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利用天冬酰胺内肽酶进行位点特异性蛋白质标记和定义的泛素-蛋白质缀合物的生成。

Site-Specific Protein Labeling and Generation of Defined Ubiquitin-Protein Conjugates Using an Asparaginyl Endopeptidase.

机构信息

Laboratory for Organic Chemistry (LOC), Department of Chemistry and Applied Biosciences (D-CHAB), ETH Zurich, Vladimir-Prelog-Weg 3, 8093 Zurich, Switzerland.

Department of Chemistry, Technical University of Munich, Lichtenbergstr. 4, 85748 Garching, Germany.

出版信息

J Am Chem Soc. 2022 Jul 27;144(29):13118-13126. doi: 10.1021/jacs.2c02191. Epub 2022 Jul 18.

Abstract

Asparaginyl endopeptidases (AEPs) have recently been widely utilized for peptide and protein modification. Labeling is however restricted to protein termini, severely limiting flexibility and scope in creating diverse conjugates as needed for therapeutic and diagnostic applications. Here, we use genetic code expansion to site-specifically modify target proteins with an isopeptide-linked glycylglycine moiety that serves as an acceptor nucleophile in AEP-mediated transpeptidation with various probes containing a tripeptidic recognition motif. Our approach allows simple and flexible labeling of recombinant proteins at any internal site and leaves a minimal, entirely peptidic footprint (NGG) in the conjugation product. We show site-specific labeling of diverse target proteins with various biophysical probes, including dual labeling at an internal site and the N-terminus. Furthermore, we harness AEP-mediated transpeptidation for generation of ubiquitin- and ubiquitin-like-modifier conjugates bearing a native isopeptide bond and only one point mutation in the linker region.

摘要

天冬酰胺内肽酶(AEPs)最近被广泛用于肽和蛋白质的修饰。然而,这种修饰方法仅限于蛋白质末端,严重限制了在治疗和诊断应用中根据需要创建各种缀合物的灵活性和范围。在这里,我们使用遗传密码扩展技术,通过天冬酰胺内肽酶介导的转肽反应,将特异性修饰的目标蛋白与异肽连接的甘氨酰-甘氨酸部分连接起来,该部分作为含有三肽识别基序的各种探针的亲核接受体。我们的方法允许在任何内部位点对重组蛋白进行简单、灵活的标记,并且在缀合产物中留下最小的、完全肽基的足迹(NGG)。我们展示了各种生物物理探针对不同靶蛋白的特异性标记,包括内部位点和 N 末端的双重标记。此外,我们利用天冬酰胺内肽酶介导的转肽反应生成带有天然异肽键和连接区仅有一个点突变的泛素和泛素样修饰物缀合物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3174/9335880/574a4e3f1f4e/ja2c02191_0002.jpg

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