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Position: Home > Articles > Cloning and expression analysis of EcRgene in Portunus trituberculatus Progress in Fishery Sciences 2014,35 (1) 98-105

三疣梭子蟹蜕皮激素受体EcR基因的cDNA克隆及表达分析

作  者:
张晓燕;李健;刘萍;陈萍;孙铭;葛红星
单  位:
农业部海洋渔业可持续发展重点实验室
关键词:
三疣梭子蟹;蜕皮激素受体;基因克隆;急性盐度胁迫;RT-PCR
摘  要:
通过简并引物扩增及Smart TM Race技术,首次克隆了三疣梭子蟹Portunus trituberculatus蜕皮激素受体EcR基因cDNA全长序列。该基因全长2 996bp,编码一个由503个氨基酸组成的多肽,预测理论等电点pI为7.33,分子量大小为55.69kDa。同源性及系统进化分析表明,三疣梭子蟹EcR基因与青蟹、拟穴青蟹、大西洋招潮蟹、陆地蟹、美洲螯虾、褐虾、日本对虾的同源性分别为94%、90%、88%、84%、82%、73%、66%。荧光定量RT-PCR结果表明,EcR在肝胰腺、卵巢、肌肉、眼柄、鳃和心脏中均有分布,在肝胰腺中表达量最高,在心脏中最低。高盐(45)胁迫下,EcR基因的表达量在24h后显著低于对照组(P<0.05),总体呈下降趋势;低盐(11)胁迫条件下,EcR转录组的表达量呈现先降低后上升的趋势,在12h达到最低,之后逐渐上升,在48h之后显著高于对照组(P<0.05)。
译  名:
Cloning and expression analysis of EcRgene in Portunus trituberculatus
作  者:
ZHANG Xiao-yan;LI Jian;LIU Ping;CHEN Ping;SUN Ming;GE Hong-xing;Key Laboratory of Sustainable Development of Marine Fisheries,Ministry of Agriculture,Yellow Sea Fisheries Research Institute,Chinese Academy of Fishery Sciences;Ocean University of Shanghai;Ocean University of China;
关键词:
Portunus trituberculatus;;EcR;;Gene cloning;;Salinity stress;;RT-PCR
摘  要:
The complete cDNA sequence of EcRgene in Portunus trituberculatus was first cloned through RT-PCR and Smart TMRace technology.The length of the EcRgene is 2,996bp and encodes a 503amino acid protein with a calculated molecular weight of 55.69kDa and a theoretical pI of 7.33.Blast analysis revealed that the similarity of EcR with C.maenas,Scylla paramamosain,U.pugilator,Gecarcinus lateralis,Homarus americanus,Crangon crangon,and Marsupenaeus japonicas was 94%,90%,88%,84%,82%,73%,and 66%,respectively.Real-time fluorescent quantitative PCR was used to assess the mRNA expression level of EcR after the salinity stress.The results showed that EcR was expressed in all tested tissues of P.trituberculatus,including hepatopancreas,muscle,eyes,gills,and heart.The highest expression level was observed in hepatopancreas,while the lowest in heart.Under salinity(45) stress for 24h,the expression level of EcR was significantly lower than the control and declined gradually.At salinity 11,the EcR expression presented a decrease-increase trend and reached the lowest level at 12h,then the expression level increased gradually,and it was significantly higher than the control group after 48h.

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