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A highly efficient and robust cell-free protein synthesis system prepared from wheat embryos: Plants apparently contain a suicide system directed at ribosomes

机译:由小麦胚制备的高效,强大的无细胞蛋白质合成系统:植物显然含有针对核糖体的自杀系统

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摘要

Current cell-free protein synthesis systems can synthesize proteins with high speed and accuracy, but produce only a low yield because of their instability over time. Here we describe the preparation of a highly efficient but also robust cell-free system from wheat embryos. We first investigated the source of the instability of existing systems in light of endogenous ribosome-inactivating proteins and found that ribosome inactivation by tritin occurs already during extract preparation and continues during incubation for protein synthesis. Therefore, we prepared our system from extensively washed embryos that are devoid of contamination by endosperm, the source of tritin and possibly other inhibitors. In a batch system, we observed continuous translation for 4 h, and sucrose density gradient analysis showed formation of large polysomes, indicating high protein synthesis activity. When the reaction was performed in a dialysis bag, enabling the continuous supply of substrates together with the continuous removal of small byproducts, translation proceeded for >60 h, yielding 1–4 mg of enzymatically active proteins, and 0.6 mg of a 126-kDa tobacco mosaic virus protein, per milliliter of reaction volume. Our results demonstrate that plants contain endogenous inhibitors of translation and that after their elimination the translational apparatus is very stable. This contrasts with the common belief that cell-free translation systems are inherently unstable, even fragile. Our method is useful for the preparation of large amounts of active protein as well as for the study of protein synthesis itself.
机译:当前的无细胞蛋白质合成系统可以高速和准确地合成蛋白质,但是由于其随时间的不稳定性而仅产生低产量。在这里,我们描述了从小麦胚中制备高效但又健壮的无细胞系统的方法。我们首先研究了内源性核糖体失活蛋白对现有系统的不稳定性,并发现三丁烯对核糖体的失活已经发生在提取物制备过程中,并在孵育过程中持续进行,以进行蛋白质合成。因此,我们从经过彻底清洗的胚中制备了我们的系统,这些胚没有胚乳,三tin精和其他抑制剂的污染。在批处理系统中,我们观察到连续翻译4小时,并且蔗糖密度梯度分析显示形成了大的多核糖体,表明蛋白质合成活性很高。当反应在透析袋中进行时,可以连续供应底物,并连续去除少量副产物,翻译进行时间超过60小时,产生1-4 mg的酶促活性蛋白和0.6 mg的126kDa烟草花叶病毒蛋白,每毫升反应量。我们的结果证明植物含有内源性翻译抑制剂,并且在消除植物后,翻译装置非常稳定。这与无细胞翻译系统天生就不稳定甚至脆弱的普遍看法形成了鲜明对比。我们的方法可用于制备大量的活性蛋白以及蛋白质合成本身的研究。

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