Characterization of Site-Specific N-Glycopeptide Isoforms of α-1-Acid Glycoprotein from an Interlaboratory Study Using LC-MS/MS

Ju Yeon Lee; Hyun Kyoung Lee; Gun Wook Park; Heeyoun Hwang; Hoi Keun Jeong; Ki Na Yun; Eun Sun Ji; Kwang Hoe Kim; Jun Seok Kim; Jong Won Kim; Sung Ho Yun; Chi Won Choi; Seung Il Kim; Jong Sun Lim; Seul Ki Jeong; Young Ki Paik; Soo Youn Lee; Jisook Park; Su Yeon Kim; Young Jin Choi; Yong In Kim; Jawon Seo; Je Yoel Cho; Myoung Jin Oh; Nari Seo; Hyun Joo An; Jin Young Kim; Jong Shin Yoo

doi:10.1021/acs.jproteome.5b01159

Characterization of Site-Specific N-Glycopeptide Isoforms of α-1-Acid Glycoprotein from an Interlaboratory Study Using LC-MS/MS

Ju Yeon Lee, Hyun Kyoung Lee, Gun Wook Park, Heeyoun Hwang, Hoi Keun Jeong, Ki Na Yun, Eun Sun Ji, Kwang Hoe Kim, Jun Seok Kim, Jong Won Kim, Sung Ho Yun, Chi Won Choi, Seung Il Kim, Jong Sun Lim, Seul Ki Jeong, Young Ki Paik, Soo Youn Lee, Jisook Park, Su Yeon Kim, Young Jin ChoiYong In Kim, Jawon Seo, Je Yoel Cho, Myoung Jin Oh, Nari Seo, Hyun Joo An, Jin Young Kim, Jong Shin Yoo

Department of Biochemistry

Research output: Contribution to journal › Article › peer-review

41 Citations (Scopus)

Abstract

Glycoprotein conformations are complex and heterogeneous. Currently, site-specific characterization of glycopeptides is a challenge. We sought to establish an efficient method of N-glycoprotein characterization using mass spectrometry (MS). Using alpha-1-acid glycoprotein (AGP) as a model N-glycoprotein, we identified its tryptic N-glycopeptides and examined the data reproducibility in seven laboratories running different LC-MS/MS platforms. We used three test samples and one blind sample to evaluate instrument performance with entire sample preparation workflow. 165 site-specific N-glycopeptides representative of all N-glycosylation sites were identified from AGP 1 and AGP 2 isoforms. The glycopeptide fragmentations by collision-induced dissociation or higher-energy collisional dissociation (HCD) varied based on the MS analyzer. Orbitrap Elite identified the greatest number of AGP N-glycopeptides, followed by Triple TOF and Q-Exactive Plus. Reproducible generation of oxonium ions, glycan-cleaved glycopeptide fragment ions, and peptide backbone fragment ions was essential for successful identification. Laboratory proficiency affected the number of identified N-glycopeptides. The relative quantities of the 10 major N-glycopeptide isoforms of AGP detected in four laboratories were compared to assess reproducibility. Quantitative analysis showed that the coefficient of variation was <25% for all test samples. Our analytical protocol yielded identification and quantification of site-specific N-glycopeptide isoforms of AGP from control and disease plasma sample.

Original language	English
Pages (from-to)	4146-4164
Number of pages	19
Journal	Journal of Proteome Research
Volume	15
Issue number	12
DOIs	https://doi.org/10.1021/acs.jproteome.5b01159
Publication status	Published - 2016 Dec 2

Bibliographical note

Publisher Copyright:
© 2016 American Chemical Society.

All Science Journal Classification (ASJC) codes

General Chemistry
Biochemistry

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10.1021/acs.jproteome.5b01159

Cite this

Lee, J. Y., Lee, H. K., Park, G. W., Hwang, H., Jeong, H. K., Yun, K. N., Ji, E. S., Kim, K. H., Kim, J. S., Kim, J. W., Yun, S. H., Choi, C. W., Kim, S. I., Lim, J. S., Jeong, S. K., Paik, Y. K., Lee, S. Y., Park, J., Kim, S. Y., ... Yoo, J. S. (2016). Characterization of Site-Specific N-Glycopeptide Isoforms of α-1-Acid Glycoprotein from an Interlaboratory Study Using LC-MS/MS. Journal of Proteome Research, 15(12), 4146-4164. https://doi.org/10.1021/acs.jproteome.5b01159

