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对来自分歧肉杆菌V41分泌的一种类片球菌素细菌素——分歧菌素V41的抗菌特性关键氨基酸侧链和肽结构域的描绘。

Delineation of key amino acid side chains and peptide domains for antimicrobial properties of divercin V41, a pediocin-like bacteriocin secreted by Carnobacterium divergens V41.

作者信息

Bhugaloo-Vial P, Douliez J P, Moll D, Dousset X, Boyaval P, Marion D

机构信息

Unité de Biochimie et Technologie des Protéines, INRA, 44316 Nantes Cedex 03, France.

出版信息

Appl Environ Microbiol. 1999 Jul;65(7):2895-900. doi: 10.1128/AEM.65.7.2895-2900.1999.

DOI:10.1128/AEM.65.7.2895-2900.1999
PMID:10388680
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC91433/
Abstract

Divercin V41 (DV41) is a class IIa bacteriocin produced by Carnobacterium divergens V41. This antilisterial peptide is homologous to pediocin PA-1 and contains two disulfide bonds. To establish the structure-activity relationships of this specific family of bacteriocin, chemical modifications and enzymatic hydrolysis were performed on DV41. Alteration of the net charge of this cationic bacteriocin by succinylation and acetylation revealed that, in a certain range, the electrostatic interactions were surprisingly not necessary for the activity of DV41. Cleavage of DV41 by endoproteinase Asp-N released two fragments N1[1-17] and N2[18-43] corresponding to the conserved hydrophilic N-terminal and the variable hydrophobic C-terminal sequences, respectively. Inhibitory assays showed that only the C-terminal fragment was active, and after trypsin cleavage at Lys42 or disulfide reduction it lost its inhibitory activity. These results suggested that both hydrophobicity and folding imposed by the Cys25-Cys43 disulfide bond were essential for antilisterial activity of the C-terminal hydrophobic peptide. Chemical oxidation of tryptophan residues by N-bromosuccinimide demonstrated that these residues were crucial for inhibitory activity since modification of any one of them rendered DV41 inactive. On the contrary, only the modification of all the three tyrosine residues caused a total loss of antilisterial activity. These latter results strengthened previous results suggesting that the N-terminal domain containing the YGNGV consensus sequence was not involved in the binding of DV41 to a potential specific receptor on listerial cells.

摘要

双歧杆菌素V41(DV41)是由分歧肉杆菌V41产生的IIa类细菌素。这种抗李斯特菌肽与片球菌素PA-1同源,含有两个二硫键。为了建立该特定细菌素家族的构效关系,对DV41进行了化学修饰和酶解。通过琥珀酰化和乙酰化改变这种阳离子细菌素的净电荷,结果表明,在一定范围内,静电相互作用对于DV41的活性并非必要。用天冬氨酸蛋白酶Asp-N对DV41进行切割,释放出两个片段N1[1-17]和N2[18-43],分别对应保守的亲水性N端和可变的疏水性C端序列。抑制试验表明只有C端片段具有活性,在赖氨酸42处进行胰蛋白酶切割或二硫键还原后,它失去了抑制活性。这些结果表明,疏水性以及由半胱氨酸25-半胱氨酸43二硫键形成的折叠对于C端疏水肽的抗李斯特菌活性至关重要。用N-溴代琥珀酰亚胺对色氨酸残基进行化学氧化表明,这些残基对于抑制活性至关重要,因为其中任何一个残基被修饰都会使DV41失活。相反,只有所有三个酪氨酸残基都被修饰才会导致抗李斯特菌活性完全丧失。后一组结果强化了先前的结果,表明含有YGNGV共有序列的N端结构域不参与DV41与李斯特菌细胞上潜在特异性受体的结合。

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