Evaluation of Differentiated/Undifferentiated State of iPS Cells Using DPiMS™-2020 and eMSTAT Solution™
Applications | 2020 | ShimadzuInstrumentation
Evaluation of the differentiated/undifferentiated state of iPS cells is a critical parameter in regenerative medicine, impacting research reproducibility and cell therapy quality control.
This work demonstrates a fast, minimally invasive approach to characterize iPS cell differentiation by analyzing culture medium components without extensive cell handling or fractionation.
Sample Preparation:
Measurement:
Multivariate analysis of mass spectral data successfully distinguished differentiated and undifferentiated culture media. Score plots revealed clustering according to cell state and progression of differentiation, with Day 7 samples separated from Day 2.
Combining DPiMS-2020 with eMSTAT enables rapid (approximately 3 minutes per sample) and simple evaluation of cell differentiation using minimal culture medium, preserving valuable cells for downstream assays and streamlining quality control workflows.
Implementation of automated sampling, expansion to additional biomarkers, and integration with high-throughput screening could further enhance this approach’s applicability in cell manufacturing and therapeutic development.
The probe electrospray ionization mass spectrometry method coupled with multivariate analysis provides a quick, reliable tool for assessing iPS cell differentiation status, offering significant advantages for regenerative medicine research and industrial quality control.
LC/MS, DART, LC/SQ
IndustriesClinical Research
ManufacturerShimadzu
Summary
Importance of the Topic
Evaluation of the differentiated/undifferentiated state of iPS cells is a critical parameter in regenerative medicine, impacting research reproducibility and cell therapy quality control.
Objectives and Study Overview
This work demonstrates a fast, minimally invasive approach to characterize iPS cell differentiation by analyzing culture medium components without extensive cell handling or fractionation.
Methodology
Sample Preparation:
- Culture media collected at differentiation time points (Day 2 and Day 7) for undifferentiated spheroids, differentiated spheroids, and adherent differentiated cells.
- Supernatant mixed with ethanol (1:1) and 10 µL applied to a dedicated liquid sample plate.
Measurement:
- DPiMS-2020 mass spectrometer using probe electrospray ionization in scan mode to acquire mass spectra within minutes per sample.
Used Instrumentation
- DPiMS-2020 mass spectrometer equipped with probe electrospray ionization.
- eMSTAT Solution software for multivariate statistical analysis.
Main Results and Discussion
Multivariate analysis of mass spectral data successfully distinguished differentiated and undifferentiated culture media. Score plots revealed clustering according to cell state and progression of differentiation, with Day 7 samples separated from Day 2.
Benefits and Practical Applications
Combining DPiMS-2020 with eMSTAT enables rapid (approximately 3 minutes per sample) and simple evaluation of cell differentiation using minimal culture medium, preserving valuable cells for downstream assays and streamlining quality control workflows.
Future Trends and Opportunities
Implementation of automated sampling, expansion to additional biomarkers, and integration with high-throughput screening could further enhance this approach’s applicability in cell manufacturing and therapeutic development.
Conclusion
The probe electrospray ionization mass spectrometry method coupled with multivariate analysis provides a quick, reliable tool for assessing iPS cell differentiation status, offering significant advantages for regenerative medicine research and industrial quality control.
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