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title = "Characterization of Site-Specific N-Glycopeptide Isoforms of α-1-Acid Glycoprotein from an Interlaboratory Study Using LC-MS/MS",

abstract = "Glycoprotein conformations are complex and heterogeneous. Currently, site-specific characterization of glycopeptides is a challenge. We sought to establish an efficient method of N-glycoprotein characterization using mass spectrometry (MS). Using alpha-1-acid glycoprotein (AGP) as a model N-glycoprotein, we identified its tryptic N-glycopeptides and examined the data reproducibility in seven laboratories running different LC-MS/MS platforms. We used three test samples and one blind sample to evaluate instrument performance with entire sample preparation workflow. 165 site-specific N-glycopeptides representative of all N-glycosylation sites were identified from AGP 1 and AGP 2 isoforms. The glycopeptide fragmentations by collision-induced dissociation or higher-energy collisional dissociation (HCD) varied based on the MS analyzer. Orbitrap Elite identified the greatest number of AGP N-glycopeptides, followed by Triple TOF and Q-Exactive Plus. Reproducible generation of oxonium ions, glycan-cleaved glycopeptide fragment ions, and peptide backbone fragment ions was essential for successful identification. Laboratory proficiency affected the number of identified N-glycopeptides. The relative quantities of the 10 major N-glycopeptide isoforms of AGP detected in four laboratories were compared to assess reproducibility. Quantitative analysis showed that the coefficient of variation was <25% for all test samples. Our analytical protocol yielded identification and quantification of site-specific N-glycopeptide isoforms of AGP from control and disease plasma sample.",

keywords = "PTM (post translational modification), interlaboratory study, isoforms, site-specific N-glycopeptide",

author = "Lee, {Ju Yeon} and Lee, {Hyun Kyoung} and Park, {Gun Wook} and Heeyoun Hwang and Jeong, {Hoi Keun} and Yun, {Ki Na} and Ji, {Eun Sun} and Kim, {Kwang Hoe} and Kim, {Jun Seok} and Kim, {Jong Won} and Yun, {Sung Ho} and Choi, {Chi Won} and Kim, {Seung Il} and Lim, {Jong Sun} and Jeong, {Seul Ki} and Paik, {Young Ki} and Lee, {Soo Youn} and Jisook Park and Kim, {Su Yeon} and Choi, {Young Jin} and Kim, {Yong In} and Jawon Seo and Cho, {Je Yoel} and Oh, {Myoung Jin} and Nari Seo and An, {Hyun Joo} and Kim, {Jin Young} and Yoo, {Jong Shin}",

note = "Publisher Copyright: {\textcopyright} 2016 American Chemical Society.",

year = "2016",

month = dec,

day = "2",

doi = "10.1021/acs.jproteome.5b01159",

language = "English",

volume = "15",

pages = "4146--4164",

journal = "Journal of Proteome Research",

issn = "1535-3893",

publisher = "American Chemical Society",

number = "12",

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Lee, JY, Lee, HK, Park, GW, Hwang, H, Jeong, HK, Yun, KN, Ji, ES, Kim, KH, Kim, JS, Kim, JW, Yun, SH, Choi, CW, Kim, SI, Lim, JS, Jeong, SK, Paik, YK, Lee, SY, Park, J, Kim, SY, Choi, YJ, Kim, YI, Seo, J, Cho, JY, Oh, MJ, Seo, N, An, HJ, Kim, JY & Yoo, JS 2016, 'Characterization of Site-Specific N-Glycopeptide Isoforms of α-1-Acid Glycoprotein from an Interlaboratory Study Using LC-MS/MS', Journal of Proteome Research, vol. 15, no. 12, pp. 4146-4164. https://doi.org/10.1021/acs.jproteome.5b01159

TY - JOUR

T1 - Characterization of Site-Specific N-Glycopeptide Isoforms of α-1-Acid Glycoprotein from an Interlaboratory Study Using LC-MS/MS

