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与环肽 kalata B1 生物合成相关的加工和环化事件的研究进展。

Insights into processing and cyclization events associated with biosynthesis of the cyclic Peptide kalata B1.

机构信息

Department of Biochemistry, La Trobe University, Melbourne Victoria 3086, Australia.

出版信息

J Biol Chem. 2012 Aug 10;287(33):28037-46. doi: 10.1074/jbc.M112.347823. Epub 2012 Jun 14.

DOI:10.1074/jbc.M112.347823
PMID:22700963
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3431668/
Abstract

Plant cyclotides are the largest family of gene-encoded cyclic proteins. They act as host defense molecules to protect plants and are promising candidates as insecticidal and nematocidal agents in agriculture. For this promise to be realized a greater understanding of the post-translational processing of these proteins is needed. Cyclotides are cleaved from precursor proteins with subsequent ligation of the N and C termini to form a continuous peptide backbone. This cyclization step is inefficient in transgenic plants and our work aims to shed light on the specificity requirements at the excision sites for cyclic peptide production. Using the prototypic cyclotide kalata B1 (kB1) expressed from the Oak1 gene, MALDI-TOF mass spectrometry was used to examine the cyclization efficiency when mutants of the Oak1 gene were expressed in transgenic Nicotiana benthamiana. Cleavage at the N terminus of the cyclotide domain occurs rapidly with no strict specificity requirements for amino acids at the cleavage site. In contrast, the C-terminal region of the cyclotide domain in the P2, P1, P1', and P2' positions is highly conserved and only specific amino acids can occupy these positions. The cyclization reaction requires an Asn at position P1 followed by a small amino acid (Ala, Gly, Ser) at the P1' position. The P2' position must be filled by Leu or Ile; in their absence an unusual post-translational modification occurs. Substitution of the P2' Leu with Ala leads to hydroxylation of the neighboring proline. Through mutational analysis this novel proline hydroxylation motif was determined to be Gly-Ala-Pro-Ser.

摘要

植物环肽是基因编码的环状蛋白中最大的家族。它们作为植物防御分子,保护植物,是农业中杀虫和杀线虫剂的有前途的候选物。为了实现这一承诺,需要对这些蛋白质的翻译后加工有更深入的了解。环肽从前体蛋白中切割出来,然后将 N 和 C 末端连接起来形成连续的肽骨架。这个环化步骤在转基因植物中效率不高,我们的工作旨在阐明产生环状肽所需的切除位点的特异性要求。使用从 Oak1 基因表达的典型环肽 kalata B1 (kB1),通过 MALDI-TOF 质谱分析,研究了在转基因 Nicotiana benthamiana 中表达 Oak1 基因突变体时环肽的环化效率。环肽结构域的 N 末端切割迅速,切割位点的氨基酸没有严格的特异性要求。相比之下,环肽结构域的 C 末端区域在 P2、P1、P1'和 P2'位置高度保守,只有特定的氨基酸可以占据这些位置。环化反应需要在 P1 位置有一个 Asn,然后在 P1'位置有一个小氨基酸(Ala、Gly、Ser)。P2'位置必须由 Leu 或 Ile 填充;否则会发生异常的翻译后修饰。用 Ala 取代 P2' Leu 会导致邻近脯氨酸的羟化。通过突变分析,确定了这个新的脯氨酸羟化模体为 Gly-Ala-Pro-Ser。

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