Analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques

BACKGROUND: Retinal cell development has been extensively investigated; however, the current knowledge of dynamic morphological and molecular changes is not yet complete. RESULTS: This study was aimed at revealing the dynamic morphological and molecular changes in retinal cell development during the...

Descripción completa

Detalles Bibliográficos
Autores principales: Doh, Sung Tae, Hao, Hailing, Loh, Stephanie C, Patel, Tapan, Tawil, Haim Y, Chen, David K, Pashkova, Anna, Shen, Andy, Wang, Huimin, Cai, Li
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2010
Materias:
Research article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2822752/
https://www.ncbi.nlm.nih.gov/pubmed/20089190
http://dx.doi.org/10.1186/1471-213X-10-8
_version_ 1782177551132655616
author Doh, Sung Tae
Hao, Hailing
Loh, Stephanie C
Patel, Tapan
Tawil, Haim Y
Chen, David K
Pashkova, Anna
Shen, Andy
Wang, Huimin
Cai, Li
author_facet Doh, Sung Tae
Hao, Hailing
Loh, Stephanie C
Patel, Tapan
Tawil, Haim Y
Chen, David K
Pashkova, Anna
Shen, Andy
Wang, Huimin
Cai, Li
author_sort Doh, Sung Tae
collection PubMed
description BACKGROUND: Retinal cell development has been extensively investigated; however, the current knowledge of dynamic morphological and molecular changes is not yet complete. RESULTS: This study was aimed at revealing the dynamic morphological and molecular changes in retinal cell development during the embryonic stages using a new method of targeted retinal injection, in ovo electroporation, and immunohistochemistry techniques. A plasmid DNA that expresses the green fluorescent protein (GFP) as a marker was delivered into the sub-retinal space to transfect the chick retinal stem/progenitor cells at embryonic day 3 (E3) or E4 with the aid of pulses of electric current. The transfected retinal tissues were analyzed at various stages during chick development from near the start of neurogenesis at E4 to near the end of neurogenesis at E18. The expression of GFP allowed for clear visualization of cell morphologies and retinal laminar locations for the indication of retinal cell identity. Immunohistochemistry using cell type-specific markers (e.g., Visinin, Xap-1, Lim1+2, Pkcα, NeuN, Pax6, Brn3a, Vimentin, etc.) allowed further confirmation of retinal cell types. The composition of retinal cell types was then determined over time by counting the number of GFP-expressing cells observed with morphological characteristics specific to the various retinal cell types. CONCLUSION: The new method of retinal injection and electroporation at E3 - E4 allows the visualization of all retinal cell types, including the late-born neurons, e.g., bipolar cells at a level of single cells, which has been difficult with a conventional method with injection and electroporation at E1.5. Based on data collected from analyses of cell morphology, laminar locations in the retina, immunohistochemistry, and cell counts of GFP-expressing cells, the time-line and dynamic morphological and molecular changes of retinal cell development were determined. These data provide more complete information on retinal cell development, and they can serve as a reference for the investigations in normal retinal development and diseases.
format Text
id pubmed-2822752
institution National Center for Biotechnology Information
language English
publishDate 2010
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-28227522010-02-17 Analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques Doh, Sung Tae Hao, Hailing Loh, Stephanie C Patel, Tapan Tawil, Haim Y Chen, David K Pashkova, Anna Shen, Andy Wang, Huimin Cai, Li BMC Dev Biol Research article BACKGROUND: Retinal cell development has been extensively investigated; however, the current knowledge of dynamic morphological and molecular changes is not yet complete. RESULTS: This study was aimed at revealing the dynamic morphological and molecular changes in retinal cell development during the embryonic stages using a new method of targeted retinal injection, in ovo electroporation, and immunohistochemistry techniques. A plasmid DNA that expresses the green fluorescent protein (GFP) as a marker was delivered into the sub-retinal space to transfect the chick retinal stem/progenitor cells at embryonic day 3 (E3) or E4 with the aid of pulses of electric current. The transfected retinal tissues were analyzed at various stages during chick development from near the start of neurogenesis at E4 to near the end of neurogenesis at E18. The expression of GFP allowed for clear visualization of cell morphologies and retinal laminar locations for the indication of retinal cell identity. Immunohistochemistry using cell type-specific markers (e.g., Visinin, Xap-1, Lim1+2, Pkcα, NeuN, Pax6, Brn3a, Vimentin, etc.) allowed further confirmation of retinal cell types. The composition of retinal cell types was then determined over time by counting the number of GFP-expressing cells observed with morphological characteristics specific to the various retinal cell types. CONCLUSION: The new method of retinal injection and electroporation at E3 - E4 allows the visualization of all retinal cell types, including the late-born neurons, e.g., bipolar cells at a level of single cells, which has been difficult with a conventional method with injection and electroporation at E1.5. Based on data collected from analyses of cell morphology, laminar locations in the retina, immunohistochemistry, and cell counts of GFP-expressing cells, the time-line and dynamic morphological and molecular changes of retinal cell development were determined. These data provide more complete information on retinal cell development, and they can serve as a reference for the investigations in normal retinal development and diseases. BioMed Central 2010-01-20 /pmc/articles/PMC2822752/ /pubmed/20089190 http://dx.doi.org/10.1186/1471-213X-10-8 Text en Copyright ©2010 Doh et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research article
Doh, Sung Tae
Hao, Hailing
Loh, Stephanie C
Patel, Tapan
Tawil, Haim Y
Chen, David K
Pashkova, Anna
Shen, Andy
Wang, Huimin
Cai, Li
Analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques
title Analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques
title_full Analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques
title_fullStr Analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques
title_full_unstemmed Analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques
title_short Analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques
title_sort analysis of retinal cell development in chick embryo by immunohistochemistry and in ovo electroporation techniques
topic Research article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2822752/
https://www.ncbi.nlm.nih.gov/pubmed/20089190
http://dx.doi.org/10.1186/1471-213X-10-8
work_keys_str_mv AT dohsungtae analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT haohailing analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT lohstephaniec analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT pateltapan analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT tawilhaimy analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT chendavidk analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT pashkovaanna analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT shenandy analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT wanghuimin analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques
AT caili analysisofretinalcelldevelopmentinchickembryobyimmunohistochemistryandinovoelectroporationtechniques

Ejemplares similares