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抗体亚基基因的协调表达在转基因烟草的根中产生高水平的功能性抗体。

Coordinate expression of antibody subunit genes yields high levels of functional antibodies in roots of transgenic tobacco.

作者信息

van Engelen F A, Schouten A, Molthoff J W, Roosien J, Salinas J, Dirkse W G, Schots A, Bakker J, Gommers F J, Jongsma M A

机构信息

Centre for Plant Breeding and Reproduction Research (CPRO-DLO), Department of Molecular Biology, Wageningen, The Netherlands.

出版信息

Plant Mol Biol. 1994 Dec;26(6):1701-10. doi: 10.1007/BF00019485.

DOI:10.1007/BF00019485
PMID:7858211
Abstract

To explore the feasibility of employing antibodies to obtain disease resistance against plant root pathogens, we have studied the expression of genes encoding antibodies in roots of transgenic plants. A model monoclonal antibody was used that binds to a fungal cutinase. Heavy and light chain cDNAs were amplified by PCR, fused to a signal sequence for secretion and cloned behind CaMV 35S and TR2' promoters in a single T-DNA. The chimeric genes were cloned both in tandem and in a divergent orientation. The roots of tobacco plants transformed with these constructs produced antibodies that were able to bind antigen in an ELISA. Immunoblotting showed assembly to a full-size antibody. In addition, a F(ab')2-like fragment was observed, which is probably formed by proteolytic processing. Both antibody species were properly targeted to the apoplast, but the full-size antibody was partially retained by the wall of suspension cells. The construct with divergent promoters showed a better performance than the construct with promoters in tandem. It directed the accumulation of functional antibodies to a maximum of 1.1% of total soluble protein, with half of the plants having levels higher than 0.35%. The high efficiency of this construct probably results from coordinated and balanced expression of light and heavy chain genes, as evidenced by RNA blot hybridization.

摘要

为了探索利用抗体获得对植物根部病原体抗病性的可行性,我们研究了转基因植物根中编码抗体的基因的表达。使用了一种与真菌角质酶结合的模型单克隆抗体。通过PCR扩增重链和轻链cDNA,将其与分泌信号序列融合,并克隆到单个T-DNA中的CaMV 35S和TR2'启动子之后。嵌合基因以串联和发散方向进行克隆。用这些构建体转化的烟草植物的根产生了能够在ELISA中结合抗原的抗体。免疫印迹显示组装成完整大小的抗体。此外,观察到一个F(ab')2样片段,可能是由蛋白水解加工形成的。两种抗体都正确地靶向质外体,但完整大小的抗体被悬浮细胞壁部分保留。具有发散启动子的构建体比具有串联启动子的构建体表现更好。它将功能性抗体的积累引导至总可溶性蛋白的1.1%,一半的植物抗体水平高于0.35%。RNA印迹杂交证明,该构建体的高效率可能源于轻链和重链基因的协调平衡表达。

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