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Isolating stem cells in the inter-follicular epidermis employing synchrotron radiation-based Fourier-transform infrared microspectroscopy and focal plane array imaging
Authors:Imran I. Patel  Wesley J. Harrison  Jemma G. Kerns  Jacob Filik  Katia Wehbe  Paul L. Carmichael  Andrew D. Scott  Mike P. Philpott  Mark D. Frogley  Gianfelice Cinque  Francis L. Martin
Affiliation:1. Centre for Biophotonics, Lancaster Environment Centre, Lancaster University, Bailrigg, Lancaster, LA1 4YQ, UK
2. Centre for Cutaneous Research, Barts and The London, Queen Mary’s School of Medicine and Dentistry, London, E1 2AD, UK
3. Diamond Light Source Ltd, Diamond House, Harwell Science and Innovation Campus, Didcot, OX11 0DE, UK
4. Safety and Environmental Assurance Centre, Unilever Colworth Science Park, Bedfordshire, MK44 1LQ, UK
Abstract:Normal function and physiology of the epidermis is maintained by the regenerative capacity of this tissue via adult stem cells (SCs). However, definitive identifying markers for SCs remain elusive. Infrared (IR) spectroscopy exploits the ability of cellular biomolecules to absorb in the mid-IR region (λ?=?2.5–25?μm), detecting vibrational transitions of chemical bonds. In this study, we exploited the cell’s inherent biochemical composition to discriminate SCs of the inter-follicular skin epidermis based on IR-derived markers. Paraffin-embedded samples of human scalp skin (n?=?4) were obtained, and 10-μm thick sections were mounted for IR spectroscopy. Samples were interrogated in transmission mode using synchrotron radiation-based Fourier-transform IR (FTIR) microspectroscopy (15?×?15?μm) and also imaged employing globar-source FTIR focal plane array (FPA) imaging (5.4?×?5.4?μm). Dependent on the location of derived spectra, wavenumber–absorbance/intensity relationships were examined using unsupervised principal component analysis. This approach showed clear separation and spectral differences dependent on cell type. Spectral biomarkers concurrently associated with segregation of SCs, transit-amplifying cells and terminally-differentiated cells of epidermis were primarily PO 2 ? vibrational modes (1,225 and 1,080?cm?1), related to DNA conformational alterations. FPA imaging coupled with hierarchical cluster analysis also indicated the presence of specific basal layer cells potentially originating from the follicular bulge, suggested by co-clustering of spectra. This study highlights PO 2 ? vibrational modes as potential putative SC markers.
Figure
“Delineating the putative stem cell lineage in interfollicular skin based on position-derived infrared spectral fingerprints”.
Keywords:
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