3D histopathology of human tumours by fast clearing and ultramicroscopy

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作者
Inna Sabdyusheva Litschauer
Klaus Becker
Saiedeh Saghafi
Simone Ballke
Christine Bollwein
Meraaj Foroughipour
Julia Gaugeler
Massih Foroughipour
Viktória Schavelová
Viktória László
Balazs Döme
Christine Brostjan
Wilko Weichert
Hans-Ulrich Dodt
机构
[1] TU Wien,Department of Bioelectronics
[2] Medical University of Vienna,Center for Brain Research
[3] Medical University of Vienna,Department of Surgery, