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双精氨酸残基处的蛋白水解切割影响羽扇豆种子11S储存球蛋白的结构和功能转变。

Proteolytic cleavage at twin arginine residues affects structural and functional transitions of lupin seed 11S storage globulin.

作者信息

Capraro Jessica, Sessa Fabio, Magni Chiara, Scarafoni Alessio, Maffioli Elisa, Tedeschi Gabriella, Croy Ron R D, Duranti Marcello

机构信息

Department of Food, Environmental and Nutritional Sciences, Università degli Studi di Milano, Milan, Italy.

Department of Veterinary Science and Public Health, Università degli Studi di Milano, Milan, Italy.

出版信息

PLoS One. 2015 Feb 6;10(2):e0117406. doi: 10.1371/journal.pone.0117406. eCollection 2015.

DOI:10.1371/journal.pone.0117406
PMID:25658355
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4319833/
Abstract

The 11S storage globulin of white lupin seeds binds to a metal affinity chromatography matrix. Two unusual stretches of contiguous histidine residues, reminiscent of the multiple histidines forming metal binding motifs, at the C-terminal end of 11S globulin acidic chains were hypothesized as candidate elements responsible for the binding capacity. To prove this, the protein was incubated with a lupin seed endopeptidase previously shown to cleave at twin arginine motifs, recurrent in the sequence region of interest. Upon incubation with this enzyme, the loss of metal binding capacity paralleled that of the anti-his-tag reactive polypeptides. The recovered small proteolytic fragment was analyzed by mass spectrometry and N-terminal sequencing and found to correspond to the 24-mer region cleaved off at twin arginine residues and containing the natural his-tag-like region. Similarly, when lupin seeds were germinated for a few days, the his-tag containing 11S globulin chain was converted to a form devoid of such region, suggesting that this mechanism is a part of the natural degradatory process of the protein. The hypothesis that the ordered and controlled dismantling of storage proteins may generate peptide fragments with potential functional roles in plant ontogenesis is presented and discussed.

摘要

白羽扇豆种子的11S贮藏球蛋白与金属亲和层析基质结合。在11S球蛋白酸性链的C末端有两段连续的异常组氨酸残基延伸,让人联想到形成金属结合基序的多个组氨酸,被推测为负责结合能力的候选元件。为了证明这一点,将该蛋白质与一种白羽扇豆种子内肽酶一起孵育,该内肽酶先前已证明能在感兴趣序列区域中反复出现的双精氨酸基序处切割。与这种酶孵育后,金属结合能力的丧失与抗组氨酸标签反应性多肽的丧失平行。对回收的小蛋白水解片段进行质谱分析和N端测序,发现其对应于在双精氨酸残基处切割下来的24肽区域,并包含天然的组氨酸标签样区域。同样,当白羽扇豆种子萌发几天时,含有组氨酸标签的11S球蛋白链会转化为不含该区域的形式,这表明这种机制是该蛋白质自然降解过程的一部分。本文提出并讨论了一个假说,即贮藏蛋白的有序和可控拆解可能产生在植物个体发育中具有潜在功能作用的肽片段。

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