Improved methods for cloning and detection in the yeast two hybrid assay

The yeast two-hybrid (Y2H) mating assay is a powerful method for detecting protein-protein interactions. Firstly, the gene of interest is cloned into specific Y2H vectors. Although multiple innovations in cloning methods were made in the past two decades, the conventional cloning method of restriction-enzyme (RE) digestion followed by ligation is still widely used. Unfortunately, many researchers, especially new-comers, often encounter difficulties in cloning a gene into a desired vector. Secondly, interaction between two proteins is commonly detected by growth of the diploids in specific media. This step takes about two weeks. Here, we describe improved cloning and detection procedures for the Y2H assay that accelerate the research progress. The changes in procedures involve running an agarose gel after the doubly digested vector and insert are ligated in the cloning step to determine the efficiency of RE digestion and ligation, and performing an additional replica-plating on plates for earlier assessment of interaction in the detection step. We show an example of Y2H interaction between Trs23 and Trs120 (respective subunits of TRAPP I and TRAPP II), as a proof of concept. By following the improved methods described here, the chances of successful cloning increased and the time for the whole Y2H experimental process is significantly shorter.

酵母双杂交筛选与RSA14-44相互作用的蛋白

构建了包含RSA14-44cDNA的pAS2-1-14诱饵质粒,并进行了人睾丸cDNA文库的酵母双杂交筛选,获得了一条编码人20S蛋白酶体蛋白PSMB5的cDNA片段;用所获得的序列编码该蛋白3’端编码框内全部氨基酸(191个氨基酸);首次证明RSA14-44与PSMB5在酵母细胞中存在相互作用。

适体家族新成员--肽适体

肽适体是一种从随机氨基酸的肽文库中筛选出来,可以高亲合力地与靶物质特异性结合的短肽序列.它的主要结构包括恒定的展示支架蛋白及通过两端限制性插入的高变肽环.酵母双杂交技术常用于筛选针对细胞内特异性靶蛋白的肽适体过程,筛选出的肽适体通过特异性结合识别靶标发挥类似"干扰基因"的作用从而影响蛋白的生物学活性.

快速LacZ检测法提高酵母双杂交试验的敏感度

目的 :建立快速简单敏感准确的LacZ检测法。方法 :将在SD/ -Trp -Leu培养液中过夜培养的待检测酵母菌直接点样在滤纸上进行LacZ检测 ,筛选出LacZ阳性克隆。结果 :将小鼠 3T3文库转化含有WWP1的酵母菌 ,选出 10个较大的SD/ -Trp -Leu -His培养阳性的克隆 ,利用快速LacZ检测法检测这 10个酵母克隆 ,结果在 5h内不同程度地变蓝 ,呈阳性结果 ;而作为对照的传统检测方法在 8h内的检测结果均显示为阴性。结论 :采用快速LacZ检测法检测蛋白质之间的相互作用可以大大缩短筛选的时间 ,简化筛选的步骤 。

香蕉红素氧还蛋白酵母双杂交cDNA文库的构建及鉴定

结合改良的BDSMARTTMPCRcDNASynthesisKitUserManualcDNA合成试剂盒，反转录合成带有目的接头cDNA第一链．通过LD—PCR，扩增双链cDNA（dscDNA）．产物经双酶切后回收，与经同样双酶切的酵母双杂交系统中pGADT7载体连接转化，并进行了鉴定．结果表明：提取的RAN的A200／A200=1．82，表明所提RNA纯度高；双链cDNA文库大于0．2kb，且弥散较长，成瀑布条带状；根据生长菌落计数，文库舍有1．2×10^6转化子。重组子不同插入片段在0．3—2kh之间。表明该文库达到建库要求，为下一步进行酵母双杂交试验奠定基础．此方法用于构建cDNA文库与酵母双杂交系统相结合的研究目前尚未见过相关报道．

棉花纤维RNA提取方法的比较及酵母双杂交文库的构建

为了从棉花纤维中提取高质量的RNA用于构建酵母双杂交文库,采用4种不同的方法提取9天和19天棉花纤维的RNA。琼脂糖凝胶电泳和紫外分光光度法检测结果表明:热硼酸法适用于初生幼嫩纤维和次生加厚纤维的RNA提取,CTAB-PVP法仅适用于初生幼嫩纤维的RNA提取,异硫氰酸胍法和高盐高pH值法提取的RNA由于杂质含量较多而影响反转录效果。采用热硼酸法大量提取总RNA,纯化后的mRNA反转录为cDNA,通过重组将扩增的cDNA片段定向插入到pGADT7-RecAD克隆载体中,得到棉纤维9天和19天的酵母双杂交cDNA文库。2个文库的滴度分别是1.01×107cfu/mL和8×106cfu/mL,cDNA插入片段长度集中分布在250～2500bp之间。由此可以看出,构建的2个棉纤维文库质量较高,可用于棉花纤维素合成和调控途径的研究。