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Global site-specific N-glycosylation analysis of HIV envelope glycoprotein

机译:HIV包膜糖蛋白的全球特定于位点的N-糖基化分析

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摘要

HIV-1 envelope glycoprotein (Env) is the sole target for broadly neutralizing antibodies (bnAbs) and the focus for design of an antibody-based HIV vaccine. The Env trimer is covered by ~90N-linked glycans, which shield the underlying protein from immune surveillance. bNAbs to HIV develop during infection, with many showing dependence on glycans for binding to Env. The ability to routinely assess the glycan type at each glycosylation site may facilitate design of improved vaccine candidates. Here we present a general mass spectrometry-based proteomics strategy that uses specific endoglycosidases to introduce mass signatures that distinguish peptide glycosites that are unoccupied or occupied by high-mannose/hybrid or complex-type glycans. The method yields >95% sequence coverage for Env, provides semi-quantitative analysis of the glycosylation status at each glycosite. We find that most glycosites in recombinant Env trimers are fully occupied by glycans, varying in the proportion of high-mannose/hybrid and complex-type glycans.
机译:HIV-1包膜糖蛋白(Env)是广泛中和抗体(bnAbs)的唯一目标,也是设计基于抗体的HIV疫苗的重点。 Env三聚体被〜90N连接的聚糖覆盖,从而保护了潜在的蛋白质免受免疫监视。在感染过程中会产生针对HIV的bNAb,其中许多都显示出对聚糖与Env结合的依赖性。常规评估每个糖基化位点的聚糖类型的能力可能有助于设计改良的候选疫苗。在这里,我们介绍了一种基于质谱的蛋白质组学通用策略,该策略使用特定的糖苷内切酶来引入质谱特征,以区分未被高甘露糖/杂合或复杂类型的聚糖占据或占据的肽糖位。该方法的Env序列覆盖率> 95%,可对每个糖位处的糖基化状态进行半定量分析。我们发现重组Env三聚体中的大多数糖位被聚糖完全占据,高甘露糖/杂种和复杂型聚糖的比例各不相同。

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