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针叶树脱落酸不敏感3转录因子的异位表达诱导转基因烟草叶片中重组人α-L-艾杜糖醛酸酶的高水平合成。

Ectopic expression of a conifer Abscisic Acid Insensitive3 transcription factor induces high-level synthesis of recombinant human alpha-L-iduronidase in transgenic tobacco leaves.

作者信息

Kermode Allison R, Zeng Ying, Hu Xiaoke, Lauson Samantha, Abrams Suzanne R, He Xu

机构信息

Department of Biological Sciences, Simon Fraser University, Burnaby, BC, Canada.

出版信息

Plant Mol Biol. 2007 Apr;63(6):763-76. doi: 10.1007/s11103-006-9122-y. Epub 2007 Jan 4.

Abstract

We are examining various plant-based systems to produce enzymes for the treatment of human lysosomal storage disorders. Constitutive expression of the gene encoding the human lysosomal enzyme, alpha-L-iduronidase (IDUA; EC 3.2.1.76) in leaves of transgenic tobacco plants resulted in low-enzyme activity, and the protein appeared to be subject to proteolysis. Toward enhancing production of this recombinant enzyme in vegetative tissues, transgenic tobacco plants were generated to co-express a CaMV35S:Chamaecyparis nootkatensis Abscisic Acid Insensitive3 (CnABI3) gene construct, along with the human gene construct. The latter contained regulatory sequences of the Phaseolus vulgaris arcelin 5-I gene (5'-flanking, signal-peptide-encoding, and 3'-flanking regions). Ectopic synthesis of the CnABI3 protein led to the transactivation of the arcelin promoter and accordingly high activity (e.g., 25,000 pmol/min/mg total soluble protein) and levels of recombinant IDUA mRNA and protein were induced in leaves of transgenic tobacco, particularly in the presence of 150-200 microM S-(+)-ABA. Synthesis of human IDUA containing a carboxy-terminal ER retention (SEKDEL) sequence was also inducible by ABA in leaves co-transformed with the CnABI3 gene. As compared to the natural S-(+)-ABA, two persistent ABA analogues, (+)-8' acetylene ABA and (+)-8'methylene ABA, led to greater levels of beta-glucuronidase (GUS) reporter activities in leaves co-expressing the CnABI3 gene and a vicilin:GUS chimeric gene. In contrast, (+)-8' acetylene ABA and natural ABA appeared to be equally effective in stimulating the CnABI3-induced expression of an arcelin:GUS gene, and of the human IDUA gene, the latter also driven by arcelin-gene-regulatory sequences. Various stress-related treatments, particularly high concentrations of NaCl, had an even greater effect than ABA in promoting accumulation of human IDUA in co-transformed tobacco leaves. This strategy provides the means of enhancing the yields of recombinant proteins in transgenic plant vegetative tissues and potentially in cultured plant cells. The human recombinant protein can be readily induced in the presence of chemicals such as NaCl that can be added to cell cultures or even whole plants without a significant increase in production costs.

摘要

我们正在研究各种基于植物的系统,以生产用于治疗人类溶酶体贮积症的酶。在转基因烟草植物叶片中组成型表达编码人类溶酶体酶α-L-艾杜糖醛酸酶(IDUA;EC 3.2.1.76)的基因,导致酶活性较低,并且该蛋白质似乎会被蛋白酶水解。为了提高这种重组酶在营养组织中的产量,构建了转基因烟草植物,使其共表达CaMV35S:黄杉脱落酸不敏感3(CnABI3)基因构建体以及人类基因构建体。后者包含菜豆arcelin 5-I基因的调控序列(5'侧翼、信号肽编码和3'侧翼区域)。CnABI3蛋白的异位合成导致arcelin启动子的反式激活,因此在转基因烟草叶片中诱导了高活性(例如,25,000 pmol/分钟/毫克总可溶性蛋白)以及重组IDUA mRNA和蛋白质的高水平表达,特别是在存在150 - 200 microM S-(+)-脱落酸的情况下。在与CnABI3基因共转化的叶片中,含有羧基末端内质网滞留(SEKDEL)序列的人类IDUA的合成也可被脱落酸诱导。与天然S-(+)-脱落酸相比,两种持久性脱落酸类似物,(+)-8'乙炔脱落酸和(+)-8'亚甲基脱落酸,在共表达CnABI3基因和豌豆球蛋白:GUS嵌合基因的叶片中导致更高水平的β-葡萄糖醛酸酶(GUS)报告基因活性。相比之下,(+)-8'乙炔脱落酸和天然脱落酸在刺激CnABI3诱导的arcelin:GUS基因以及人类IDUA基因(后者也由arcelin基因调控序列驱动)的表达方面似乎同样有效。各种与胁迫相关的处理,特别是高浓度的氯化钠,在促进共转化烟草叶片中人类IDUA的积累方面比脱落酸具有更大的作用。该策略提供了提高转基因植物营养组织以及潜在地在培养的植物细胞中重组蛋白产量的方法。在存在诸如氯化钠等化学物质的情况下,可以很容易地诱导人类重组蛋白的产生,这些化学物质可以添加到细胞培养物甚至整株植物中,而不会显著增加生产成本。

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