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通过一种超活性肽天冬酰胺连接酶的前酶成熟、底物识别和连接的结构基础。

Structural basis for proenzyme maturation, substrate recognition, and ligation by a hyperactive peptide asparaginyl ligase.

机构信息

School of Biological Sciences, Nanyang Technological University, Singapore City, 637551, Singapore.

NTU Institute of Structural Biology, Nanyang Technological University, Singapore City, 636921, Singapore.

出版信息

Plant Cell. 2022 Nov 29;34(12):4936-4949. doi: 10.1093/plcell/koac281.

Abstract

Peptide ligases are versatile enzymes that can be utilized for precise protein conjugation for bioengineering applications. Hyperactive peptide asparaginyl ligases (PALs), such as butelase-1, belong to a small class of enzymes from cyclotide-producing plants that can perform site-specific, rapid ligation reactions after a target peptide asparagine/aspartic acid (Asx) residue binds to the active site of the ligase. How PALs specifically recognize their polypeptide substrates has remained elusive, especially at the prime binding side of the enzyme. Here we report crystal structures that capture VyPAL2, a catalytically efficient PAL from Viola yedoensis, in an activated state, with and without a bound substrate. The bound structure shows one ligase with the N-terminal polypeptide tail from another ligase molecule trapped at its active site, revealing how Asx inserts in the enzyme's S1 pocket and why a hydrophobic residue is required at the P2' position. Besides illustrating the anchoring role played by P1 and P2' residues, these results uncover a role for the Gatekeeper residue at the surface of the S2 pocket in shifting the nonprime portion of the substrate and, as a result, the activity toward ligation or hydrolysis. These results suggest a picture for proenzyme maturation in the vacuole and will inform the rational design of peptide ligases with tailored specificities.

摘要

肽连接酶是一种多功能酶,可用于生物工程应用中的精确蛋白质偶联。超活性肽天冬酰胺连接酶(PALs),如 butelase-1,属于一类来自环肽产生植物的小酶类,可在靶肽天冬酰胺/天冬氨酸(Asx)残基结合到连接酶的活性位点后,进行特异性、快速的连接反应。PALs 如何特异性识别其多肽底物仍然难以捉摸,尤其是在酶的主要结合侧。在这里,我们报告了晶体结构,捕获了 VyPAL2,一种来自 Viola yedoensis 的催化效率高的 PAL,在激活状态下,有和没有结合的底物。结合结构显示一个连接酶与另一个连接酶分子的 N 端多肽尾巴被困在其活性位点,揭示了 Asx 如何插入酶的 S1 口袋,以及为什么 P2' 位置需要一个疏水残基。除了说明 P1 和 P2' 残基的锚定作用外,这些结果还揭示了 S2 口袋表面的“守门员”残基在移动底物的非主要部分中的作用,以及因此对连接或水解的活性。这些结果为液泡中酶原的成熟提供了一个图景,并将为具有定制特异性的肽连接酶的合理设计提供信息。

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