Disease resistance in plants is commonly activated by the product of an avirulence (Avr) gene of a pathogen after interaction with the product of a matching resistance (R) gene in the host. In susceptible plants, Avr products might function as virulence or pathogenicity factors. The AVR9 elicitor from the fungus Cladosporium fulvum induces defense responses in tomato plants carrying the Cf-9 resistance gene. This 28-residue beta-sheet AVR9 peptide contains three disulfide bridges, which were identified in this study as Cys2-Cys16, Cys6-Cys19, and Cys12-Cys26. For this purpose, AVR9 was partially reduced, and the thiol groups of newly formed cysteines were modified to prevent reactions with disulfides. After HPLC purification, the partially reduced peptides were sequenced to determine the positions of the modified cysteines, which originated from the reduced disulfide bridge(s). All steps involving molecules with free thiol groups were performed at low pH to suppress disulfide scrambling. For that reason, cysteine modification by N-ethylmaleimide was preferred over modification by iodoacetamide. Upon (partial) reduction of native AVR9, the Cys2-Cys16 bridge opened selectively. The resulting molecule was further reduced to two one-bridge intermediates, which were subsequently completely reduced. The (partially) reduced cysteine-modified AVR9 species showed little or no necrosis-inducing activity, demonstrating the importance of the disulfide bridges for biological activity. Based on peptide length and cysteine spacing, it was previously suggested that AVR9 isa cystine-knotted peptide. Now, we have proven that the bridging pattern of AVR9 is indeed identical to that of cystine-knotted peptides. Moreover, NMR data obtained for AVR9 show that it is structurally closely related to the cystine-knotted carboxypeptidase inhibitor. However, AVR9 does not show any carboxypeptidase inhibiting activity, indicating that the cystine-knot fold is a commonly occurring motif with varying biological functions.

译文

植物中的抗病性通常在与宿主中匹配抗性 (R) 基因的产物相互作用后,由病原体的无毒 (Avr) 基因的产物激活。在易感植物中,Avr产物可能起着毒力或致病性因子的作用。来自真菌枯枝菌的AVR9激发子在携带Cf-9抗性基因的番茄植物中诱导防御反应。该28个残基 β-折叠AVR9肽包含三个二硫键,在本研究中被鉴定为Cys2-Cys16,Cys6-Cys19和Cys12-Cys26。为此,AVR9被部分还原,并且新形成的半胱氨酸的硫醇基团被修饰以防止与二硫化物反应。HPLC纯化后,对部分还原的肽进行测序以确定修饰的半胱氨酸的位置,该半胱氨酸源自还原的二硫键。所有涉及具有游离硫醇基团的分子的步骤均在低pH下进行,以抑制二硫键加扰。因此,与碘乙酰胺修饰不同,N-乙基马来酰亚胺修饰半胱氨酸是优选的。在 (部分) 减少天然AVR9时,Cys2-Cys16桥选择性地打开。所得分子进一步还原为两个一桥中间体,随后完全还原。(部分) 还原的半胱氨酸修饰的AVR9物种几乎没有或没有坏死诱导活性,表明二硫键对生物活性的重要性。根据肽长度和半胱氨酸间距,以前曾建议AVR9是胱氨酸结肽。现在,我们已经证明AVR9的桥接模式确实与胱氨酸结肽的桥接模式相同。此外,为AVR9获得的NMR数据表明,它在结构上与胱氨酸结羧肽酶抑制剂密切相关。然而,AVR9没有显示出任何羧肽酶抑制活性,表明胱氨酸结折叠是具有不同生物学功能的常见基序。

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