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Motility imaging via optical coherence phase microscopy enables label-free monitoring of tissue growth and viability in 3D tissue-engineering scaffolds.

TitleMotility imaging via optical coherence phase microscopy enables label-free monitoring of tissue growth and viability in 3D tissue-engineering scaffolds.
Publication TypeJournal Article
Year of Publication2015
AuthorsHolmes C, Tabrizian M, Bagnaninchi PO
JournalJ Tissue Eng Regen Med
Volume9
Issue5
Pagination641-5
Date Published2015 May
ISSN1932-7005
Keywords3T3 Cells, Adipose Tissue, Animals, Cell Culture Techniques, Cell Movement, Cell Proliferation, Cell Survival, Humans, Lactic Acid, Mice, Microscopy, Phase-Contrast, Polyglycolic Acid, Polymers, Stem Cells, Tissue Engineering, Tissue Scaffolds, Tomography, Optical Coherence
Abstract

As the field of tissue engineering continues to progress, there is a deep need for non-invasive, label-free imaging technologies that can monitor tissue growth and health within thick three-dimensional (3D) constructs. Amongst the many imaging modalities under investigation, optical coherence tomography (OCT) has emerged as a promising tool, enabling non-destructive in situ characterization of scaffolds and engineered tissues. However, the lack of optical contrast between cells and scaffold materials using this technique remains a challenge. In this communication, we show that mapping the optical phase fluctuations resulting from cellular viability and motility allows for the distinction of live cells from their surrounding scaffold environment. Motility imaging was performed via a common-path optical coherence phase microscope (OCPM), an OCT modality that has been shown to be sensitive to nanometer-level fluctuations. More specifically, we examined the development of human adipose-derived stem cells and/or murine pre-osteoblasts within two distinct scaffold systems, commercially available alginate sponges and custom-microfabricated poly(d, l-lactic-co-glycolic acid) fibrous scaffolds. Cellular motility is demonstrated as an endogenous source of contrast for OCPM, enabling real-time, label-free monitoring of 3D engineered tissue development.

DOI10.1002/term.1687
Alternate JournalJ Tissue Eng Regen Med
PubMed ID23401413
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