46, 60528 Frankfurt, DE, ou_3381216              

内容説明

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キーワード: DART-AAV Capsid engineering Hippocampal slice culture Parvalbumin Inhibitory neuron
 要旨: Background
Adeno-associated viral vectors (AAVs) are a widely used gene transfer platform in neuroscience. Although naturally AAV serotypes can have preferences for certain tissues, selectivity for particular cell types in the CNS does not exist. Towards interneuron targeting, capsid engineering of AAV2 including display of the designed ankyrin repeat protein (DARPin) 2K19 specific for the glutamate receptor subunit 4 (GluA4) at the N-terminus of the VP2 capsid protein has been established. The resulting AAV-VP2N is highly specific for interneurons, but exhibits rather moderate transduction efficiencies.

Methods
Two alternative insertion sites for 2K19 in the GH2/GH3 loop of capsid proteins VP1 (AAV-VP1L) or VP2 (AAV-VP2L) were exploited to yield second generation GluA4-AAVs. Having packaged reporter genes under ubiquitous promoters, the vectors were characterized for biochemical properties as well as gene delivery into cell lines and rat hippocampal slice cultures. Electrophysiological recordings monitored the functional properties of transduced cells.

Results
Compared to AAV-VP2N, the second-generation vectors, especially AAV-VP1L, achieved about 2-fold higher genomic titers as well as a substantially improved GluA4 binding. Improvements in gene transfer activities were 18-fold on GluA4-overexpressing A549 cells and five-fold on rat hippocampal organotypic slice cultures reaching approximately 60 % of all parvalbumin positive interneurons upon a single administration. The spiking behaviour of transduced cells was unaltered and characteristic for a heterogeneous group of interneurons.

Conclusion
The substantially improved gene transfer activity of the second generation GluA4-targeted AAV combined with low toxicity makes this vector an attractive tool for interneuron-directed gene transfer with unrestricted promotor and transgene choice.

資料詳細

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 日付: 2023-09-302023
 出版の状態: 出版
 ページ: -
 出版情報: -
 目次: -
 査読: 査読あり
 識別子(DOI, ISBNなど): DOI: 10.1016/j.jneumeth.2023.109981
 学位: -

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出版物 1

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出版物名: Journal of Neuroscience Methods
種別: 学術雑誌
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出版社, 出版地: -
ページ: - 巻号: 399 通巻号: 109981 開始・終了ページ: - 識別子(ISBN, ISSN, DOIなど): ISSN: 01650270