Absolute quantification of viral proteins during single-round replication of MDCK suspension cells

Jan Küchler; Sebastian Püttker; Patrick Lahmann; Yvonne Genzel; Sascha Kupke; Dirk Benndorf; Udo Reichl

doi:10.1016/j.jprot.2022.104544

Absolute quantification of viral proteins during single-round replication of MDCK suspension cells

J Proteomics. 2022 May 15:259:104544. doi: 10.1016/j.jprot.2022.104544. Epub 2022 Mar 1.

Authors

Jan Küchler¹, Sebastian Püttker², Patrick Lahmann², Yvonne Genzel³, Sascha Kupke³, Dirk Benndorf⁴, Udo Reichl⁴

Affiliations

¹ Bioprocess Engineering, Max Planck Institute for Dynamics of Complex Technical Systems, Magdeburg, Germany. Electronic address: kuechler@mpi-magdeburg.mpg.de.
² Bioprocess Engineering, Otto von Guericke University Magdeburg, Magdeburg, Germany.
³ Bioprocess Engineering, Max Planck Institute for Dynamics of Complex Technical Systems, Magdeburg, Germany.
⁴ Bioprocess Engineering, Max Planck Institute for Dynamics of Complex Technical Systems, Magdeburg, Germany; Bioprocess Engineering, Otto von Guericke University Magdeburg, Magdeburg, Germany.

PMID: 35240312
DOI: 10.1016/j.jprot.2022.104544

Abstract

Madin-Darby canine kidney (MDCK) cells are widely used in basic research and for the propagation of influenza A viruses (IAV) for vaccine production. To identify targets for antiviral therapies and to optimize vaccine manufacturing, a detailed understanding of the viral life cycle is important. This includes the characterization of virus entry, the synthesis of the various viral RNAs and proteins, the transfer of viral compounds in the cell and virus budding. In case quantitative information is available, the analysis can be complemented by mathematical modelling approaches. While comprehensive studies focusing on IAV entry as well as viral mRNA, vRNA and cRNA accumulation in the nucleus of cells have been performed, quantitative data regarding IAV protein synthesis and accumulation was mostly lacking. In this study, we present a mass spectrometry (MS)-based method to evaluate whether an absolute quantification of viral proteins is possible for single-round replication in suspension MDCK cells. Using influenza A/PR/8/34 (H1N1, RKI) as a model strain at a multiplicity of infection of ten, defined amounts of isotopically labelled peptides of synthetic origin of four IAV proteins (hemagglutinin, neuraminidase, nucleoprotein, matrix protein 1) were added as an internal standard before tryptic digestion of samples for absolute quantification (AQUA). The first intracellular protein detected was NP at 1 h post infection (hpi). A maximum extracellular concentration of 7.7E+12 copies/mL was achieved. This was followed by hemagglutinin (3 hpi, maximum 4.1E+12 copies/mL at 13 hpi), matrix protein 1 (5 hpi, maximum 2.2E+12 copies/mL at 13 hpi) and neuraminidase (5 hpi, 6.0E+11 copies/mL at 13 hpi). In sum, for the first time absolute IAV protein copy numbers were quantified by a MS-based method for infected MDCK cells providing important insights into viral protein dynamics during single-round virus replication. SIGNIFICANCE: Influenza A virus is a significant human pathogen worldwide. To improve therapies against influenza and overcome bottlenecks in vaccine production in cell culture, it is critical to gain a detailed understanding of the viral life cycle. In addition to qPCR-based models, this study will examine the dynamics of influenza virus proteins during infection of producer cells to gain initial insights into changes in absolute copy numbers.

Keywords: AQUA peptides; Absolute quantification; Influenza a virus; MDCK cells.

MeSH terms

Animals
Dogs
Hemagglutinins / metabolism
Humans
Influenza A Virus, H1N1 Subtype* / metabolism
Influenza A virus* / chemistry
Influenza A virus* / genetics
Influenza A virus* / metabolism
Influenza, Human*
Madin Darby Canine Kidney Cells
Neuraminidase / genetics
Neuraminidase / metabolism
Viral Proteins / metabolism
Virus Replication

Substances

Hemagglutinins
Viral Proteins
Neuraminidase