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人类针对合成隐孢子虫糖肽抗体反应的微阵列分析。

Microarray analysis of the human antibody response to synthetic Cryptosporidium glycopeptides.

机构信息

Department of Biochemistry, Emory University, Atlanta, GA 30322, USA.

出版信息

Int J Parasitol. 2013 Oct;43(11):901-7. doi: 10.1016/j.ijpara.2013.05.012. Epub 2013 Jul 12.

Abstract

Glycoproteins expressed by Cryptosporidium parvum are immunogenic in infected individuals but the nature of the epitopes recognised in C. parvum glycoproteins is poorly understood. Since a known immunodominant antigen of Cryptosporidium, the 17kDa glycoprotein, has previously been shown to bind to lectins that recognise the Tn antigen (GalNAcα1-Ser/Thr-R), a large number of glycopeptides with different Tn valency and presentation were prepared. In addition, glycopeptides were synthesised based on a 40kDa cryptosporidial antigen, a polymorphic surface glycoprotein with varying numbers of serine residues, to determine the reactivity with sera from C. parvum-infected humans. These glycopeptides and non-glycosylated peptides were used to generate a glycopeptide microarray to allow screening of sera from C. parvum-infected individuals for the presence of IgM and IgG antibodies. IgG but not IgM in sera from C. parvum-infected individuals bound to multivalent Tn antigen epitopes presented on glycopeptides, suggesting that glycoproteins from C. parvum that contain the Tn antigen induce immune responses upon infection. In addition, molecular differences in glycosylated peptides (e.g. substituting Ser for Thr) as well as the site of glycosylation had a pronounced effect on reactivity. Lastly, pooled sera from individuals infected with either Toxoplasma or Plasmodium were also tested against the modified Cryptosporidium peptides and some sera showed specific binding to glycopeptide epitopes. These studies reveal that specific anti-glycopeptide antibodies that recognise the Tn antigen may be useful diagnostically and in defining the roles of parasite glycoconjugates in infections.

摘要

隐孢子虫表达的糖蛋白在感染个体中具有免疫原性,但对隐孢子虫糖蛋白中识别的表位的性质了解甚少。由于隐孢子虫的一种已知免疫优势抗原,即 17kDa 糖蛋白,先前已被证明与识别 Tn 抗原(GalNAcα1-Ser/Thr-R)的凝集素结合,因此制备了大量具有不同 Tn 价和呈现方式的糖肽。此外,还根据一种 40kDa 的隐孢子虫抗原(一种具有不同丝氨酸残基数的多态表面糖蛋白)合成了糖肽,以确定其与隐孢子虫感染人类的血清的反应性。这些糖肽和非糖基化肽被用于生成糖肽微阵列,以允许筛选隐孢子虫感染个体的血清中是否存在 IgM 和 IgG 抗体。感染隐孢子虫的个体血清中的 IgG 而不是 IgM 与糖肽上呈现的多价 Tn 抗原表位结合,表明含有 Tn 抗原的隐孢子虫糖蛋白在感染时会诱导免疫反应。此外,糖基化肽(例如用 Thr 取代 Ser)和糖基化位点的分子差异对反应性有显著影响。最后,还针对经修饰的隐孢子虫肽测试了来自感染弓形虫或疟原虫个体的混合血清,一些血清显示出对糖肽表位的特异性结合。这些研究表明,识别 Tn 抗原的特异性抗糖肽抗体可能在诊断和确定寄生虫糖缀合物在感染中的作用方面具有有用性。

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本文引用的文献

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Preparation and analysis of glycan microarrays.聚糖微阵列的制备与分析
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BMJ. 2009 Oct 19;339:b4168. doi: 10.1136/bmj.b4168.

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