3.9 Article

Nondestructive imaging of live human keloid and facial tissue using multiphoton microscopy

Journal

ARCHIVES OF FACIAL PLASTIC SURGERY
Volume 10, Issue 1, Pages 38-43

Publisher

AMER MEDICAL ASSOC
DOI: 10.1001/archfacial.2007.18

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Funding

  1. NCRR NIH HHS [P41RR01192, P41 RR001192] Funding Source: Medline
  2. NIDCD NIH HHS [R03 DC005572, DC005572] Funding Source: Medline
  3. NATIONAL CENTER FOR RESEARCH RESOURCES [P41RR001192] Funding Source: NIH RePORTER
  4. NATIONAL INSTITUTE ON DEAFNESS AND OTHER COMMUNICATION DISORDERS [R03DC005572] Funding Source: NIH RePORTER

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Objectives: To use multiphoton microscopy to image collagen fibers and matrix structure in nonfixed human keloid tissue and normal human facial skin obtained following surgery and to compare the findings to existing knowledge of normal skin and keloid morphology to determine if this technology is a suitable adjunct for conventional histology. Methods: Epidermis was removed to expose the fibroblast-rich dermal layer that was then imaged using a multiphoton confocal microscope (Zeiss-Meta 510; Carl Zeiss, Jena, Germany). An 800-nm tunable titanium/sapphire femtosecond laser (Mai-Tai; Newport Co Spectra-Physics, Mountain View, California) was used to excite the tissues second harmonic generation between 397 and 408 nm and autofluorescent signals were collected. Images were obtained using a Plan-Neofluar x 40 oil immersion objective lens and a Plan-Apochromat x 63 oil immersion lens. Results: Compared with normal skin, keloids showed disorganized collagen fibers arranged in complex swirls and bundles 20 to 30 pm in diameter. Normal tissue showed collagen fibers as distinct, straight strands less than 10 pm in diameter. Differences between normal and keloid tissue were subtle but apparent. Conclusions: The value of imaging living tissue is a significant benefit. Because keloids and hypertrophic scars result from altered collagen metabolism, the development of clinical multiphoton microscopy systems may allow examination of wound healing dynamics in vivo and potentially provides a means to monitor therapy without the need for biopsy or the risk of injury to tissue.

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