Highly efficient enrichment method for human plasma glycoproteome analyses using tandem hydrophilic interaction liquid chromatography workflow

Jianzheng Jie; Dan Liu; Bin Yang; Xiajuan Zou

doi:10.1016/j.chroma.2019.460546

Highly efficient enrichment method for human plasma glycoproteome analyses using tandem hydrophilic interaction liquid chromatography workflow

J Chromatogr A. 2020 Jan 11:1610:460546. doi: 10.1016/j.chroma.2019.460546. Epub 2019 Sep 16.

Authors

Jianzheng Jie¹, Dan Liu², Bin Yang², Xiajuan Zou³

Affiliations

¹ Department of Gastrointestinal Surgery, China-Japan Friendship Hospital, 2 Yinghua Dongjie, Chaoyang District, Beijing 100029, PR China.
² Medical and Healthy Analysis Center, Beijing Key Laboratory of Tumor Systems Biology, Peking University, Xueyuan Road 38, Haidian District, Beijing 100191, PR China.
³ Medical and Healthy Analysis Center, Beijing Key Laboratory of Tumor Systems Biology, Peking University, Xueyuan Road 38, Haidian District, Beijing 100191, PR China. Electronic address: [email protected].

PMID: 31570191
DOI: 10.1016/j.chroma.2019.460546

Abstract

Selective enrichment of glycopeptides from complex sample with hydrophilic interaction liquid chromatography (HILIC) method, followed by cleavage of N-glycans by PNGase F to expose an easily detectable mark on the former glycosylation sites is used extensively as a sample preparation for comprehensive glycoproteome analysis. However, the coenrichment of hydrophilic nonglycosylated peptides and the released N-glycans seriously affect the identification of deglycopeptides with nano-LC-MS/MS. Here, we developed a new method for highly efficient and specific enrichment of human plasma N-glycopeptides using HILIC-PNGaseF-HILIC workflow (HPH). The first HILIC enriches the N-glycopeptides from the complex peptide mixtures. After the enriched N-glycopeptides are deglycosylated with PNGase F, the second HILIC captures the coenrichment of hydrophilic nonglycosylated peptides and the N-glycans, and then further enriches the deglycosylated peptides. The glycopeptide enrichment efficiency can be notably improved by employing HPH, evaluated by the highly recovery (more than 93.6%) and specific capturing glycopeptides from tryptic digest of IgG and BSA up to the molar ratios of 1:200. Meanwhile, we found that the alkylated proteins with IAA can affect the enrichment efficiency for N-glycopeptides with HILIC method. Moreover, after optimism the protein digestion, this novel HPH strategy allowed for the identified 722 N-glycopeptides within 202 unique glycoproteins from 1 µL human plasma digest using PNGase F in H₂¹⁶O. Meanwhile, this new HPH strategy identified an average 501 N-glycopeptides within averagely 134 unique glycoproteins from 1 µL human plasma digest using PNGase F in H₂¹⁸O. The enhanced glycopeptide detection was promoted by a substantial depletion of nonglycosylated peptides in the second HILIC. It was found that 52.2% more N-glycosylation peptides were identified by the HPH strategy compared with the using one HILIC enrichment alone.

Keywords: Enrichment; HILIC; Human plasma; Mass spectrometry; N-glycopeptides; Nanomaterials.

MeSH terms

Chromatography, Liquid / methods*
Glycopeptides / blood*
Glycopeptides / isolation & purification
Glycoproteins / blood*
Glycoproteins / isolation & purification
Humans
Hydrophobic and Hydrophilic Interactions
Proteome / analysis*
Proteome / isolation & purification
Proteomics

Substances

Glycopeptides
Glycoproteins
Proteome