Diagnosing 12 prostate needle cores within an hour of biopsy via open-top light-sheet microscopy

Xie, Weisi; Glaser, Adam K.; Vakar-López, Funda; Wright, Jonathan L.; Reder, Nicholas P.; Liu, Jonathan; True, Lawrence D.

doi:10.1117/1.jbo.25.12.126502

Cited by 19 publications

(21 citation statements)

References 20 publications

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“…By taking advantage of fluorescence counterstaining, we were able to acquire strong fluorescence signals with an emission spectrum distinct from that achievable with immunofluorescence. Although several fluorescence microscopy techniques based on the use of nucleic acid staining dyes have been described for assessing prostate needle biopsies, 23,24 the proSTAT workflow met the requirements for a complete analysis of the specimen with membrane staining and IHC. Specifically, the integration of a lipophilic tracer and p63 immunostaining was of great benefit not only for the distinction between malignant and benign lesions but also for avoiding alternative radiation-based techniques (e.g., microCT).…”

Section: Discussionmentioning

confidence: 99%

Rapid Histological Assessment of Prostate Specimens in the Three-dimensional Space by Hydrophilic Tissue Clearing and Confocal Microscopy

Peng

Lin

Hung

et al. 2022

J Histochem Cytochem.

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Microscopic examination of biopsied and resected prostatic specimens is the mainstay in the diagnosis of prostate cancer. However, conventional analysis of hematoxylin and eosin (H&E)-stained tissue is time-consuming and offers limited two-dimensional (2D) information. In the current study, we devised a method—termed Prostate Rapid Optical examination for cancer STATus (proSTAT)—for rapid screening of prostate cancer using high-resolution 2D and three-dimensional (3D) confocal images obtained after hydrophilic tissue clearing of 100-µm-thick tissue slices. The results of the proSTAT method were compared with those of traditional H&E stains for the analysis of cores ( n=15) obtained from radical prostatectomy specimens ( n=5). Gland lumen formation, consistent with Gleason pattern 3, was evident following tracking of multiple optical imaging sections. In addition, 3D rendering allowed visualizing a tubular network of interconnecting branches. Rapid 3D fluorescent labeling of tumor protein p63 accurately distinguished prostate adenocarcinoma from normal tissue and benign lesions. Compared with conventional stains, the 3D spatial and molecular information extracted from proSTAT may significantly increase the amount of available data for pathological assessment of prostate specimens. Our approach is amenable to automation and—subject to independent validation—can find a wide spectrum of clinical and research applications.

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Section: Discussionmentioning

confidence: 99%

Rapid Histological Assessment of Prostate Specimens in the Three-dimensional Space by Hydrophilic Tissue Clearing and Confocal Microscopy

Peng

Lin

Hung

et al. 2022

J Histochem Cytochem.

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“…With additional multimagnification, multiimmersion, and rapid optical-clearing features, this optical design has demonstrated extraordinary performance and usability in 3D histopathology samples with a wide range of geometries. 64,78 Deep, Vibrant CellsdFull-Field Optical Coherence Tomography Fluorescence microscopy often depends on extrinsic staining for the generation of optical contrast. Although the staining procedures of most slide-free histopathology techniques are simple, fast, and minimally affect the quality of the sample, any extra manual steps present potential burdens in a clinical process.…”

Section: Slide-free Histopathologymentioning

confidence: 99%

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Liu

Levenson

Jenkins

2022

The American Journal of Pathology

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Conventional analysis using clinical histopathology is based on bright-field microscopy of thinly sliced tissue specimens. Although bright-field microscopy is a simple and robust method of examining microscope slides, the preparation of the slides needed is a lengthy and labor-intensive process. Slide-free histopathology, however, uses direct imaging of intact, minimally processed tissue samples using advanced optical-imaging systems, bypassing the extended workflow now required for the preparation of tissue sections. This article explains the technical basis of slide-free microscopy, reviews common slide-free optical microscopy techniques, and discusses the opportunities and challenges involved in clinical implementation.

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“… 6 , 7 , 8 Light-sheet microscopy (LSM) achieves optical sectioning by a thin “selective” illumination plane and the signal collection from the orthogonal direction. 9 , 10 , 11 , 12 Although these technologies can be applied to the pathological assessment of thick tissues and shorten turnaround time, fluorescence labeling is still required to provide image contrast. Fluorescence labeling is challenging to be integrated into the current clinical practice, especially intraoperative pathological examination.…”

Section: Introductionmentioning

confidence: 99%

Rapid and label-free histological imaging of unprocessed surgical tissues via dark-field reflectance ultraviolet microscopy

Zou

Huang

et al. 2023

iScience

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Diagnosing 12 prostate needle cores within an hour of biopsy via open-top light-sheet microscopy

Cited by 19 publications

References 20 publications

Rapid Histological Assessment of Prostate Specimens in the Three-dimensional Space by Hydrophilic Tissue Clearing and Confocal Microscopy

Rapid Histological Assessment of Prostate Specimens in the Three-dimensional Space by Hydrophilic Tissue Clearing and Confocal Microscopy

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Rapid and label-free histological imaging of unprocessed surgical tissues via dark-field reflectance ultraviolet microscopy

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