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T7 RNA聚合酶介导的抗体片段转基因在质体中的表达导致半致死的淡绿色幼苗表型。

T7 RNA polymerase-directed expression of an antibody fragment transgene in plastids causes a semi-lethal pale-green seedling phenotype.

作者信息

Magee Alan M, Coyne Seamus, Murphy David, Horvath Eva M, Medgyesy Peter, Kavanagh Tony A

机构信息

Plant Molecular Biology Laboratory, Smurfit Institute of Genetics, Trinity College, Dublin 2, Ireland.

出版信息

Transgenic Res. 2004 Aug;13(4):325-37. doi: 10.1023/b:trag.0000040019.35147.a4.

DOI:10.1023/b:trag.0000040019.35147.a4
PMID:15517992
Abstract

A T7 promoter-controlled transgene, AbL, encoding a camel single-domain antibody fragment that binds to the model antigen chicken egg-white lysozyme was introduced into the plastid genome of tobacco. AbL expression was activated in the transplastomic line by introducing a nuclear transgene, ST7, encoding a light-regulated plastid-targeted T7RNAP by cross-pollination. The resulting AbL x ST7 progeny seedlings developed a pale-green phenotype and ceased growth soon after germination. High levels of AbL transcripts accumulated in AbL x ST7 seedlings and expression of functional AbL antibody was detected by ELISA. Transplastomic AbL plants were also crossed with nuclear-transformed tobacco plants containing a salicylic acid-inducible transgene encoding a plastid-targeted T7RNAP (PR-T7 transgene). The resulting AbL x PR-T7 progeny were wild-type in appearance but were slow growing and prone to wilting even when provided with adequate water. Although AbL transcription was inducible by treating AbL x PR-T7 leaves with salicylic acid, high levels of T7RNAP-dependent AbL transcripts also accumulated in the absence of induction. However, AbL antibody did not accumulate at levels detectable by immunoblotting or ELISA in AbL x PR-T7 plants despite the fact that total leaf RNA containing AbL transcripts was capable of directing AbL antibody synthesis in an E. coli-derived in vitro translation system.

摘要

一个由T7启动子控制的转基因AbL被导入烟草的质体基因组中,该转基因编码一种能与模型抗原鸡卵清溶菌酶结合的骆驼单域抗体片段。通过异花授粉引入一个核转基因ST7,其编码一种光调控的质体靶向T7 RNA聚合酶,从而在转基因植株系中激活AbL的表达。由此产生的AbL×ST7后代幼苗呈现淡绿色表型,发芽后不久便停止生长。在AbL×ST7幼苗中积累了高水平的AbL转录本,并通过酶联免疫吸附测定法检测到了功能性AbL抗体的表达。转基因AbL植株还与含有水杨酸诱导型转基因(编码质体靶向T7 RNA聚合酶,即PR-T7转基因)的核转化烟草植株杂交。由此产生的AbL×PR-T7后代外观呈野生型,但生长缓慢,即使在提供充足水分的情况下也容易枯萎。尽管通过用水杨酸处理AbL×PR-T7叶片可诱导AbL转录,但在未诱导的情况下也积累了高水平的依赖T7 RNA聚合酶的AbL转录本。然而,尽管含有AbL转录本的总叶RNA能够在大肠杆菌衍生的体外翻译系统中指导AbL抗体的合成,但在AbL×PR-T7植株中,AbL抗体并未积累到免疫印迹或酶联免疫吸附测定法可检测到的水平。

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