Bicistronic Lentiviruses Containing a Viral 2A Cleavage Sequence Reliably Co-Express Two Proteins and Restore Vision to an Animal Model of LCA1

The disease processes underlying inherited retinal disease are complex and are not completely understood. Many of the corrective gene therapies designed to treat diseases linked to mutations in genes specifically expressed in photoreceptor cells restore function to these cells but fail to stop progr...

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Autores principales: Verrier, Jonathan D., Madorsky, Irina, Coggin, William E., Geesey, Mero, Hochman, Michael, Walling, Elleanor, Daroszewski, Daniel, Eccles, Kristofer S., Ludlow, Rachel, Semple-Rowland, Susan L.
Formato: Texto
Lenguaje:English
Publicado: Public Library of Science 2011
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3103589/
https://www.ncbi.nlm.nih.gov/pubmed/21647387
http://dx.doi.org/10.1371/journal.pone.0020553
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author Verrier, Jonathan D.
Madorsky, Irina
Coggin, William E.
Geesey, Mero
Hochman, Michael
Walling, Elleanor
Daroszewski, Daniel
Eccles, Kristofer S.
Ludlow, Rachel
Semple-Rowland, Susan L.
author_facet Verrier, Jonathan D.
Madorsky, Irina
Coggin, William E.
Geesey, Mero
Hochman, Michael
Walling, Elleanor
Daroszewski, Daniel
Eccles, Kristofer S.
Ludlow, Rachel
Semple-Rowland, Susan L.
author_sort Verrier, Jonathan D.
collection PubMed
description The disease processes underlying inherited retinal disease are complex and are not completely understood. Many of the corrective gene therapies designed to treat diseases linked to mutations in genes specifically expressed in photoreceptor cells restore function to these cells but fail to stop progression of the disease. There is growing consensus that effective treatments for these diseases will require delivery of multiple therapeutic proteins that will be selected to treat specific aspects of the disease process. The purpose of this study was to design a lentiviral transgene that reliably expresses all of the proteins it encodes and does so in a consistent manner among infected cells. We show, using both in vitro and in vivo analyses, that bicistronic lentiviral transgenes encoding two fluorescent proteins fused to a viral 2A-like cleavage peptide meet these expression criteria. To determine if this transgene design is suitable for therapeutic applications, we replaced one of the fluorescent protein genes with the gene encoding guanylate cyclase -1 (GC1) and delivered lentivirus carrying this transgene to the retinas of the GUCY1*B avian model of Leber congenital amaurosis – 1 (LCA1). GUCY1*B chickens carry a null mutation in the GC1 gene that disrupts photoreceptor function and causes blindness at hatching, a phenotype that closely matches that observed in humans with LCA1. We found that treatment of these animals with the 2A lentivector encoding GC1 restored vision to these animals as evidenced by the presence of optokinetic reflexes. We conclude that 2A-like peptides, with proper optimization, can be successfully incorporated into therapeutic vectors designed to deliver multiple proteins to neural retinal. These results highlight the potential of this vector design to serve as a platform for the development of combination therapies designed to enhance or prolong the benefits of corrective gene therapies.
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spelling pubmed-31035892011-06-06 Bicistronic Lentiviruses Containing a Viral 2A Cleavage Sequence Reliably Co-Express Two Proteins and Restore Vision to an Animal Model of LCA1 Verrier, Jonathan D. Madorsky, Irina Coggin, William E. Geesey, Mero Hochman, Michael Walling, Elleanor Daroszewski, Daniel Eccles, Kristofer S. Ludlow, Rachel Semple-Rowland, Susan L. PLoS One Research Article The disease processes underlying inherited retinal disease are complex and are not completely understood. Many of the corrective gene therapies designed to treat diseases linked to mutations in genes specifically expressed in photoreceptor cells restore function to these cells but fail to stop progression of the disease. There is growing consensus that effective treatments for these diseases will require delivery of multiple therapeutic proteins that will be selected to treat specific aspects of the disease process. The purpose of this study was to design a lentiviral transgene that reliably expresses all of the proteins it encodes and does so in a consistent manner among infected cells. We show, using both in vitro and in vivo analyses, that bicistronic lentiviral transgenes encoding two fluorescent proteins fused to a viral 2A-like cleavage peptide meet these expression criteria. To determine if this transgene design is suitable for therapeutic applications, we replaced one of the fluorescent protein genes with the gene encoding guanylate cyclase -1 (GC1) and delivered lentivirus carrying this transgene to the retinas of the GUCY1*B avian model of Leber congenital amaurosis – 1 (LCA1). GUCY1*B chickens carry a null mutation in the GC1 gene that disrupts photoreceptor function and causes blindness at hatching, a phenotype that closely matches that observed in humans with LCA1. We found that treatment of these animals with the 2A lentivector encoding GC1 restored vision to these animals as evidenced by the presence of optokinetic reflexes. We conclude that 2A-like peptides, with proper optimization, can be successfully incorporated into therapeutic vectors designed to deliver multiple proteins to neural retinal. These results highlight the potential of this vector design to serve as a platform for the development of combination therapies designed to enhance or prolong the benefits of corrective gene therapies. Public Library of Science 2011-05-27 /pmc/articles/PMC3103589/ /pubmed/21647387 http://dx.doi.org/10.1371/journal.pone.0020553 Text en Verrier 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, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Verrier, Jonathan D.
Madorsky, Irina
Coggin, William E.
Geesey, Mero
Hochman, Michael
Walling, Elleanor
Daroszewski, Daniel
Eccles, Kristofer S.
Ludlow, Rachel
Semple-Rowland, Susan L.
Bicistronic Lentiviruses Containing a Viral 2A Cleavage Sequence Reliably Co-Express Two Proteins and Restore Vision to an Animal Model of LCA1
title Bicistronic Lentiviruses Containing a Viral 2A Cleavage Sequence Reliably Co-Express Two Proteins and Restore Vision to an Animal Model of LCA1
title_full Bicistronic Lentiviruses Containing a Viral 2A Cleavage Sequence Reliably Co-Express Two Proteins and Restore Vision to an Animal Model of LCA1
title_fullStr Bicistronic Lentiviruses Containing a Viral 2A Cleavage Sequence Reliably Co-Express Two Proteins and Restore Vision to an Animal Model of LCA1
title_full_unstemmed Bicistronic Lentiviruses Containing a Viral 2A Cleavage Sequence Reliably Co-Express Two Proteins and Restore Vision to an Animal Model of LCA1
title_short Bicistronic Lentiviruses Containing a Viral 2A Cleavage Sequence Reliably Co-Express Two Proteins and Restore Vision to an Animal Model of LCA1
title_sort bicistronic lentiviruses containing a viral 2a cleavage sequence reliably co-express two proteins and restore vision to an animal model of lca1
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3103589/
https://www.ncbi.nlm.nih.gov/pubmed/21647387
http://dx.doi.org/10.1371/journal.pone.0020553
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