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利用噬菌体促进的抗体筛选质粒cDNA文库分离番茄乙醇脱氢酶2编码cDNA

Isolation of a tomato alcohol dehydrogenase 2-encoding cDNA using phage-promoted antibody screening of a plasmid cDNA library.

作者信息

Genez A L, Staraci L C, Alexander D C, Rejda J M, Williamson V M, Chase T, Williams B G

机构信息

Plant Cell Research Institute, Inc., Dublin, CA 94568.

出版信息

Gene. 1993 Jan 30;123(2):157-64. doi: 10.1016/0378-1119(93)90119-n.

Abstract

We describe the cloning of a cDNA encoding tomato alcohol dehydrogenase 2 (Adh2) by screening plasmid cDNA clones in phage plaques. A cDNA library constructed in a plasmid vector containing a unique SstI site at the 5' end of the cDNA insert was transferred into the SstI site of the lacZ gene of phage lambda Charon16, and screened by anti-Adh2 antibody to identify reactive plaques. Plasmid cDNA clones were recovered by SstI digestion, ligation, and transformation from phage minipreps for subsequent characterization. This system preserves the original plasmid library for subsequent screening with nucleic acid probes to identify full-length, multiple independent, or related cDNA clones not subject to the selection pressure of phage growth or lysogeny, or negative antibody reactivity. Thirty-two cDNA clones were identified with polyclonal antiserum to Adh2. Three of these reacted with monoclonal anti-Adh2 and only those three hybridized to maize adh1 sequence. One of these cDNAs, Adh31, was further characterized as encoding Adh2 by hybrid-selected translation and high sequence homology with the maize adh1 gene.

摘要

我们描述了通过筛选噬菌体噬菌斑中的质粒cDNA克隆来克隆编码番茄乙醇脱氢酶2(Adh2)的cDNA的方法。在质粒载体中构建的cDNA文库,该载体在cDNA插入片段的5'端含有一个独特的SstI位点,将其转移到噬菌体λCharon16的lacZ基因的SstI位点,并通过抗Adh2抗体进行筛选以鉴定反应性噬菌斑。通过SstI消化、连接和从噬菌体小量制备物转化来回收质粒cDNA克隆,用于后续表征。该系统保留了原始质粒文库,以便随后用核酸探针进行筛选,以鉴定不受噬菌体生长或溶原性选择压力或阴性抗体反应影响的全长、多个独立或相关的cDNA克隆。用针对Adh2的多克隆抗血清鉴定出32个cDNA克隆。其中三个与单克隆抗Adh2反应,并且只有这三个与玉米adh1序列杂交。其中一个cDNA,Adh31,通过杂交选择翻译和与玉米adh1基因的高度序列同源性进一步表征为编码Adh2。

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