【摘要】目的：克隆小鼠CD1d2编码区基因。方法：提取小鼠胸腺组织总RNA，用RT-PCR技术扩增CD1d2 cDNA，PCR产物连接pGEM-T载体，转化大肠杆菌，用限制性酶切反应和DNA测序对阳性克隆进行鉴定，用BLAST软件进行序列分析。结果：扩增出一条特异DNA条带，DNA序列测定表明获取了大小为1008 bp的小鼠CD1d2基因编码区基因。结论：成功克隆了小鼠CD1d2 编码区基因。

    【关键词】小鼠；CD1d2；基因；克隆；鉴定

    文章编号：1009-5519(2008)07-0953-02 中图分类号：R392 文献标识码：A

    Cloning and identification of the gene encoding mouse CD1d2

    CHEN Zhang-quan，HUANG Zhen，LIANG Xiao-dong

    (Department of Clinical Immunology，Guangdong Medical College， Zhanjiang 524023，China)

    【Abstract】Objective：To clone the gene encoding mouse CD1d2(mCD1d2). Methods：Total RNA was extracted from the thymus tissue ......