2种PCR方法扩增盐藻肌动蛋白基因3’旁侧序列比较

目的 :比较扩增盐藻肌动蛋白基因 3’旁侧序列的 2种PCR方法。方法 :用pvuⅡ、EcoRⅤ和StuⅠ 3种限制性内切酶消化盐藻基因组DNA后 ,供 2种PCR用 ,一种是连接介导法PCR(LMPCR) ,与用人工合成的适配子相连并用适配子引物和盐藻肌动蛋白基因特异引物扩增未知序列 ;另一种是反向PCR(IPCR) ,酶切后的DNA自身环化做模板 ,用 2对基因特异引物反向扩增。结果 :2轮PCR后 ,LMPCR中得到大量的非特异扩增产物 ,测序结果发现许多产物是由适配子引物AP2单独扩增引起。而反向PCR在得到pvuⅡ和StuⅠ消化的自连文库中扩增得到 2 .5kb特异产物 ,经测序发现 ,片段两侧为基因特异引物 ,部分序列与已知序列相一致。Southern也进一步证实了IPCR扩增片段来源于盐藻基因组DNA。结论 :IPCR技术在克隆基因旁侧序列时优于LMPCR方法。

Randomized Terminal Linker-dependent PCR: A Versatile and Sensitive Method for Detection of DNA Damage

Objective To design and develop a novel, sensitive and versatile method for in vivo foot printing and studies of DNA damage, such as DNA adducts and strand breaks. Methods Starting with mammalian genomic DNA, single-stranded products were made by repeated primer extension, these products were ligated to a double-stranded linker having a randomized 3 overhang, and used for PCR. DNA breaks in p53 gene produced by restriction endonuclease AfaI were detected by using this new method followed by Southern hybridization with DIG-labeled probe. Results This randomized terminal linker-dependent PCR (RDPCR) method could generate band signals many-fold stronger than conventional ligation-mediated PCR (LMPCR), and it was more rapid, convenient and accurate than the terminal transferase-dependent PCR (TDPCR). Conclusion DNA strand breakage can be detected sensitively in the gene level by RDPCR. Any lesion that blocks primer extension should be detectable.

HTLV-1病毒相关HAM/TSP的发病机制研究

目的:研究HTLV-1病毒通过血脑屏障(BBB)的方式,提示HTLV-1侵犯中枢神经系统(CNS)的机制,从而提示人嗜T淋巴细胞病毒Ⅰ型相关性脊髓病/热带痉挛性截瘫(HAM/TSP)病发病机制和感染途径。方法:通过连接介导多聚酶链反应(LMPCR)分别扩增出5例HAM/TSP患者脑脊液和外周血淋巴细胞中的HTLV-1前病毒DNA片段的序列,然后将扩增产物进行琼脂糖凝胶电泳检测序列的扩增情况,并比较HTLV-1前病毒在脑脊液和外周血淋巴细胞中整合序列的相同机率。结果:HAM/TSP患者脑脊液中存在HTLV-1感染的淋巴细胞数多克隆增殖,而且在脑脊液与外周血中存在HTLV-1病毒整合位点的淋巴细胞克隆。结论:HTLV-1感染可能是通过细胞与细胞间作用而通过血脑屏障的,尤其是通过HTLV-1感染的淋巴细胞迁移至CNS,继而进行增殖并激活CNS中的其它T淋巴细胞,通过对CNS细胞特异性免疫反应和释放细胞因子导致HAM/TSP的病理改变。