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13C Glucose Qualitative Flux Analysis in HepG2 cells

Applications | 2020 | Agilent TechnologiesInstrumentation
LC/TOF, LC/HRMS, LC/MS, LC/MS/MS
Industries
Metabolomics
Manufacturer
Agilent Technologies

Summary

Importance of the topic


Stable isotope tracing provides unique insights into intracellular metabolic fluxes that are hidden by concentration-based metabolomic profiling. By following 13C labels, researchers can assess pathway activity, anaplerotic contributions and enzyme function, enabling a more precise understanding of cellular metabolism in health and disease.

Objectives and study overview


This study demonstrates a qualitative flux analysis workflow in human HepG2 liver carcinoma cells. Using uniformly labeled U-13C glucose as a tracer, the aim was to investigate how pyruvate carboxylase (PC) knockdown alters glucose oxidation and TCA cycle dynamics. Data acquisition was performed on an Agilent 6546 LC/Q-TOF system and processed with Agilent MassHunter VistaFlux software.

Methodology and instrumentation


Cells with siRNA-mediated PC knockdown and control lines were incubated with U-13C glucose for 30 minutes. Metabolites were extracted by methanol-chloroform-water partitioning and analyzed by hydrophilic interaction chromatography (HILIC) coupled to high-resolution Q-TOF mass spectrometry.

Used instrumentation:
  • Agilent 1290 Infinity II UHPLC system with InfinityLab Poroshell 120 HILIC-Z column
  • Agilent 6546 LC/Q-TOF with Jet Stream electrospray source
  • MassHunter Acquisition v10.0, Profinder v10.0, Omix Premium v1.9.30, PCDL Manager B.08, Pathways to PCDL B.08

Main results and discussion


The 6546 Q-TOF delivered high mass resolution (>40,000) and isotope ratio fidelity (<5% CV), reducing interference and enabling confident isotopologue detection. Malate and citrate measurements showed robust reproducibility across technical replicates. In control HepG2 cells, citrate exhibited ~50% 13C enrichment, whereas PC-deficient cells displayed ~25%, indicating reduced pyruvate-driven anaplerosis.

Visualization in Omix Premium revealed dominant m+2 and m+3 labeling patterns after short U-13C glucose exposure. Glutamate isotopologue profiles indicated elevated unlabeled pools in PC knockdown cells, confirming reliance on alternative anaplerotic substrates when PC activity is suppressed.

Benefits and practical applications


The combined Agilent 6546 LC/Q-TOF and VistaFlux workflow offers:
  • Accurate isotope correction and throughput for qualitative flux studies
  • Automated feature extraction and pathway mapping
  • High confidence in metabolite identification and isotopologue quantitation

This approach supports drug development, cancer metabolism research, and quality control in bioproduction.

Future trends and opportunities


Advancements may include integration with quantitative flux analysis, expanded compound libraries, real-time flux monitoring, and machine-learning-driven data interpretation. Coupling multi-omic layers (proteomics, transcriptomics) will further enhance metabolic pathway elucidation.

Conclusion


The Agilent 6546 LC/Q-TOF paired with VistaFlux software constitutes a powerful platform for qualitative 13C flux analysis. Application to PC knockdown HepG2 cells revealed significant reductions in glucose-driven TCA cycle flux and increased dependence on alternative anaplerotic routes.

References


  • Phannasil P.; et al. Mass spectrometry analysis shows the biosynthetic pathways supported by pyruvate carboxylase in highly invasive breast cancer cells. Biochimica et Biophysica Acta, 2017, 1863(2), 537–551.
  • Hsiao J. J.; et al. Monitoring of Mammalian Cell Culture Media with HILIC LC/MS. Agilent Technologies Application Note, 5994-0024EN, 2018.

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