Literature DB >> 11421069

Autofluorescence microscopy of fresh cervical-tissue sections reveals alterations in tissue biochemistry with dysplasia.

R Drezek1, C Brookner, I Pavlova, I Boiko, A Malpica, R Lotan, M Follen, R Richards-Kortum.   

Abstract

Fluorescence spectroscopy offers an effective, noninvasive approach to the detection of precancers in multiple organ sites. Clinical studies have demonstrated that fluorescence spectroscopy can provide highly sensitive, specific and cost-effective diagnosis of cervical precancers. However, the underlying biochemical mechanisms responsible for differences in the fluorescence spectra of normal and dysplastic tissue are not fully understood. We designed a study to assess the differences in autofluorescence of normal and dysplastic cervical tissue. Transverse, fresh tissue sections were prepared from colposcopically normal and abnormal biopsies in a 34-patient study. Autofluorescence images were acquired at 380 and 460 nm excitation. Results showed statistically significant increases in epithelial fluorescence intensity (arbitrary units) at 380 nm excitation in dysplastic tissue (106 +/- 39) relative to normal tissue (85 +/- 30). The fluorophore responsible for this increase is possibly reduced nicotinamide adenine dinucleotide. Stromal fluorescence intensities in the dysplastic samples decreased at both 380 nm (102 +/- 34 [dysplasia] vs 151 +/- 44 [normal]) and 460 nm excitation (93 +/- 35 [dysplasia] vs 137 +/- 49 [normal]), wavelengths at which collagen is excited. Decreased redox ratio (17-40% reduction) in dysplastic tissue sections, indicative of increased metabolic activity, was observed in one-third of the paired samples. These results provide valuable insight into the biological basis of the differences in fluorescence of normal and precancerous cervical tissue.

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Year:  2001        PMID: 11421069     DOI: 10.1562/0031-8655(2001)073<0636:AMOFCT>2.0.CO;2

Source DB:  PubMed          Journal:  Photochem Photobiol        ISSN: 0031-8655            Impact factor:   3.421


  58 in total

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2.  Experimental recovery of intrinsic fluorescence and fluorophore concentration in the presence of hemoglobin: spectral effect of scattering and absorption on fluorescence.

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3.  Detection and diagnosis of oral neoplasia with an optical coherence microscope.

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Review 4.  Molecular contrast optical coherence tomography: a review.

Authors:  Changhuei Yang
Journal:  Photochem Photobiol       Date:  2005 Mar-Apr       Impact factor: 3.421

5.  In vivo multiphoton microscopy of NADH and FAD redox states, fluorescence lifetimes, and cellular morphology in precancerous epithelia.

Authors:  Melissa C Skala; Kristin M Riching; Annette Gendron-Fitzpatrick; Jens Eickhoff; Kevin W Eliceiri; John G White; Nirmala Ramanujam
Journal:  Proc Natl Acad Sci U S A       Date:  2007-11-27       Impact factor: 11.205

6.  Autofluorescence and diffuse reflectance spectroscopy of oral epithelial tissue using a depth-sensitive fiber-optic probe.

Authors:  Richard A Schwarz; Wen Gao; Dania Daye; Michelle D Williams; Rebecca Richards-Kortum; Ann M Gillenwater
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Review 7.  Fluorescence lifetime imaging microscopy in the medical sciences.

Authors:  René Ebrecht; Craig Don Paul; Fred S Wouters
Journal:  Protoplasma       Date:  2014-01-04       Impact factor: 3.356

8.  Real-time snapshot hyperspectral imaging endoscope.

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9.  Clinical label-free biochemical and metabolic fluorescence lifetime endoscopic imaging of precancerous and cancerous oral lesions.

Authors:  Elvis Duran-Sierra; Shuna Cheng; Rodrigo Cuenca-Martinez; Bilal Malik; Kristen C Maitland; Y S Lisa Cheng; John Wright; Beena Ahmed; Jim Ji; Mathias Martinez; Moustafa Al-Khalil; Hussain Al-Enazi; Javier A Jo
Journal:  Oral Oncol       Date:  2020-04-02       Impact factor: 5.337

Review 10.  Optical imaging for cervical cancer detection: solutions for a continuing global problem.

Authors:  Nadhi Thekkek; Rebecca Richards-Kortum
Journal:  Nat Rev Cancer       Date:  2008-09       Impact factor: 60.716

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