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引用本文:柴玉荣,侯卫红,王天云,王宁,袁保梅,王建民,薛乐勋.盐藻的一种盐诱导碳酸酐酶基因转录起始点的确定及表达载体的构建[J].海洋科学,2005,29(4):26-30.
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盐藻的一种盐诱导碳酸酐酶基因转录起始点的确定及表达载体的构建
柴玉荣1, 侯卫红1, 王天云1, 王宁1, 袁保梅1, 王建民1, 薛乐勋1
郑州大学细胞生物学研究室
摘要:
采用5′RACE和巢式PCR的方法确定盐藻(Dunaliella salina)一种盐诱导碳酸酐酶基因的转录起始位点,通过序列分析得出转录起始位点为A,从而确定核心启动子及上游调控区的位置。应用巢式PCR技术分别扩增盐藻这种碳酸酐酶基因上游调控区的2个片段,长度大约分别为0.8和1.2kb,序列经测定无误后分别与带β-葡糖苷酸酶(GUS)报告基因的载体相连接,经酶切鉴定这两种表达载体构建正确。用基因枪法将这两个载体导入盐藻细胞中,经染色检测,GUS基因在转化藻株中得到瞬时表达。
关键词:  盐藻(Dunaliella salina)  碳酸酐酶  转录起始位点  启动子  GUS报告基因
DOI:
分类号:
基金项目:国家自然科学基金资助项目(30270031);国家863基金项目(2002AA628050)
Identification of transcription start site of Dunaliella salina salt inducible carbonic anhydrase gene and construction of its expression vector
Abstract:
The enzyme activity of carbonic anhydrase (CA) from Dunaliella salina can be stimulated by high salinity, so the 5' franking region of carbonic anhydrase gene can be used as a potential inducible promoter to regulate heterogeneous gene expression in D. salina, an extremely halotolerant laga which would be used as a new type bioreactor to produce valuable materials. Th understand and elucidate the regulation of CA, the transcription start site was identified by 5' rapid amplification of cDNA end (5' RACE) and nested PCR. The expression vectors containing two 5' franking regions of CA and the coding sequence of the Escherichia coli beta-glucuronidase (GUS) reporter gene were also constructed. The transcription start site was defined as A. DNA sequence analysis and restriction enzyme digestion revealed that 5' franking regions of CA were not only identical to those published sequences but also contained in the recombination vectors. The two vectors were then thansformed into D. salina by gene gun bombardment. Histochemical analysis demonstrated that the GUS reporter gnen could be expressed transiently in transformed D. salina.
Key words:  Dunaliella salina  carbonic anhydrase  transcription start site  promoter  GUS
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