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豌豆白蛋白1基因在转基因白三叶草和烟草中的表达。

Expression of the pea albumin 1 gene in transgenic white clover and tobacco.

作者信息

Ealing P M, Hancock K R, White D W

机构信息

Plant Molecular Genetics Laboratory, AgResearch, Grasslands Research Centre, Palmerston North, New Zealand.

出版信息

Transgenic Res. 1994 Nov;3(6):344-54. doi: 10.1007/BF01976766.

DOI:10.1007/BF01976766
PMID:8000431
Abstract

In order to improve the quality of pasture protein for ruminant animal nutrition, we are introducing genes encoding rumen-protected proteins, rich in essential amino acids, into white clover (Trifolium repens L.). We have introduced a chimaeric gene transcribed from the 35S CaMV promoter, and encoding the pea albumin 1 (PA1) protein, rich in sulphur amino acids, into the white clover genotype WR8 by Agrobacterium-mediated transformation. A transgenic plant with high levels of PA1 mRNA was crossed with a commercial genotype from cv. Regal Ladino and both the parent and progeny plants were analyzed for expression and accumulation of PA1 gene products. Steady-state mRNA levels and transcript sizes in transgenic parent and progeny were comparable. The abundance and stability of the PA1 protein in transgenic white clover plants was examined by immunoselection of in vivo [35S]Na2SO4-labelled plant proteins. Evidence is presented here, that the 11 kDa PA1 proprotein precursor is processed correctly in petiole tissues of newly regenerated white clover plantlets but only the 6 kDa PA1a subunit accumulates in leaflets of tissue-culture-grown and older glasshouse-grown clover plants. Attempts to enhance PA1 abundance by altering its subcellular target in transgenic tobacco plants suggest that the endomembrane system is a relatively stable environment compared with the cytoplasm or chloroplast, for the accumulation of PA1, despite its low abundance there (< 0.001% total cell protein).

摘要

为了提高反刍动物营养用牧草蛋白质的质量,我们正在将编码富含必需氨基酸的瘤胃保护蛋白的基因导入白三叶草(Trifolium repens L.)中。我们已通过农杆菌介导的转化,将一个由35S CaMV启动子转录、编码富含硫氨基酸的豌豆白蛋白1(PA1)蛋白的嵌合基因导入白三叶草基因型WR8中。将一株PA1 mRNA水平较高的转基因植物与来自Regal Ladino品种的商业基因型进行杂交,并对亲本和子代植物进行PA1基因产物的表达和积累分析。转基因亲本和子代中的稳态mRNA水平和转录本大小相当。通过对体内[35S]Na2SO4标记的植物蛋白进行免疫选择,检测了转基因白三叶草植物中PA1蛋白的丰度和稳定性。本文提供的证据表明,11 kDa的PA1前体蛋白前体在新再生的白三叶草幼苗的叶柄组织中能正确加工,但只有6 kDa的PA1a亚基在组织培养生长和温室生长的老龄三叶草植物的小叶中积累。通过改变转基因烟草植物中PA1的亚细胞定位来提高其丰度的尝试表明,与细胞质或叶绿体相比,内膜系统对于PA1的积累是一个相对稳定的环境,尽管其在那里的丰度较低(<总细胞蛋白的0.001%)。

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本文引用的文献

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