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作 者:王晶[1,2,3] 朱千政[1,2,3] 陈秀珠[1,2,3] 陈望秋 侯云德
机构地区:[1]武汉同济医科大学基础医学院微生物学教研室 [2]北京军事医学科学院微生物流行病研究所 [3]中国预防医学科学院病毒学研究所
出 处:《同济医科大学学报》1999年第1期4-6,共3页Acta Universitatis Medicinae Tongji
基 金:国家863高科技技术资助项目
摘 要:为了逐步阐明中国人IFN-α基因结构与功能的特点,将从一中国汉族正常胎儿肝细胞染色体DNA中获得的一组PCR克隆产物(PCRA01、PCRA02)分别进行核苷酸序列测定。结果表明,以上两次PCR产物序列完全相同,它们与过去分离的IFN-α1和IFN-αD基因之间的氨基酸序列差异小于1%,为IFN-α1基因的不同变种。PCRA01、PCRA02开放读码框架完全相同,与IFN-α1和IFN-αD基因相比较,其第299位为T,与其相应编码的第100位氨基酸为Val。该基因为继黎孟枫等1991年所分离的IFN-α1C基因之后所发现的又一中国人α1型干扰素基因新变种——IFN-α1/100V,建议命名为IFN-α1d基因。将该基因克隆于原核表达载体PBV220,测定其抗病毒活性为2.4×107U/L。In order to elucidate the structure and function character of Chinese interferon α(IFN α) gene, the nucleotide sequences of one group of PCR cloning products PCRA01, PCRA02 which were separated from chromosome DNA of Chinese (Han nationality) fetal liver, were detected. The sequences of PCRA01 and PCRA02 were completely identical, and their differences of amino acid sequence between IFN α1 and IFN αD gene were less than 1 %, suggesting that they were probably one allelic variant of IFN α1 gene. PCRA01 and PCRA02 differed from IFN α1 and IFN αD by change in their coding regions at nucleotide position 299, thus position 100 of the amino acid sequence would be Val. It revealed that the gene we cloned was another novel variant of IFN α1 gene-IFN α1/100V after IFN α 1C gene reported by Li Mengfeng in 1991. It was proposed that IFN-α 1/100V gene was named IFN α1d gene. In addition, the anti viral activity of IFN α1/100 V was 2.4×10 7 U/L when the gene expressed in prokaryotic expression vector PBV220.
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