Efficient Transfection of Chicken Blastoderms in vivo by Lipofection and Electroporation Using Green Fluorescent Protein Gene as a Marker
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- NAITO Mitsuru
- National Institute of Animal Industry
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- SANO Akiko
- National Institute of Animal Industry
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- TAGAMI Takahiro
- National Institute of Animal Industry
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- HARUMI Takashi
- National Institute of Animal Industry
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- MATSUBARA Yuko
- National Institute of Animal Industry
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Chicken blastoderms of freshly laid and unincubated eggs at stage X were transfected in vivo by lipofection and electroporation using green fluorescent protein (GFP) gene as a marker. DNA was injected into the blastoderm with or without lipofection solution. Electroporation was carried out using a pair of electrodes in parallel on both sides of the blastoderm. The manipulated embryos were cultured in host eggshells and the GFP gene expression was detected through the aperture of the reconstituted eggs under a fluorescent microscope. When blastoderms were transfected by lipofection, expression of the GFP gene tended to be detected in the whole blastoderm. When blastoderms were transfected by electroporation, the GFP gene tended to express intensely in a limited part of the blastoderm. By combining both lipofection and electroporation, transfection efficiency was enhanced and the GFP gene expression in the whole blastoderm was observed more intensely. Embryonic and extra-embryonic tissue expression of the GFP gene was observed in 2-3 day incubated embryos both by lipofection and electroporation. GFP gene is very useful as a marker for detecting the gene expression because GFP gene expression can continuously be monitored in developing live embryos cultured in host eggshells.
収録刊行物
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- 日本畜産学会報
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日本畜産学会報 71 (4), 377-385, 2000
公益社団法人 日本畜産学会
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詳細情報 詳細情報について
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- CRID
- 1390001205196844032
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- NII論文ID
- 10021721218
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- NII書誌ID
- AN00195188
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- ISSN
- 18808255
- 1346907X
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- 本文言語コード
- en
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- データソース種別
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- JaLC
- Crossref
- CiNii Articles
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- 抄録ライセンスフラグ
- 使用不可