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引用本文:叶志云,金利华,邹海鹰,骆晶晶,林圣彩.凡纳滨对虾G蛋白Gαq基因的克隆和功能鉴定[J].海洋科学,2008,32(8):64-69.
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凡纳滨对虾G蛋白Gαq基因的克隆和功能鉴定
叶志云1, 金利华1,2, 邹海鹰1, 骆晶晶1,3, 林圣彩1
1.厦门大学生命科学学院;2.厦门大学材料学院生物医学工程研究中心;3.加拿大阿尔伯特卡尔加里大学生物化学与分子生物学系
摘要:
为了寻找并克隆凡纳滨对虾(Litopenaeus vannamei)G蛋白α亚基,为研究对虾的生理调控提供理论基础,通过简并PCR和RACE反应获得目的基因的全长cDNA序列;用Blast, DNAstar和Genedoc软件对所得序列进行分析,确定所得序列为凡纳滨对虾G蛋白q基因,命名为pvq。将该基因的编码序列克隆到表达载体,通过免疫共沉淀实验和胞内Ca2+, IP3浓度的测定鉴定该q亚基的功能,发现该亚基的序列和功能与其他q家族成员具有高度保守性。用Western blotting分析发现pvq在对虾身体各部位存在普遍分布,尤其在脑神经、眼柄、腮和颚片中有大量表达,在嗅觉器官触角也有适量分布。说明了pvq在对虾生命活动中的重要性,为研究对虾的生理调控奠定了理论基础。
关键词:  G蛋白  克隆  凡纳滨对虾(Litopenaeus vannamei)
DOI:
分类号:
基金项目:国家863 计划资助项目(2002AA629060)
Identif ication of a novel G2protein Gαq gene in shrimp (Litopenaeus vannamei)
Abstract:
In this study, we aimed to identify new functional genes encoding G protein alpha subunits from Litopenaeus vannamei and elucidate the critical roles that Gα subunits assume in a signal transduction process of shrimp. Degenerate PCR and RACE techniques were employed to achieve the full length of Gα subunit in L. vannamei. Co-immunop recipitation analysis and measurement of second messengers of Ca2+ and IP3 in HEK 293 cells overexpressed with this new Gα subunit were used to identify the basic functions. Western blotting analysis was employed to detect the distribution of the Gα subunit. In the results, the predicted encoding protein of the novel cDNA sequence shared high similarity to q from other organisms, and was thus termed pvq. pvq was highly conserved in both primary structures and basic functions. The expression pattern revealed that pvq was widely expressed in many shrimp tissues, especially enriched in brain and eyes, it also obviously existed in gills, maxillas and antennae. These results indicated that pvq may play critical roles in sensory responses and nerve system of shrimp L. vannamei, which provided a basis for the research of physiological regulation of shrimp.
Key words:  G protein  Cloning  Litopenaeus vannamei
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