| 盐生杜氏藻RNAi应用中的电激转化条件 |
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| 引用本文: | 孙国华,隋正红,张学成.盐生杜氏藻RNAi应用中的电激转化条件[J].武汉大学学报(理学版),2007,53(4):503-508. |
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| 作者姓名: | 孙国华 隋正红 张学成 |
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| 作者单位: | 中国海洋大学,海洋生命学院,山东,青岛,266003 |
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| 摘 要: | 采用了两种电激模式-高电场强度低电容模式下3~7kV/cm和低电场强度高电容模式下300-500V/cm转化质粒pBl221-cat;PCR扩增检测cat基因部分序列及组织化学染色法GUS检测也同时证明质粒pBl221-cat在盐生杜氏藻中瞬时表达。在此基础之上,插入pds基因的正反向重复序列,构建RNAi表达载体pBIRNAI-Dsa,电激方法转入杜氏盐藻细胞,荧光定量PCR结果表明,转入干涉载体pBIRNAI-Dsa的实验组的pds基因表达显著下降,最低达对照组的28%,表明表达受到抑制。
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| 关 键 词: | 盐生杜氏藻 电激转化 RNA干扰 基因表达 |
| 文章编号: | 1671-8836(2007)04-0503-06 |
| 修稿时间: | 2007-01-09 |
Electroporation Transformation Condition of RNAi Application in Dunaliella salina |
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| SUN Guohua,SUI Zhenghong,ZHANG Xuecheng.Electroporation Transformation Condition of RNAi Application in Dunaliella salina[J].JOurnal of Wuhan University:Natural Science Edition,2007,53(4):503-508. |
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| Authors: | SUN Guohua SUI Zhenghong ZHANG Xuecheng |
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| Institution: | College of Marine Life Science, Ocean University of China, Qingdao 266003, Shandong, China |
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| Abstract: | Plasmid pBI211-cat was transferred into D. salina via electroporation and was proved transiently expressed. Vector pBIRNAI-Dsa was constructed from pBI211-cat and transformed into Dunalilla salina inducing pds gene silencing. Two modes, high-voltage and low-pitched of 3-7 kV/cm and low-volt- age and high-tension of 300-500 V/cm, were adopted to transform ceils and the results were detected from different aspects. PCR amplification and GUS histochemistry staining also proved that pBI221-cat had been delivered into cells and expressed transiently. Partial pds sense sequence and its reverse were inserted into pBI221-cat to form the RNAi vector pBIRNAI-Dsa. Pds gene expressing of the treated group transformed with pBIRNAI-Dsa was reduced, even to 28% of the control group, suggesting that pds gene expressing was restrained. |
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| Keywords: | Dunaliella salina electroporation RNA interference gene expressing |
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