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Cell-free protein synthesis from genomically recoded bacteria enables multisite incorporation of noncanonical amino acids

机译:通过基因组编码细菌合成无细胞蛋白质可实现非典型氨基酸的多位点整合

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摘要

Cell-free protein synthesis has emerged as a powerful approach for expanding the range of genetically encoded chemistry into proteins. Unfortunately, efforts to site-specifically incorporate multiple non-canonical amino acids into proteins using crude extract-based cell-free systems have been limited by release factor 1 competition. Here we address this limitation by establishing a bacterial cell-free protein synthesis platform based on genomically recoded Escherichia coli lacking release factor 1. This platform was developed by exploiting multiplex genome engineering to enhance extract performance by functionally inactivating negative effectors. Our most productive cell extracts enabled synthesis of 1,780 ± 30 mg/L superfolder green fluorescent protein. Using an optimized platform, we demonstrated the ability to introduce 40 identical p-acetyl-l-phenylalanine residues site specifically into an elastin-like polypeptide with high accuracy of incorporation ( ≥ 98%) and yield (96 ± 3 mg/L). We expect this cell-free platform to facilitate fundamental understanding and enable manufacturing paradigms for proteins with new and diverse chemistries.
机译:无细胞蛋白质合成已成为将遗传编码化学方法扩展到蛋白质的有效方法。不幸的是,使用基于粗提取物的无细胞系统将多种非规范氨基酸位点特异性掺入蛋白质的努力受到释放因子1竞争的限制。在这里,我们通过建立基于基因组重新编码的缺乏释放因子1的大肠杆菌的细菌无细胞蛋白质合成平台来解决这一局限性。该平台是通过利用多重基因组工程技术开发的,可通过功能性失活负效应子来增强提取性能。我们最高效的细胞提取物能够合成1,780±±30μmg/ L的超级文件夹绿色荧光蛋白。使用优化的平台,我们证明了能够将40个相同的对乙酰基-1-苯基丙氨酸残基特异性地引入到弹性蛋白样多肽中,并具有很高的掺入准确度(≥98%)和产率(96±3 mg / L)。我们希望这个无细胞的平台能够促进基本的了解,并使具有新型化学方法的蛋白质制造范例成为可能。

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