EGFP基因在中国明对虾原代培养细胞中的导入和表达

中国生物工程杂志

研究报告

EGFP基因在中国明对虾原代培养细胞中的导入和表达

张晓军余黎明李富花相建海

中国科学院海洋研究所实验海洋生物学重点实验室中国科学院海洋研究所实验海洋生物学重点实验室中国科学院海洋研究所实验海洋生物学重点实验室中国科学院海洋研究所实验海洋生物学重点实验室

Transfection and Expression the EGFP Gene in the Primarily Cultured Cells from Chinese Shrimp Fenneropenaeus chinensis

全文: PDF HTML

摘要： 本文以我国重要水产养殖动物中国明对虾（Fenneropenaeus chinensis）贴壁培养和悬浮培养的血细胞、植块培养的类淋巴器官（Oka器官）细胞和卵巢细胞为材料，通过磷酸钙共沉淀法、脂质体介导的转染（脂染）和电穿孔法等多种方法进行了导入EGFP基因的实验。结果表明，通过脂染可以成功地将质粒DNA导入悬浮培养的血细胞、植块培养的Oka器官细胞和卵巢细胞，并使报告基因EGFP得到表达。

Abstract: The study tried to develop the technology related to introducing the eukaryotic expression plasmid into the primarily cultured cells from Chinese shrimp (Fenneropenaeus chinensis), one of the most commercially important aquaculture marine invertebrates in China. The primary cell cultures included the adherent or suspension cultures from the haemocytes and the cell adherent cultures from the lymphoid organ（Oka organ）and ovary of the shrimp. The methods of gene transfer tried in this paper included calcium phosphate mediated transfection, liposome mediated transfection（lipofection）and electroporation. Lipofectin could be used to introduce the plasmid into the cultured cells and to express the reporter gene, EGFP（enhanced green fluorescence protein）gene, in the haemocyte suspension cultures and the cell adherent cultures from the Oka organ and ovary. The present work is to facilitate the study of shrimp immunology and transgenic studies by developing a primary culture system of the shrimp.

收稿日期: 2005-09-13 出版日期: 2006-02-25

通讯作者: 相建海

	服务
	把本文推荐给朋友
	加入引用管理器
	E-mail Alert
	RSS
	作者相关文章
	余黎明
	相建海
	李富花
	张晓军

引用本文:

张晓军,余黎明,李富花,相建海. EGFP基因在中国明对虾原代培养细胞中的导入和表达[J]. 中国生物工程杂志, .

. Transfection and Expression the EGFP Gene in the Primarily Cultured Cells from Chinese Shrimp Fenneropenaeus chinensis. China Biotechnology, .

链接本文:

https://manu60.magtech.com.cn/biotech/CN/ 或 https://manu60.magtech.com.cn/biotech/CN/Y2006/V26/I02/38

No related articles found!

Viewed

Full text

Abstract

Cited

Shared

Discussed