Gene transfer to primary corneal epithelial cells with an integrating lentiviral vector

Gene transfer to primary corneal epithelial cells with an integrating lentiviral vector

PURPOSE: To evaluate the transfer of heterologous genes carrying a Green Fluorescent Protein (GFP) reporter cassette to primary corneal epithelial cells ex vivo. METHODS: Freshly enucleated rabbit corneoscleral tissue was used to obtain corneal epithelial cell suspension via enzymatic digestion. Cel...

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Main Authors: Lauro Augusto de Oliveira, Charles Kim, Luciene Barbosa de Sousa, Ivan R. Schwab, Mark I. Rosenblatt
Format: Article
Language:English
Published: Conselho Brasileiro de Oftalmologia 2010-10-01
Series:Arquivos Brasileiros de Oftalmologia
Subjects:
Terapia de genes
Doenças da córnea
Lentivírus
Trangenes
Células tronco
Epitélio anterior
Expressão gênica
Online Access:http://www.scielo.br/scielo.php?script=sci_arttext&pid=S0004-27492010000500012&lng=en&tlng=en
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spelling doaj-3dc893af5a9741fc92b9df8fbc75040e2020-11-24T22:21:25ZengConselho Brasileiro de OftalmologiaArquivos Brasileiros de Oftalmologia1678-29252010-10-0173544745310.1590/S0004-27492010000500012S0004-27492010000500012Gene transfer to primary corneal epithelial cells with an integrating lentiviral vectorLauro Augusto de Oliveira0Charles Kim1Luciene Barbosa de Sousa2Ivan R. Schwab3Mark I. Rosenblatt4Universidade Federal de São PauloUniversity of CaliforniaUniversidade Federal de São PauloUniversity of CaliforniaCornell UniversityPURPOSE: To evaluate the transfer of heterologous genes carrying a Green Fluorescent Protein (GFP) reporter cassette to primary corneal epithelial cells ex vivo. METHODS: Freshly enucleated rabbit corneoscleral tissue was used to obtain corneal epithelial cell suspension via enzymatic digestion. Cells were plated at a density of 5×10³ cells/cm² and allowed to grow for 5 days (to 70-80% confluency) prior to transduction. Gene transfer was monitored using fluorescence microscopy and fluorescence activated cell sorter (FACS). We evaluated the transduction efficiency (TE) over time and the dose-response effect of different lentiviral particles. One set of cells were dual sorted by fluorescence activated cell sorter for green fluorescent protein expression as well as Hoechst dye exclusion to evaluate the transduction of potentially corneal epithelial stem cells (side-population phenotypic cells). RESULTS: Green fluorescent protein expressing lentiviral vectors were able to effectively transduce rabbit primary epithelial cells cultured ex vivo. Live cell imaging post-transduction demonstrated GFP-positive cells with normal epithelial cell morphology and growth. The transduction efficiency over time was higher at the 5th post-transduction day (14.1%) and tended to stabilize after the 8th day. The number of transduced cells was dose-dependent, and at the highest lentivirus concentrations approached 7%. When double sorted by fluorescence activated cell sorter to isolate both green fluorescent protein positive and side population cells, transduced side population cells were identified. CONCLUSIONS: Lentiviral vectors can effectively transfer heterologous genes to primary corneal epithelial cells expanded ex vivo. Genes were stably expressed over time, transferred in a dose-dependence fashion, and could be transferred to mature corneal cells as well as presumable putative stem cells.http://www.scielo.br/scielo.php?script=sci_arttext&pid=S0004-27492010000500012&lng=en&tlng=enTerapia de genesDoenças da córneaLentivírusTrangenesCélulas troncoEpitélio anteriorExpressão gênica
collection DOAJ
language English
format Article
sources DOAJ
author Lauro Augusto de Oliveira
Charles Kim
Luciene Barbosa de Sousa
Ivan R. Schwab
Mark I. Rosenblatt
spellingShingle Lauro Augusto de Oliveira
Charles Kim
Luciene Barbosa de Sousa
Ivan R. Schwab
Mark I. Rosenblatt
Gene transfer to primary corneal epithelial cells with an integrating lentiviral vector
Arquivos Brasileiros de Oftalmologia
Terapia de genes
Doenças da córnea
Lentivírus
Trangenes
Células tronco
Epitélio anterior
Expressão gênica
author_facet Lauro Augusto de Oliveira
Charles Kim
Luciene Barbosa de Sousa
Ivan R. Schwab
Mark I. Rosenblatt
author_sort Lauro Augusto de Oliveira
title Gene transfer to primary corneal epithelial cells with an integrating lentiviral vector
title_short Gene transfer to primary corneal epithelial cells with an integrating lentiviral vector
title_full Gene transfer to primary corneal epithelial cells with an integrating lentiviral vector
title_fullStr Gene transfer to primary corneal epithelial cells with an integrating lentiviral vector
title_full_unstemmed Gene transfer to primary corneal epithelial cells with an integrating lentiviral vector
title_sort gene transfer to primary corneal epithelial cells with an integrating lentiviral vector
publisher Conselho Brasileiro de Oftalmologia
series Arquivos Brasileiros de Oftalmologia
issn 1678-2925
publishDate 2010-10-01
description PURPOSE: To evaluate the transfer of heterologous genes carrying a Green Fluorescent Protein (GFP) reporter cassette to primary corneal epithelial cells ex vivo. METHODS: Freshly enucleated rabbit corneoscleral tissue was used to obtain corneal epithelial cell suspension via enzymatic digestion. Cells were plated at a density of 5×10³ cells/cm² and allowed to grow for 5 days (to 70-80% confluency) prior to transduction. Gene transfer was monitored using fluorescence microscopy and fluorescence activated cell sorter (FACS). We evaluated the transduction efficiency (TE) over time and the dose-response effect of different lentiviral particles. One set of cells were dual sorted by fluorescence activated cell sorter for green fluorescent protein expression as well as Hoechst dye exclusion to evaluate the transduction of potentially corneal epithelial stem cells (side-population phenotypic cells). RESULTS: Green fluorescent protein expressing lentiviral vectors were able to effectively transduce rabbit primary epithelial cells cultured ex vivo. Live cell imaging post-transduction demonstrated GFP-positive cells with normal epithelial cell morphology and growth. The transduction efficiency over time was higher at the 5th post-transduction day (14.1%) and tended to stabilize after the 8th day. The number of transduced cells was dose-dependent, and at the highest lentivirus concentrations approached 7%. When double sorted by fluorescence activated cell sorter to isolate both green fluorescent protein positive and side population cells, transduced side population cells were identified. CONCLUSIONS: Lentiviral vectors can effectively transfer heterologous genes to primary corneal epithelial cells expanded ex vivo. Genes were stably expressed over time, transferred in a dose-dependence fashion, and could be transferred to mature corneal cells as well as presumable putative stem cells.
topic Terapia de genes
Doenças da córnea
Lentivírus
Trangenes
Células tronco
Epitélio anterior
Expressão gênica
url http://www.scielo.br/scielo.php?script=sci_arttext&pid=S0004-27492010000500012&lng=en&tlng=en
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AT ivanrschwab genetransfertoprimarycornealepithelialcellswithanintegratinglentiviralvector
AT markirosenblatt genetransfertoprimarycornealepithelialcellswithanintegratinglentiviralvector
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