人CD154基因真核细胞表达载体的构建、鉴定于序列分析

目的 构建人CD154基因真核细胞表达载体。方法 采用RT-PCR方法，从激活的人外周血淋巴细胞的总cDNA中扩增得到820bp的人CD154cDNA片段，再用BamHI和EcoRI双酶切后定向克隆到真核细胞表达载体PcDNA3.1中，限制性内切酶酶切分析重组质粒和DNA序列分析。结果 人CD154cDNA已经正确克隆到真核细胞表达载体pcDNA3.1中。结论本研究为探讨CD154分子与淋巴细胞活化的关系及其信号传导机制。为进一步用于抗移植排斥反应的研究，或对由于CD154遗传缺陷所致的免疫缺陷病的基因治疗奠定了基础。

Construction of mammalian cell expression vector of human CD154 gene from active peripheral blood mononuclear cell and analysis of its sequence

Objective　To obtain mammalian cell expression vector of human CD154 gene. Methods　A 820 bp cDNA fragment was amplified by RT-PCR method from total RNA of human peripheral blood mononuclear cell（PBMC） activated with 10 ng／mL PMA and 1 μg／mL PHA for 8 hours. The fragment was cloned into pcDNA3.1（＋） plasmids.The cloned insert was identified by double digestion of the recombinant plasmid with restriction enzymes BamH Ⅰ and EcoR Ⅰ and sequenced by Sangers-dideory-mediated chain termination. Results　This cDNA fragment included 820 bp entire coding region and a part of the 3 non-coding region. The recombinant mammalian cell expression vector of pcDNA3.1（＋）／hCD154 was constructed， the sequence of the insert was identical to the published sequence encoding human CD154 antigen. Conclusion　The recombinant mammalian cell expression vector of pcDNA3.1（＋）／hCD154 was successfully constructed.