小鼠免疫共刺激信号B7-1和B7-2联合表达载体的构建及包装  

The construction and packaging of double expressing vector of mouse immune-costimulating signal B7-1 and B7-2

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作  者:秦雪梅[1] 张庆英[2] 马道新[1] 徐从高[1] 

机构地区:[1]山东大学齐鲁医院,山东济南250012 [2]青岛市第三人民医院

出  处:《山东医药》2007年第4期16-18,共3页Shandong Medical Journal

基  金:山东省优秀中青年科学家科研奖励基金(02BS095)

摘  要:目的构建含小鼠B7-1和B7-2基因的双表达载体pLXSN-mB7-1-IRES-mB7-2,并包装到PA317细胞中。方法1将EcoRI和BamHI酶切下来的pMD18-mB7-2质粒上的mB7-2基因片段克隆到含有IRES片段的MINV质粒上,得到MINV-IRES-mB7-2载体;2MunI酶切载体MINV-IRES-mB7-2,末端钝化,然后BamHI再酶切,得到含钝末端和BamHI粘末端的IRES-mB7-2基因片段;3XhoI酶切质粒pLXSN-mB7-1,末端钝化,然后BamHI再酶切,形成含钝末端和BamHI粘末端的开环pLXSN-mB7-1质粒,将IRES-mB7-2基因片段插入其中,得到pLXSN-mB7-1-IRES-mB7-2双表达载体;并PA317细胞包装,PCR和电镜鉴定。结果经酶切、PCR、测序等鉴定载体构建成功,并包装到PA317细胞内。结论成功得到了双表达载体pLXSN-mB7-1-IRES-mB7-2和包装后的PA317/mB7-1-mB7-2细胞。[Objective]To construct double expressing vector pLXSN-mB7-1-IRES-mB7-2 with murine B7-1 and B7-2 gene and package them into PA317 cell. [Methods](1)The mB7-2 fragment obtained from plasmid pMD18-mB7-2 which was cutted by EcoRⅠ and BamHⅠ was inserted into vector MINV to gain vector MINV- IRES-mB7-2, which include IRES gene fragment. (2)Digesting vector MINV-IRES-mB7-2 by enzyme MuntI and BamHⅠ to obtain IRES-mB7-2 gene fragment with ambly end and BamHⅠ sticking end. (3)Digesting pLXSN-mB7- 1 by enzyme XhoI and BamHⅠ to gain the opened plasmid pLXSN-mB7-1 with ambly end and BamHI sticking end; Inserting IRES-mB7-2 gene fragment into it to gain the double expressing vector pLXSN-mB7-1-IRES- mB7-2;Then, pLXSN-mB7-1-IRES-mB7-2 was packaged into PA317 cells, which were detected by PCR and electron microscope. [Results] Vector was constructed successfully which was proved by cutting, PCR and sequencing, and packaged into PA317. [Conclusion] Double expressing vector pLXSN-mB7-1-IRES-mB7-2 and PA317/mB7-1-mBT-2 cells were obtained successfully.

关 键 词:载体构建 鉴定 病毒包装 pLXSN—mB7—1-IRES—mB7—2 

分 类 号:R392.1[医药卫生—免疫学]

 

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