AU - Lee, Ju Yeon

AU - Lee, Hyun Kyoung

AU - Park, Gun Wook

AU - Hwang, Heeyoun

AU - Jeong, Hoi Keun

AU - Yun, Ki Na

AU - Ji, Eun Sun

AU - Kim, Kwang Hoe

AU - Kim, Jun Seok

AU - Kim, Jong Won

AU - Yun, Sung Ho

AU - Choi, Chi Won

AU - Kim, Seung Il

AU - Lim, Jong Sun

AU - Jeong, Seul Ki

AU - Paik, Young Ki

AU - Lee, Soo Youn

AU - Park, Jisook

AU - Kim, Su Yeon

AU - Choi, Young Jin

AU - Kim, Yong In

AU - Seo, Jawon

AU - Cho, Je Yoel

AU - Oh, Myoung Jin

AU - Seo, Nari

AU - An, Hyun Joo

AU - Kim, Jin Young

AU - Yoo, Jong Shin

PY - 2016/12/2

Y1 - 2016/12/2

N2 - Glycoprotein conformations are complex and heterogeneous. Currently, site-specific characterization of glycopeptides is a challenge. We sought to establish an efficient method of N-glycoprotein characterization using mass spectrometry (MS). Using alpha-1-acid glycoprotein (AGP) as a model N-glycoprotein, we identified its tryptic N-glycopeptides and examined the data reproducibility in seven laboratories running different LC-MS/MS platforms. We used three test samples and one blind sample to evaluate instrument performance with entire sample preparation workflow. 165 site-specific N-glycopeptides representative of all N-glycosylation sites were identified from AGP 1 and AGP 2 isoforms. The glycopeptide fragmentations by collision-induced dissociation or higher-energy collisional dissociation (HCD) varied based on the MS analyzer. Orbitrap Elite identified the greatest number of AGP N-glycopeptides, followed by Triple TOF and Q-Exactive Plus. Reproducible generation of oxonium ions, glycan-cleaved glycopeptide fragment ions, and peptide backbone fragment ions was essential for successful identification. Laboratory proficiency affected the number of identified N-glycopeptides. The relative quantities of the 10 major N-glycopeptide isoforms of AGP detected in four laboratories were compared to assess reproducibility. Quantitative analysis showed that the coefficient of variation was <25% for all test samples. Our analytical protocol yielded identification and quantification of site-specific N-glycopeptide isoforms of AGP from control and disease plasma sample.

AB - Glycoprotein conformations are complex and heterogeneous. Currently, site-specific characterization of glycopeptides is a challenge. We sought to establish an efficient method of N-glycoprotein characterization using mass spectrometry (MS). Using alpha-1-acid glycoprotein (AGP) as a model N-glycoprotein, we identified its tryptic N-glycopeptides and examined the data reproducibility in seven laboratories running different LC-MS/MS platforms. We used three test samples and one blind sample to evaluate instrument performance with entire sample preparation workflow. 165 site-specific N-glycopeptides representative of all N-glycosylation sites were identified from AGP 1 and AGP 2 isoforms. The glycopeptide fragmentations by collision-induced dissociation or higher-energy collisional dissociation (HCD) varied based on the MS analyzer. Orbitrap Elite identified the greatest number of AGP N-glycopeptides, followed by Triple TOF and Q-Exactive Plus. Reproducible generation of oxonium ions, glycan-cleaved glycopeptide fragment ions, and peptide backbone fragment ions was essential for successful identification. Laboratory proficiency affected the number of identified N-glycopeptides. The relative quantities of the 10 major N-glycopeptide isoforms of AGP detected in four laboratories were compared to assess reproducibility. Quantitative analysis showed that the coefficient of variation was <25% for all test samples. Our analytical protocol yielded identification and quantification of site-specific N-glycopeptide isoforms of AGP from control and disease plasma sample.

KW - PTM (post translational modification)

KW - interlaboratory study

KW - isoforms

KW - site-specific N-glycopeptide

UR - http://www.scopus.com/inward/record.url?scp=85000770403&partnerID=8YFLogxK

UR - http://www.scopus.com/inward/citedby.url?scp=85000770403&partnerID=8YFLogxK

U2 - 10.1021/acs.jproteome.5b01159

DO - 10.1021/acs.jproteome.5b01159

M3 - Article

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AN - SCOPUS:85000770403

SN - 1535-3893

VL - 15

SP - 4146

EP - 4164

JO - Journal of Proteome Research

JF - Journal of Proteome Research

IS - 12

ER -

Characterization of Site-Specific N-Glycopeptide Isoforms of α-1-Acid Glycoprotein from an Interlaboratory Study Using LC-MS/MS

Abstract

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