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Immunoproteomics approach for EPC1 antigenic epitope prediction of G1 and G6 strains of Echinococcus granulosus

机译:EPC1抗原表位预测的细粒棘球GG1和G6株的免疫免疫组学方法

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摘要

It is important to establish the diagnosis of cystic echinococcosis (CE) infection and begin control management. Currently, it is difficult to make an accurate diagnosis of CE without the availability of an accurate test, which requires the use of sensitive and specific antigens. Using recombinant antigens the sensitivity and specificity of the CE serology assays could be improved considerably. Recently, a highly antigenic protein named EPC1was characterized and isolated from an Echinococcus granulosus protoscoleces. The current study was designed to assess the sequences of EPC1 isolated from different intermediate hosts of E. granulosus. In addition, identification of a highly antigenic linear B cell epitope was found within EPC1 antigen candidate. The EPC1 sequence contains coding and non-coding regions and was compared between two predominant strains (G1 and G6) in Iran. Sequence polymorphism was not found in protein coding regions, suggesting that these regions may be useful for identification of protein expression as an antigen. The average antigenic activity for the whole protein is above 1.1, and hydrophobicity below 0 indicates that it is hydrophilic. Structural analysis showed alpha helical regions in amino acids 6-25, 35-44, 52-62, and 72-78. Nine B cell epitope residues were identified out of 67 total residues. The identity of EPC1 sequence in both G1 and G6 genotypes affects the antigenic efficacy of EPC1and suggests the recombinant protein will be useful in serological assays in the regions where the two strains are prevalent.
机译:建立囊性棘球the病(CE)感染的诊断并开始控制管理非常重要。当前,在没有准确测试的情况下很难对CE进行准确的诊断,这需要使用敏感和特异的抗原。使用重组抗原可以显着提高CE血清学检测的灵敏度和特异性。最近,一种高抗原性蛋白称为EPC1的特征是从粒棘棘球菌的原粘菌中分离出来的。当前的研究旨在评估从粒状大肠杆菌的不同中间宿主分离的EPC1的序列。另外,在EPC1抗原候选物中发现了高抗原性线性B细胞表位的鉴定。 EPC1序列包含编​​码区和非编码区,并在伊朗的两个主要菌株(G1和G6)之间进行了比较。在蛋白质编码区中未发现序列多态性,表明这些区域可用于鉴定蛋白质表达为抗原。整个蛋白质的平均抗原活性高于1.1,而疏水性低于0则表明它是亲水的。结构分析显示氨基酸6-25、35-44、52-62和72-78中的α螺旋区。在总共67个残基中鉴定出9个B细胞表位残基。 EPC1序列在G1和G6基因型中的同一性会影响EPC1的抗原效力,并表明重组蛋白将在两种菌株普遍存在的区域用于血清学检测。

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