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作 者:蒋黎华[1,2] 杨珏琴[1,2] 范丽安 姚芳娟[1,2]
机构地区:[1]上海第二医科大学 [2]上海市免疫学研究所
出 处:《中华微生物学和免疫学杂志》1998年第3期230-234,共5页Chinese Journal of Microbiology and Immunology
基 金:国家自然科学基金;卫生部基金
摘 要:目的建立检测HLA-B27等位基因的聚合酶链反应/顺序特异的寡核苷酸探针方法,并分析其实用性。方法采用4对引物E40s、E90as;E91as、E136as;E91bs、E181as;E40s、E130as分别扩增靶DNA,用10个探针CL-1~9和PAN-B27分别进行杂交,探针用地高辛系统标记和检测,可检定B*2701~2708共8个等位基因。结果通过对B27等位基因已明确的8个阳性对照DNA、5例B27阴性标本及75例阳性标本的检测,表明本方法技术稳定结果可靠,不会与其它HLAⅠ类基因产生交叉杂交而影响结果的指定。结论本研究为HLA-B27多态性和强直性脊椎炎关联研究提供了一种有效方法,也为HLAⅠ类分子基因分型研究积累了经验。Objective To establish a method of polymerase chain reaction and sequence specific oligonucleotide probes for identification of HLA B27 alleles,and analyse the practicability of the method. Methods Genomic DNA was amplified by using four pairs of primers and amplified DNA was hybridized with ten probes ,respectively.The probes were labelled with Dig 11 dd UTP at the 3end by using terminale transferase.The hybridized probes were detected with antidigoxigenin alkaline phosphatase conjugate Fab fragments and CSPD for visualization.Eight HLA B27 alleles named B*2701,02,03,04,05,06,07 and 08 can be identified. Results A total of seventy five B27(+) and five B27(-) samples from Shanghai were analysed with this method.Eight DNA samples which have been well typed as B*2701,02,03,04,05,06,07 and 08 were used as hybridization controls.The results showed that the method is simple,highly specificitic and sensitive . Conclusions The results suggest that PCR/SSO method will be useful for the study on HLA B27 alleles and Ankylosing spondylitis in Chinese.
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