Direct monitoring of single-cell response to biomaterials by Raman spectroscopy

Mary Josephine McIvor; Preetam K Sharma; Catherine E Birt; Hayley McDowell; Shannon Wilson; Stephen McKillop; Jonathan G Acheson; Adrian R Boyd; Brian J Meenan

doi:10.1007/s10856-021-06624-5

Direct monitoring of single-cell response to biomaterials by Raman spectroscopy

J Mater Sci Mater Med. 2021 Dec 4;32(12):148. doi: 10.1007/s10856-021-06624-5.

Authors

Mary Josephine McIvor¹, Preetam K Sharma^{2

3}, Catherine E Birt², Hayley McDowell², Shannon Wilson², Stephen McKillop², Jonathan G Acheson², Adrian R Boyd², Brian J Meenan²

Affiliations

¹ Nanotechnology and Integrated Bioengineering Centre (NIBEC), School of Engineering, University of Ulster, Shore Road, Newtownabbey, Co. Antrim, BT37 0QB, Northern Ireland, UK. mj.mcivor@ulster.ac.uk.
² Nanotechnology and Integrated Bioengineering Centre (NIBEC), School of Engineering, University of Ulster, Shore Road, Newtownabbey, Co. Antrim, BT37 0QB, Northern Ireland, UK.
³ Department of Chemical Engineering, Loughborough University, Loughborough, LE11 3TU, England, UK.

Abstract

There is continued focus on the development of new biomaterials and associated biological testing methods needed to reduce the time taken for their entry to clinical use. The application of Raman spectroscopy to the study of individual cells that have been in contact with biomaterials offers enhanced in vitro information in a potentially non-destructive testing regime. The work presented here reports the Raman spectral analysis of discreet U-2 OS bone cells after exposure to hydroxyapatite (HA) coated titanium (Ti) substrates in both the as-deposited and thermally annealed states. These data show that cells that were in contact with the bioactive HA surface for 7 days had spectral markers similar to those cultured on the Ti substrate control for the same period. However, the spectral features for those cells that were in contact with the annealed HA surface had indicators of significant differentiation at day 21 while cells on the as-deposited surface did not show these Raman changes until day 28. The cells adhered to pristine Ti control surface showed no spectral changes at any of the timepoints studied. The validity of these spectroscopic results has been confirmed using data from standard in vitro cell viability, adhesion, and proliferation assays over the same 28-day culture period. In this case, cell maturation was evidenced by the formation of natural bone apatite, which precipitated intracellularly for cells exposed to both types of HA-coated Ti at 21 and 28 days, respectively. The properties of the intracellular apatite were markedly different from that of the synthetic HA used to coat the Ti substrate with an average particle size of 230 nm, a crystalline-like shape and Ca/P ratio of 1.63 ± 0.5 as determined by SEM-EDX analysis. By comparison, the synthetic HA particles used as a control had an average size of 372 nm and were more-rounded in shape with a Ca/P ratio of 0.8 by XPS analysis and 1.28 by SEM-EDX analysis. This study shows that Raman spectroscopy can be employed to monitor single U-2 OS cell response to biomaterials that promote cell maturation towards de novo bone thereby offering a label-free in vitro testing method that allows for non-destructive analyses.

MeSH terms

Biocompatible Materials
Biomarkers
Bone and Bones / cytology*
Cell Line
Durapatite / pharmacology*
Humans
Materials Testing
Single-Cell Analysis*
Spectrum Analysis, Raman*
Titanium / pharmacology*

Substances

Biocompatible Materials
Biomarkers
Durapatite
Titanium