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在 SARS-CoV-2 刺突糖蛋白的氢/氘交换质谱分析中加入氘代糖肽可提高序列覆盖率。

Inclusion of deuterated glycopeptides provides increased sequence coverage in hydrogen/deuterium exchange mass spectrometry analysis of SARS-CoV-2 spike glycoprotein.

机构信息

Structure Laboratory, Clinical Chemistry Branch, Division of Laboratory Sciences, Centers for Disease Control and Prevention, Atlanta, Georgia, USA.

出版信息

Rapid Commun Mass Spectrom. 2024 Mar 15;38(5):e9690. doi: 10.1002/rcm.9690.

Abstract

RATIONALE

Hydrogen/deuterium exchange mass spectrometry (HDX-MS) can provide precise analysis of a protein's conformational dynamics across varied states, such as heat-denatured versus native protein structures, localizing regions that are specifically affected by such conditional changes. Maximizing protein sequence coverage provides high confidence that regions of interest were located by HDX-MS, but one challenge for complete sequence coverage is N-glycosylation sites. The deuteration of peptides post-translationally modified by asparagine-bound glycans (glycopeptides) has not always been identified in previous reports of HDX-MS analyses, causing significant sequence coverage gaps in heavily glycosylated proteins and uncertainty in structural dynamics in many regions throughout a glycoprotein.

METHODS

We detected deuterated glycopeptides with a Tribrid Orbitrap Eclipse mass spectrometer performing data-dependent acquisition. An MS scan was used to identify precursor ions; if high-energy collision-induced dissociation MS/MS of the precursor indicated oxonium ions diagnostic for complex glycans, then electron transfer low-energy collision-induced dissociation MS/MS scans of the precursor identified the modified asparagine residue and the glycan's mass. As in traditional HDX-MS, the identified glycopeptides were then analyzed at the MS level in samples labeled with D O.

RESULTS

We report HDX-MS analysis of the SARS-CoV-2 spike protein ectodomain in its trimeric prefusion form, which has 22 predicted N-glycosylation sites per monomer, with and without heat treatment. We identified glycopeptides and calculated their average isotopic mass shifts from deuteration. Inclusion of the deuterated glycopeptides increased sequence coverage of spike ectodomain from 76% to 84%, demonstrated that glycopeptides had been deuterated, and improved confidence in results localizing structural rearrangements.

CONCLUSION

Inclusion of deuterated glycopeptides improves the analysis of the conformational dynamics of glycoproteins such as viral surface antigens and cellular receptors.

摘要

原理

氢/氘交换质谱(HDX-MS)可以提供对蛋白质构象动力学的精确分析,跨越不同状态,如热变性与天然蛋白质结构,定位受这种条件变化影响的特定区域。最大限度地提高蛋白质序列覆盖率可提供高置信度,表明 HDX-MS 已定位到感兴趣的区域,但完全序列覆盖的一个挑战是 N-糖基化位点。在先前的 HDX-MS 分析报告中,翻译后由天冬酰胺结合糖基化修饰的肽(糖肽)的氘化一直未被识别,这导致在高度糖基化蛋白质中存在显著的序列覆盖缺口,并在糖蛋白的许多区域中导致结构动力学的不确定性。

方法

我们使用三重四极杆轨道阱 Eclipse 质谱仪在数据依赖型采集模式下检测氘化糖肽。MS 扫描用于鉴定前体离子;如果前体的高能碰撞诱导解离 MS/MS 指示复杂聚糖的氧鎓离子,则电子转移低能碰撞诱导解离 MS/MS 扫描前体鉴定修饰的天冬酰胺残基和聚糖的质量。与传统的 HDX-MS 一样,然后在标记有 DO 的样品中在 MS 水平上分析鉴定的糖肽。

结果

我们报告了 SARS-CoV-2 刺突蛋白三聚体预融合形式的 HDX-MS 分析,每个单体有 22 个预测的 N-糖基化位点,包括和不包括热处理。我们鉴定了糖肽并计算了它们从氘化而来的平均同位素质量位移。包括氘化糖肽可将刺突外域的序列覆盖率从 76%提高到 84%,表明糖肽已被氘化,并提高了定位结构重排的结果的可信度。

结论

包括氘化糖肽可改善病毒表面抗原和细胞受体等糖蛋白构象动力学的分析。

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