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Increased transgene expression level of rabies virus vector for transsynaptic tracing

Viral vectors that can infect neurons transsynaptically and can strongly express foreign genes are useful for investigating the organization of neural circuits. We previously developed a propagation-competent rabies virus (RV) vector based on a highly attenuated HEP-Flury strain (rHEP5.0-CVSG), whic...

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Autores principales: Ohara, Shinya, Sota, Yasuhiro, Sato, Sho, Tsutsui, Ken-Ichiro, Iijima, Toshio
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2017
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5507306/
https://www.ncbi.nlm.nih.gov/pubmed/28700657
http://dx.doi.org/10.1371/journal.pone.0180960
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author Ohara, Shinya
Sota, Yasuhiro
Sato, Sho
Tsutsui, Ken-Ichiro
Iijima, Toshio
author_facet Ohara, Shinya
Sota, Yasuhiro
Sato, Sho
Tsutsui, Ken-Ichiro
Iijima, Toshio
author_sort Ohara, Shinya
collection PubMed
description Viral vectors that can infect neurons transsynaptically and can strongly express foreign genes are useful for investigating the organization of neural circuits. We previously developed a propagation-competent rabies virus (RV) vector based on a highly attenuated HEP-Flury strain (rHEP5.0-CVSG), which selectively infects neurons and propagates between synaptically connected neurons in a retrograde direction. Its relatively low level of transgene expression, however, makes immunostaining necessary to visualize the morphological features of infected neurons. To increase the transgene expression level of this RV vector, in this study we focused on two viral proteins: the large protein (L) and matrix protein (M). We first attempted to enhance the expression of L, which is a viral RNA polymerase, by deleting the extra transcription unit and shortening the intergenic region between the G and L genes. This viral vector (rHEP5.0-GctL) showed increased transgene expression level with efficient transsynaptic transport. We next constructed an RV vector with a rearranged gene order (rHEP5.0-GML) with the aim to suppress the expression of M, which plays a regulatory role in virus RNA synthesis. Although this vector showed high transgene expression level, the efficiency of transsynaptic transport was low. To further evaluate the usability of rHEP5.0-GctL as a transsynaptic tracer, we inserted a fluorescent timer as a transgene, which changes the color of its fluorescence from blue to red over time. This viral vector enabled us the differentiation of primary infected neurons from secondary infected neurons in terms of the fluorescence wavelength. We expect this propagation-competent RV vector to be useful for elucidating the complex organization of the central nervous system.
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spelling pubmed-55073062017-07-25 Increased transgene expression level of rabies virus vector for transsynaptic tracing Ohara, Shinya Sota, Yasuhiro Sato, Sho Tsutsui, Ken-Ichiro Iijima, Toshio PLoS One Research Article Viral vectors that can infect neurons transsynaptically and can strongly express foreign genes are useful for investigating the organization of neural circuits. We previously developed a propagation-competent rabies virus (RV) vector based on a highly attenuated HEP-Flury strain (rHEP5.0-CVSG), which selectively infects neurons and propagates between synaptically connected neurons in a retrograde direction. Its relatively low level of transgene expression, however, makes immunostaining necessary to visualize the morphological features of infected neurons. To increase the transgene expression level of this RV vector, in this study we focused on two viral proteins: the large protein (L) and matrix protein (M). We first attempted to enhance the expression of L, which is a viral RNA polymerase, by deleting the extra transcription unit and shortening the intergenic region between the G and L genes. This viral vector (rHEP5.0-GctL) showed increased transgene expression level with efficient transsynaptic transport. We next constructed an RV vector with a rearranged gene order (rHEP5.0-GML) with the aim to suppress the expression of M, which plays a regulatory role in virus RNA synthesis. Although this vector showed high transgene expression level, the efficiency of transsynaptic transport was low. To further evaluate the usability of rHEP5.0-GctL as a transsynaptic tracer, we inserted a fluorescent timer as a transgene, which changes the color of its fluorescence from blue to red over time. This viral vector enabled us the differentiation of primary infected neurons from secondary infected neurons in terms of the fluorescence wavelength. We expect this propagation-competent RV vector to be useful for elucidating the complex organization of the central nervous system. Public Library of Science 2017-07-10 /pmc/articles/PMC5507306/ /pubmed/28700657 http://dx.doi.org/10.1371/journal.pone.0180960 Text en © 2017 Ohara et al http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Ohara, Shinya
Sota, Yasuhiro
Sato, Sho
Tsutsui, Ken-Ichiro
Iijima, Toshio
Increased transgene expression level of rabies virus vector for transsynaptic tracing
title Increased transgene expression level of rabies virus vector for transsynaptic tracing
title_full Increased transgene expression level of rabies virus vector for transsynaptic tracing
title_fullStr Increased transgene expression level of rabies virus vector for transsynaptic tracing
title_full_unstemmed Increased transgene expression level of rabies virus vector for transsynaptic tracing
title_short Increased transgene expression level of rabies virus vector for transsynaptic tracing
title_sort increased transgene expression level of rabies virus vector for transsynaptic tracing
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5507306/
https://www.ncbi.nlm.nih.gov/pubmed/28700657
http://dx.doi.org/10.1371/journal.pone.0180960
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