Subsurface tumor progression investigated by noninvasive optical second harmonic tomography

Guo, Yici; Savage, Howard E.; Lin, Feng; Schantz, Stimson P.; Ho, P. P.; Alfano, R. R.

doi:10.1073/pnas.96.19.10854

Cited by 66 publications

(41 citation statements)

References 11 publications

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“…By contrast, multiphoton microscopy in conjunction with NIR light allows for reduced photodamage and deeper sensing depth. These advantages of multiphoton microscopy, along with its z-sectioning, have been employed as an encouraging imaging method in studying of living cells (König et al, 1996;Piston, 1999), mapping ligand-gated ion channel distributions (Denk, 1994), organelles and DNA imaging (Malak et al, 1997;König et al, 2000;Dedov et al, 2001), imaging mammalian embryos (Squirrell et al, 1999), skin probing (Masters et al, 1997;So et al, 1998), imaging of tumourous tissues (Guo et al, 1999), membrane imaging and visualizing of biomolecular array Moreaux et al, 2000;Campagnola & Loew, 2003). Fluorescence spectroscopy of NAD(P)H and flavoprotein under 2-photon absorption were furthermore addressed (Huang et al, 2002).…”

Section: Keratinmentioning

confidence: 99%

Two‐photon microscopy of deep intravital tissues and its merits in clinical research

Wang

König

2010

Journal of Microscopy

180

131

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SummaryMultiphoton excitation laser scanning microscopy, relying on the simultaneous absorption of two or more photons by a molecule, is one of the most exciting recent developments in biomedical imaging. Thanks to its superior imaging capability of deeper tissue penetration and efficient light detection, this system becomes more and more an inspiring tool for intravital bulk tissue imaging. Two-photon excitation microscopy including 2-photon fluorescence and second harmonic generated signal microscopy is the most common multiphoton microscopic application. In the present review we take diverse ocular tissues as intravital samples to demonstrate the advantages of this approach. Experiments with registration of intracellular 2-photon fluorescence and extracellular collagen second harmonic generated signal microscopy in native ocular tissues are focused. Data show that the in-tandem combination of 2-photon fluorescence and second harmonic generated signal microscopy as two-modality microscopy allows for in situ co-localization imaging of various microstructural components in the whole-mount deep intravital tissues. New applications and recent developments of this high technology in clinical studies such as 2-photon-controlled drug release, in vivo drug screening and administration in skin and kidney, as well as its uses in tumourous tissues such as melanoma and glioma, in diseased lung, brain and heart are additionally reviewed. Intrinsic emission two-modal 2-photon microscopy/tomography, acting as an efficient and sensitive non-injurious imaging approach featured by high contrast and subcellular spatial resolution, has been proved to be a promising tool for intravital deep tissue imaging and clinical studies. Given the level of its performance, we believe Correspondence to B.-G. Wang. Tel: +49 3641 938496; fax: +49 3641 938552; e-mail: Baogui.Wang@mti.uni-jena.de that the non-linear optical imaging technique has tremendous potentials to find more applications in biomedical fundamental and clinical research in the near future.

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Section: Keratinmentioning

confidence: 99%

Two‐photon microscopy of deep intravital tissues and its merits in clinical research

Wang

König

2010

Journal of Microscopy

180

131

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“…The dependence of the SHG signal on tissue structure and local symmetry has been used for macroscopic mapping [20,21] . SHG was observed in type I collagen by nanosecond laser irradiation over a broad spectral region [21].…”

Section: Mpm and Second Harmonic Generation (Shg) Imagingmentioning

confidence: 99%

“…Nonlinear susceptibility is an optical property characteristic of chiral molecules. The microcrystalline structure of collagen [21][22][23][24] makes it capable of SHG [19,20]. Several researchers have reported endogenous second harmonic generation in biological tissues.…”

Section: Mpm and Second Harmonic Generation (Shg) Imagingmentioning

confidence: 99%

“…Cross-beam scanning SHG microscopy was studied in transmission geometry to show detailed variation of collagenous filaments in rat tail tendon [19]. The dependence of the SHG signal on tissue structure and local symmetry has been used for macroscopic mapping [20,21] . SHG was observed in type I collagen by nanosecond laser irradiation over a broad spectral region [21].…”

Section: Mpm and Second Harmonic Generation (Shg) Imagingmentioning

confidence: 99%

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In vivo multiphoton fluorescence imaging: A novel approach to oral malignancy

et al. 2004

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Background and Objective: Current techniques for oral diagnosis require surgical biopsy of lesions, and may fail to detect early malignant change. Non-invasive, sensitive tools providing early detection of oral cancer and a better understanding of malignant change are needed. These studies evaluated in vivo multiphoton excited fluorescence (MPM) techniques to (1) map epithelial and subepithelial changes through out oral carcinogenesis and (2) serve as an effective diagnostic modality. Study Design/Materials and Methods: In the hamster model (n ¼ 70), epithelial and subepithelial change was imaged in vivo throughout carcinogenesis. MPM-and histopathology-based diagnoses on a scale of 0 (healthy)-6 (squamous cell carcinoma [s.c.c.]) were scored by two prestandardized investigators. Results: Collagen matrix and fibers, cellular infiltrates, blood vessels, and microtumors were clearly visible. MPM agreed with the histopathology for 88.6% of diagnoses. Conclusions: In vivo MPM images provide (1) high resolution information on specific components of the carcinogenesis process (2) an excellent basis for oral diagnostics.

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“…Since SHG is dependent on the scale and the form of molecular ordering within the tissue Zipfel et al, 2003) and collagen is highly organized in the tendon, the method yields high contrast signals in that tissue. SHG has been shown to produce optically sectioned images of the plasma membrane (Campagnola et al, 2002;Peleg et al, 1999), tumor development in hamster cheek pouch mucosa (Guo et al, 1999), collagen in RAFT tissue models (Zoumi et al, 2002), and sarcomeres with the C. elegans nematode (Campagnola and Loew, 2003;Fig. 3).…”

Section: Nonlinear Imagingmentioning

confidence: 99%