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作 者:石伟[1] 朱立平[1] 崔莲仙[1] 张淑珍[1] 王汛[1] 李国燕[1]
机构地区:[1]中国医学科学院基础医学研究所中国协和医科大学基础医学院,北京100005
出 处:《中华微生物学和免疫学杂志》1996年第2期83-86,共4页Chinese Journal of Microbiology and Immunology
基 金:中国医学科学院基金;国家教委博士点基金
摘 要:用识别人活化B细胞分化抗原5C5的单克隆抗体5C5和5C5-G1的混合物从人扁桃体细胞λgt11cDNA文库筛选到3个阳性克隆。其cDNA插入到质粒pUC18,经双链双脱氧测序法作核苷酸序列分析,知其中一个cDNA长613bp,另二个长467bp,后者与前者的前467bp完全重叠。613bpcDNA中有一个开放阅读框架,从103bp到429bp,共327bp。Northern印迹分析显示,此613bp cDNA与人扁桃体细胞和3D5细胞的RNA在2.0kb左右有杂交带。与国际上有关基因库的资料比较,未发现有任何同源核苷酸序列。由于这是一个新的cDNA序列,GenBank已接受(接受号为U25041)。从此cDNA的读框推断的蛋白质中第20-30氨基酸为明显的疏水区,故这个蛋白有典型的膜蛋白结构。positive clones have been obtained from a human tonsil cell lambda gt 11 cDNA library screened with a mixture of McAb 5C5 and 5C5-G1 . The cDNAs of the positive clones were inserted into plasmid pUC1 8. The cDNAs were sequenced with . dideoxy-necleotide chain termination method. One cDNA was 613bp long and the length of the other two were 467bp. The latter overlapped the first 467bp of the former completely. There existed an open reading frame of 327bp (from 103bp to 429bp ) in the 6 1 3bp cDNA, Northern blot analysis revealed that the 6 1 3bp cDNA hybridized the RNA extracted from human tonsil cells or 3D5 cells at the site around 2. 0kb. The sequence of the cDNA is not homologous to any DNA saquence published in the world , hance has been accessioned by GenBank with a accessed number of U25041. In the protein deduced from the nucleotide sequence there existed a hydrophobic region from amino acid residue 20 to 30.
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