Leibniz Institute of Plant Genetics and Crop Plant Research (IPK), Corrensstrasse 3, 06466 Stadt Seeland, OT Gatersleben, Germany.
Transgenic Res. 2013 Apr;22(2):369-77. doi: 10.1007/s11248-012-9655-6. Epub 2012 Sep 22.
The synthesis of native-sized proteins is a pre-requisite for exploiting the potential of spider silk as a bio-based material. The unique properties of spider silk, such as extraordinary tensile strength and elasticity, result from the highly repetitive nature of spider silk protein motifs. The present report describes the combination of spider silk flagelliform protein (FLAG) production in the endoplasmic reticulum of tobacco plant leaf cells with an intein-based posttranslational protein fusion technology. The repeated ligation of FLAG monomers resulted in the formation of large multimers. This method avoids the need for highly repetitive transgenes, which may result in a higher genetic and transcriptional stability. Here we show, for the first time, the production of synthetic, high molecular weight spider silk proteins larger than 250 kDa based on the assembly of protein monomers via intein-mediated trans-splicing in planta. The resulting multimeric structures form microfibers, thereby demonstrating their great potential as a biomaterial.
天然大小蛋白质的合成是开发蜘蛛丝作为生物基材料潜力的前提条件。蜘蛛丝的独特性质,如非凡的拉伸强度和弹性,源于蜘蛛丝蛋白基序的高度重复性质。本报告描述了将蜘蛛丝鞭毛状蛋白(FLAG)在烟草植物叶片细胞的内质网中生产与基于内含子的翻译后蛋白融合技术相结合。FLAG 单体的重复连接导致形成大的多聚体。该方法避免了对可能导致更高遗传和转录稳定性的高度重复转基因的需求。在这里,我们首次展示了基于在植物体内通过内含子介导的反剪接将蛋白单体组装来生产大于 250 kDa 的合成、高分子量蜘蛛丝蛋白的方法。所得的多聚体结构形成微纤维,从而证明了它们作为生物材料的巨大潜力。
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