风湿性心脏病心肌组织噬菌体表达文库的构建和分析

目的:构建风湿性心脏病患者心脏组织噬菌体表达文库。方法:外科手术治疗中取风湿性心脏病患者新鲜心耳组织,用QIAGEN试剂盒提取RNA,用逆转录酶合成cDNA第一链,用长距离PCR合成双链cDNA,SfiⅠ酶切cDNA后过柱分级收集,用T4 DNA连接酶重组连接入λTripl Ex2载体,最后用λ噬菌体包装后构建成原始文库,用PCR、X-gal等方法进行文库质量鉴定。结果:构建了风湿性心脏病心肌组织噬菌体表达文库,原始文库滴度为3.3×106pfu/mL,重组率为99%,81.25%外源重组片段大于1kb。结论:成功构建了高质量的风湿性心脏病患者心肌组织噬菌体表达文库,为风湿性心脏病的分子机制寻找新的研究策略奠定了实验基础。

一种新的乙型肝炎病毒表面抗原结合蛋白的筛选、表达及其生物学活性的初步研究

为了研究乙肝病毒侵染肝细胞过程中的功能蛋白 ,通过印迹免疫分析技术从人肝cDNA噬菌体表达库中筛选出一株编码乙肝表面抗原结合蛋白 (hepatitisBsurfaceantigenbindingprotein ,HBsAg BP)的cDNA克隆 .基因测序结果表明 ,该cDNA具有独立的开放阅读框架 ,编码 1个由 344个氨基酸残基构成的可溶性蛋白分子 ,属于免疫球蛋白超家族成员 .将该基因克隆到原核表达载体pTriplEx后 ,在E .coliXL1 Blue菌株中获得 4 4kD的重组蛋白 .重组蛋白经Western印迹和ELISA实验证明具有与乙肝表面抗原特异性结合的能力 .进一步经流式细胞仪实验显示 ,在纯化的重组蛋白存在的情况下 ,天然的HBsAg与肝细胞株HepG2的亲和力显著增高 .结果显示 ,该乙肝表面抗原结合蛋白可能是介导乙肝病毒对肝细胞亲和侵染的可溶性辅助受体 .

人源性大肠癌抗原基因的SEREX筛选

目的:寻找人源性大肠癌相关抗原基因.方法:构建3个以入Tripl Ex2噬菌体作载体的大肠癌抗原cDNA表达文库,用自体或异体大肠癌患者血清应用SEREX方法进行免疫筛选.用平板法扩增阳性克隆噬菌体,提取纯化DNA,用SfiI酶切和PCR鉴定插入片段的大小.结果:构建成3个大肠癌抗原cDNA噬菌体表达文库,滴度分别为2.39×106nfu/L,2.07×106nfu/L和1.86×106nfu/L,插入片段长度为0.5-4kb,平均分别为1.4kb,1.6kb和1.3kb.筛选发现4个阳性克隆,插入cDNA片段大小分别为2.4 kb,1.8 kb,2.3 kb和2.2 kb.结论:用SEREX方法筛选大肠癌抗原cDNA表达文库,可获得有价值的大肠癌的重组抗原基因克隆,将有利于大肠癌的早期诊断和重组疫苗的研究.

鼠源抗烟曲霉单链抗体库制备及鉴定

目的构建鼠源抗曲霉菌单链抗体(sc Fv)噬菌体展示文库并进行初步鉴定,为制备用于侵袭性曲霉感染实验室诊断的特异性抗体提供新的方法。方法利用噬菌体展示技术构建鼠源抗烟曲霉半乳甘露聚糖(GM)Sc Fv库,经过4轮"吸附-洗脱-扩增"淘选富集,随机挑选克隆进行可变区基因测序确定文库多样性,并用phageELISA筛选烟曲霉特异性结合的克隆。结果构建的sc Fv噬菌体表达文库,库容量约为1.8×107;经4轮富集筛选,洗脱的表达sc Fv噬菌体滴度渐增;随机挑选出4轮筛选后的20个克隆,其可变区基因序列不同;随机挑选出4轮筛选后的90个克隆,其中6个克隆与烟曲霉GM特异性结合,而与对照的白假丝酵母菌无结合。结论构建并初步鉴定了抗曲霉菌单链抗体库,库容量大,VH和VL区具备多样性;筛选的sc Fv与曲霉菌GM特异性结合,提供了快速制备、筛选GM高特异性抗体分子的新方法。

Construction and primary characterization of Echinococcus multilocularis protoscolex cDNA expression library

Objective To construct a λgt11 cDNA expression library of Echinococcus multilocularis protoscolex isolated in China. Methods Echinococcus multilocularis protoscolex mRNA was extracted using a Quickprep MicromRNA purification kit based on combining of the disruptive and protective properties of guanidinium thiocyanate (GTC) with the speed and selectivity of oligo (dT)-cellulose chromatography in a spum-column with some modification. Purified mRNA (1.8 μg) was submitted to reverse transcription using random hexamers ［pd(N6)］. The double-strand blunt-ended cDNAs were ligated with an EcoRI/NotI adaptor to form a cohesive EcoRI end. Subsequently the synthesized cDNA was inserted into vector λgt11 EcoRI arms. After being packaged in vitro, λgt11 was put to an infectious bacteria Echinococcus coli (E.coli) strain Y1090; the recombinants were screened by color selection. PCR amplification was performed to evaluate the size of insertion DNA fragments.Results The recombinant ratio was nearly 100% and approximately 1×106 clones could be derived from this λgt11 cDNA library. PCR results indicated that the insertion DNAs were about 1.48 kb. Conclusions A λgt11 cDNA expression library consisting of a million recombinant clones has been constructed from Echinococcus multicularis protoscolex mRNA. Further studies on this library are deserved.