人干燥综合征A抗原重组体的构建及鉴定  被引量:4

Construction and Identification of Recombinant Expressing of Human Sjogren's Syndrome Antigen A

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作  者:李倩[1] 高扬[2] 倪安平[1] 于孟学[1] 朱立平[2] 刘音[2] 李永哲[1] 林嘉友[2] 甘晓丹[1] 

机构地区:[1]中国医学科学院/中国协和医科大学北京协和医院检验科,100730 [2]中国医学科学院/中国协和医科大学基础医学研究所免疫研究室,北京100005

出  处:《医学研究杂志》2008年第2期47-49,共3页Journal of Medical Research

基  金:国家863高技术研究发展计划(20024032)

摘  要:目的克隆人干燥综合征A抗原基因(SSA-52kD),为SSA抗原的表达和使用重组抗原用于自身抗体的临床检测奠定基础。方法根据GenBank中检索到的人SSA-52kDcDNA序列,在5′非编码区和3′非编码区设计特异性引物,提取人源Hela细胞总RNA作为模板,反转录RT-PCR扩增人干燥综合征SSA-52kD抗原cDNA。PCR产物纯化后连接至载体PET-30a,导入大肠杆菌DH5α,构建重组质粒PET-30a-SSA-52kD。对重组质粒进行酶切鉴定,选择阳性克隆测序;对DNA测序结果进行鉴定分析。结果RT-PCR扩增产物为1447bp。重组质粒PET-30a-SSA-52kD经BglⅡ和HindⅢ双酶切证实含目的基因片段。序列分析提示与GenBank中检索到的一致。结论成功克隆人SSA-52kD基因,并构建重组质粒PET-30a-SSA-52kD。Objective To clone human Sjogren' s syndrome antigen A(SSA) for expressing of antigen SSA -52kD and establishing a new clinical detecting method. Methods According to the human SSA - 52kD cDNA sequence reported in GenBank,primers of human SSA - 52kD cDNA were designed and synthesized. Human SSA - 52kD cDNA was amplified from RNA of cultured Hela cell by reverse transcriptase polymerase chain reaction( RT - PCR). The production of amplification was ligated to PET -30a vector and then transformed into the competent bacteria DHSctto construct the recombinant plasmid PET- 30a - SSA -52kD. The recombinant plasmid was digested with BglⅡ and Hind Ⅲ ,and positive clones were sequenced. Results The Human SSA -52kD cDNA fragment containing 1447bp was amplified by RT - PCR. Restriction endonuclease mapping using Bgl Ⅱ and Hind Ⅲ showed that the target gene was inserted into the recombinant plasmid. The complete coding sequence of Human SSA - 52kD was consistent with that of GenBank through DNA sequencing. Conclusions The full length of human SSA - 52kD cDNA was successfully cloned and the recombinant plasmid PET - 30a - SSA - 52kD was constructed.

关 键 词:人干燥综合征A抗原 CDNA克隆 重组体 

分 类 号:R442.8[医药卫生—诊断学] R446.62[医药卫生—临床医学]

 

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