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Online μSEC2-nRPLC-MS for improved sensitivity of intact protein detection of IEF separated non-human primate cerebrospinal fluid proteins

View ORCID ProfileErika N. Cline, Carina Alvarez, Jiana Duan, View ORCID ProfileSteven M. Patrie
doi: https://doi.org/10.1101/2021.06.08.447575
Erika N. Cline
*Department of Chemistry and the Proteomics Center of Excellence, Northwestern University, 2145 Sheridan Rd, Evanston, IL 60208, Email: ; Telephone: 847-491-3731
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  • For correspondence: steven.patrie@northwestern.edu
Carina Alvarez
*Department of Chemistry and the Proteomics Center of Excellence, Northwestern University, 2145 Sheridan Rd, Evanston, IL 60208, Email: ; Telephone: 847-491-3731
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  • For correspondence: steven.patrie@northwestern.edu
Jiana Duan
*Department of Chemistry and the Proteomics Center of Excellence, Northwestern University, 2145 Sheridan Rd, Evanston, IL 60208, Email: ; Telephone: 847-491-3731
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  • For correspondence: steven.patrie@northwestern.edu
Steven M. Patrie
*Department of Chemistry and the Proteomics Center of Excellence, Northwestern University, 2145 Sheridan Rd, Evanston, IL 60208, Email: ; Telephone: 847-491-3731
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  • For correspondence: steven.patrie@northwestern.edu steven.patrie@northwestern.edu
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ABSTRACT

Proteoform-resolved information, obtained by top-down (TD) “intact protein” proteomics, is expected to contribute substantially to the understanding of molecular pathogenic mechanisms and in turn, identify novel therapeutic and diagnostic targets. However, the robustness of mass spectrometry (MS) analysis of intact proteins in complex biological samples is hindered by high dynamic range in protein concentration and mass, protein instability, and buffer complexity. Here, we describe an evolutionary step for intact protein investigations through the online implementation of tandem microflow size exclusion chromatography with nanoflow reversed-phase liquid chromatography and MS (μSEC2-nRPLC-MS). Online serial high-/low-pass SEC filtration overcomes the aforementioned hurdles to intact proteomic analysis through automated sample desalting/cleanup and enrichment of target mass ranges (5-155 kDa) prior to nRPLC-MS. The coupling of μSEC to nRPLC is achieved through a novel injection volume control (IVC) strategy of inserting protein trap columns pre- and post-μSEC columns to enable injection of dilute samples in high volumes without loss of sensitivity or resolution. Critical characteristics of the approach are tested via rigorous investigations on samples of varied complexity and chemical background. Application of the platform to cerebrospinal fluid (CSF) pre-fractionated by OFFGEL isoelectric focusing drastically increases the number of intact mass tags (IMTs) detected within the target mass range (5-30 kDa) in comparison to one-dimensional nRPLC-MS with approximately 100x less CSF than previous OFFGEL studies. Furthermore, the modular design of the μSEC2-nRPLC-MS platform is robust and promises significant flexibility for large-scale TDMS analysis of diverse samples either directly or in concert with other multidimensional fractionation steps.

Competing Interest Statement

The authors have declared no competing interest.

Footnotes

  • This includes two new supplemental figures (S5 & S7) regarding application of our platform for detection of proteins >30 kDa, as well as, justification of the need for multi-dimensional workflows over 1D RPLC for detection of glycoproteoforms <30 kDa.

Copyright 
The copyright holder for this preprint is the author/funder, who has granted bioRxiv a license to display the preprint in perpetuity. All rights reserved. No reuse allowed without permission.
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Posted September 16, 2021.
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Online μSEC2-nRPLC-MS for improved sensitivity of intact protein detection of IEF separated non-human primate cerebrospinal fluid proteins
Erika N. Cline, Carina Alvarez, Jiana Duan, Steven M. Patrie
bioRxiv 2021.06.08.447575; doi: https://doi.org/10.1101/2021.06.08.447575
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Online μSEC2-nRPLC-MS for improved sensitivity of intact protein detection of IEF separated non-human primate cerebrospinal fluid proteins
Erika N. Cline, Carina Alvarez, Jiana Duan, Steven M. Patrie
bioRxiv 2021.06.08.447575; doi: https://doi.org/10.1101/2021.06.08.447575

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