Transgenic mouse offspring generated by ROSI
The production of transgenic animals is an important tool for experimental and applied biology. Over the years, many approaches for the production of transgenic animals have been tried, including pronuclear microinjection, spermmediated gene transfer, transfection of male germ cells, somatic cell nuclear transfer and the use of lentiviral vectors. In the present study, we developed a new transgene delivery approach, and we report for the first time the production of transgenic animals by co-injection of DNA and round spermatid nuclei into non-fertilized mouse oocytes (ROSI). The transgene used was a construct containing the human CMV immediate early promoter and the enhanced GFP gene. With this procedure, 12% of the live offspring we obtained carried the transgene. This efficiency of transgenic production by ROSI was similar to the efficiency by pronuclear injection or intracytoplasmic injection of male gamete nuclei (ICSI). However, ICSI required fewer embryos to produce the same number of transgenic animals. The expression of Egfp mRNA and fluorescence of EGFP were found in the majority of the organs examined in 4 transgenic lines generated by ROSI. Tissue morphology and transgene expression were not distinguishable between transgenic animals produced by ROSI or pronuclear injection. Furthermore, our results are of particular interest because they indicate that the transgene incorporation mediated by intracytoplasmic injection of male gamete nuclei is not an exclusive property of mature sperm cell nuclei with compact chromatin but it can be accomplished with immature sperm cell nuclei with decondensed chromatin as well. The present study also provides alternative procedures for transgene delivery into embryos or reconstituted oocytes. © 2016 by the Society for Reproduction and Development.
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| Format: | artículo biblioteca |
| Language: | English |
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Japanese Society of Animal Reproduction
2016
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| Subjects: | Intracytoplasmic sperm injection (ICSI), Round spermatid nucleus injection (ROSI), Transgenesis, |
| Online Access: | http://hdl.handle.net/20.500.12792/2989 http://hdl.handle.net/10261/289972 |
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dig-inia-es-10261-2899722023-02-17T08:26:04Z Transgenic mouse offspring generated by ROSI Moreira, P. Pérez Cerezales, Serafín Laguna, R. Fernández González, Raúl Sanjuanbenito, B. P. Gutiérrez Adán, Alfonso Intracytoplasmic sperm injection (ICSI) Round spermatid nucleus injection (ROSI) Transgenesis The production of transgenic animals is an important tool for experimental and applied biology. Over the years, many approaches for the production of transgenic animals have been tried, including pronuclear microinjection, spermmediated gene transfer, transfection of male germ cells, somatic cell nuclear transfer and the use of lentiviral vectors. In the present study, we developed a new transgene delivery approach, and we report for the first time the production of transgenic animals by co-injection of DNA and round spermatid nuclei into non-fertilized mouse oocytes (ROSI). The transgene used was a construct containing the human CMV immediate early promoter and the enhanced GFP gene. With this procedure, 12% of the live offspring we obtained carried the transgene. This efficiency of transgenic production by ROSI was similar to the efficiency by pronuclear injection or intracytoplasmic injection of male gamete nuclei (ICSI). However, ICSI required fewer embryos to produce the same number of transgenic animals. The expression of Egfp mRNA and fluorescence of EGFP were found in the majority of the organs examined in 4 transgenic lines generated by ROSI. Tissue morphology and transgene expression were not distinguishable between transgenic animals produced by ROSI or pronuclear injection. Furthermore, our results are of particular interest because they indicate that the transgene incorporation mediated by intracytoplasmic injection of male gamete nuclei is not an exclusive property of mature sperm cell nuclei with compact chromatin but it can be accomplished with immature sperm cell nuclei with decondensed chromatin as well. The present study also provides alternative procedures for transgene delivery into embryos or reconstituted oocytes. © 2016 by the Society for Reproduction and Development. 2023-02-17T08:26:04Z 2023-02-17T08:26:04Z 2016 artículo Journal of Reproduction and Development 62(1): 37-42 (2016) 0916-8818 http://hdl.handle.net/20.500.12792/2989 http://hdl.handle.net/10261/289972 10.1262/jrd.2015-105 1348-4400 en open Japanese Society of Animal Reproduction |
