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Evaluation of Undifferentiated State of Human iPS Cells Using C2MAP™ Cell Culture Media Analysis Platform

Applications | 2020 | ShimadzuInstrumentation
LC/MS, LC/MS/MS, LC/QQQ
Industries
Clinical Research
Manufacturer
Shimadzu

Summary

Importance of the Topic


The ability to evaluate human induced pluripotent stem cell (iPS) status non invasively using culture supernatant analysis addresses a key bottleneck in regenerative medicine and cell manufacturing. Conventional evaluations rely on invasive gene expression assays that disrupt cells and only provide terminal readouts.

Objectives and Study Overview


This study aimed to develop a non disruptive method for real time assessment of iPS cell undifferentiation and ectodermal differentiation. Using the C2MAP cell culture media analysis platform with LC MS MS, 95 medium components were monitored and statistical tools were applied to identify candidate biomarkers in supernatants.

Methodology


Human iPS cells were cultured in TeSR E8 medium on vitronectin N coated 6 well plates with daily medium replacement. Differentiation stimuli targeting each germ layer were applied by adding specific factors. Culture supernatants were collected daily for six days. Samples were processed and analyzed automatically on the Shimadzu C2MAP LC MS MS system. Data were interrogated using C2MAP TRENDS viewer and the Multi omics Analysis Gadget Package for volcano plot comparisons and time course profiling.

Used Instrumentation


  • Shimadzu C2MAP cell culture media analysis platform
  • Shimadzu LC MS MS system for simultaneous multi component quantitation
  • C2MAP TRENDS viewer software for statistical analysis
  • Multi omics Analysis Gadget Package for biomarker discovery

Key Results and Discussion


Out of 95 targets, 55 metabolites were reliably detected in culture supernatants. Volcano plot analysis highlighted kynurenine as a marker of the undifferentiated state and 2 aminoadipic acid as a marker of ectodermal differentiation. Time course data showed progressive tryptophan consumption and increased kynurenine secretion in undifferentiated cultures, while 2 aminoadipic acid accumulated during ectodermal differentiation.

Inhibition of IDO1 suppressed kynurenine production and impaired undifferentiated iPS cell growth. Blocking the aryl hydrocarbon receptor AhR likewise reduced kynurenine secretion and down regulated pluripotency transcription factors POU5F1 NANOG and EP300. For ectodermal cultures, KAT2 inhibition decreased 2 aminoadipic acid secretion and attenuated lineage specific gene expression. These findings support a model in which tryptophan metabolism through kynurenine AhR signaling maintains pluripotency, whereas differentiation stimuli redirect kynurenine flux toward 2 aminoadipic acid formation to initiate lineage commitment.

Benefits and Practical Applications


This non invasive approach enables continuous monitoring of stem cell status without sacrificing cells. It can serve as a quality control tool in cell production workflows, reducing reliance on destructive assays and accelerating process optimization for research and commercial cell therapies.

Future Trends and Opportunities


Expanding the panel of monitored metabolites and integrating online supernatant sampling could enable real time feedback control of culture conditions. Combining this method with transcriptomic or proteomic data may further refine biomarker signatures. Applications may extend to other stem cell types disease models and large scale biomanufacturing quality assurance.

Conclusion


This study demonstrates that simultaneous multi component LC MS MS analysis of iPS cell culture supernatants using C2MAP can identify metabolic biomarkers for undifferentiation and ectodermal differentiation. Kynurenine and 2 aminoadipic acid serve as robust non invasive indicators of cell state, offering a practical solution for ongoing monitoring in regenerative medicine applications.

Reference


1. Yamamoto T Hatabayashi K Arita M Yajima N Takenaka C Suzuki T Takahashi M Oshima Y Hara K Kagawa K Kawamata S Kynurenine signaling through the aryl hydrocarbon receptor maintains the undifferentiated state of human embryonic stem cells Sci Signal 2019 12 586 eaaw3306

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