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构建核糖体使非规范氨基酸能够在蛋白质中多点掺入。

-Constructed Ribosomes Enable Multi-site Incorporation of Noncanonical Amino Acids into Proteins.

出版信息

Biochemistry. 2021 Jan 26;60(3):161-169. doi: 10.1021/acs.biochem.0c00829. Epub 2021 Jan 11.

Abstract

Efforts to expand the scope of ribosome-mediated polymerization to incorporate noncanonical amino acids (ncAAs) into peptides and proteins hold promise for creating new classes of enzymes, therapeutics, and materials. Recently, the integrated synthesis, assembly, and translation (iSAT) system was established to construct functional ribosomes in cell-free systems. However, the iSAT system has not been shown to be compatible with genetic code expansion. Here, to address this gap, we develop an iSAT platform capable of manufacturing pure proteins with site-specifically incorporated ncAAs. We first establish an iSAT platform based on extracts from genomically recoded lacking release factor 1 (RF-1). This permits complete reassignment of the amber codon translation function. Next, we optimize orthogonal translation system components to demonstrate the benefits of genomic RF-1 deletion on incorporation of ncAAs into proteins. Using our optimized platform, we demonstrate high-level, multi-site incorporation of -acetyl-phenylalanine (pAcF) and -azido-phenylalanine into superfolder green fluorescent protein (sfGFP). Mass spectrometry analysis confirms the high accuracy of incorporation for pAcF at one, two, and five amber sites in sfGFP. The iSAT system updated for ncAA incorporation sets the stage for investigating ribosomal mutations to better understand the fundamental basis of protein synthesis, manufacturing proteins with new properties, and engineering ribosomes for novel polymerization chemistries.

摘要

努力扩大核糖体介导的聚合范围,将非典型氨基酸(ncAAs)掺入肽和蛋白质中,有望创造新的酶、治疗剂和材料类别。最近,建立了集成合成、组装和翻译(iSAT)系统,以在无细胞系统中构建功能性核糖体。然而,iSAT 系统尚未显示与遗传密码扩展兼容。在这里,为了解决这一差距,我们开发了一种 iSAT 平台,能够制造具有特异性掺入 ncAAs 的纯蛋白质。我们首先建立了一个基于缺乏释放因子 1(RF-1)的基因组重编码的 iSAT 平台。这允许完全重新分配琥珀密码子的翻译功能。接下来,我们优化正交翻译系统组件,以展示基因组 RF-1 缺失对将 ncAAs 掺入蛋白质中的益处。使用我们优化的平台,我们证明了在 sfGFP 中的一个、两个和五个琥珀色位点上高度、多位点掺入 -乙酰苯丙氨酸(pAcF)和 -叠氮苯丙氨酸。质谱分析证实了 pAcF 在 sfGFP 中一个、两个和五个琥珀色位点的高掺入准确性。更新后的用于 ncAA 掺入的 iSAT 系统为研究核糖体突变奠定了基础,以更好地理解蛋白质合成的基本原理、制造具有新特性的蛋白质以及为新的聚合化学工程设计核糖体。

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