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Intracytoplasmic sperm injection (ICSI) Round spermatid nucleus injection (ROSI) Transgenesis Intracytoplasmic sperm injection (ICSI) Round spermatid nucleus injection (ROSI) Transgenesis |
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Intracytoplasmic sperm injection (ICSI) Round spermatid nucleus injection (ROSI) Transgenesis Intracytoplasmic sperm injection (ICSI) Round spermatid nucleus injection (ROSI) Transgenesis Moreira, P. Pérez Cerezales, Serafín Laguna, R. Fernández González, Raúl Sanjuanbenito, B. P. Gutiérrez Adán, Alfonso Transgenic mouse offspring generated by ROSI |
| description |
The production of transgenic animals is an important tool for experimental and applied biology. Over the years, many approaches for the production of transgenic animals have been tried, including pronuclear microinjection, spermmediated gene transfer, transfection of male germ cells, somatic cell nuclear transfer and the use of lentiviral vectors. In the present study, we developed a new transgene delivery approach, and we report for the first time the production of transgenic animals by co-injection of DNA and round spermatid nuclei into non-fertilized mouse oocytes (ROSI). The transgene used was a construct containing the human CMV immediate early promoter and the enhanced GFP gene. With this procedure, 12% of the live offspring we obtained carried the transgene. This efficiency of transgenic production by ROSI was similar to the efficiency by pronuclear injection or intracytoplasmic injection of male gamete nuclei (ICSI). However, ICSI required fewer embryos to produce the same number of transgenic animals. The expression of Egfp mRNA and fluorescence of EGFP were found in the majority of the organs examined in 4 transgenic lines generated by ROSI. Tissue morphology and transgene expression were not distinguishable between transgenic animals produced by ROSI or pronuclear injection. Furthermore, our results are of particular interest because they indicate that the transgene incorporation mediated by intracytoplasmic injection of male gamete nuclei is not an exclusive property of mature sperm cell nuclei with compact chromatin but it can be accomplished with immature sperm cell nuclei with decondensed chromatin as well. The present study also provides alternative procedures for transgene delivery into embryos or reconstituted oocytes. © 2016 by the Society for Reproduction and Development. |
| format |
artículo |
| topic_facet |
Intracytoplasmic sperm injection (ICSI) Round spermatid nucleus injection (ROSI) Transgenesis |
| author |
Moreira, P. Pérez Cerezales, Serafín Laguna, R. Fernández González, Raúl Sanjuanbenito, B. P. Gutiérrez Adán, Alfonso |
| author_facet |
Moreira, P. Pérez Cerezales, Serafín Laguna, R. Fernández González, Raúl Sanjuanbenito, B. P. Gutiérrez Adán, Alfonso |
| author_sort |
Moreira, P. |
| title |
Transgenic mouse offspring generated by ROSI |
| title_short |
Transgenic mouse offspring generated by ROSI |
| title_full |
Transgenic mouse offspring generated by ROSI |
| title_fullStr |
Transgenic mouse offspring generated by ROSI |
| title_full_unstemmed |
Transgenic mouse offspring generated by ROSI |
| title_sort |
transgenic mouse offspring generated by rosi |
| publisher |
Japanese Society of Animal Reproduction |
| publishDate |
2016 |
| url |
http://hdl.handle.net/20.500.12792/2989 http://hdl.handle.net/10261/289972 |
| work_keys_str_mv |
AT moreirap transgenicmouseoffspringgeneratedbyrosi AT perezcerezalesserafin transgenicmouseoffspringgeneratedbyrosi AT lagunar transgenicmouseoffspringgeneratedbyrosi AT fernandezgonzalezraul transgenicmouseoffspringgeneratedbyrosi AT sanjuanbenitobp transgenicmouseoffspringgeneratedbyrosi AT gutierrezadanalfonso transgenicmouseoffspringgeneratedbyrosi |
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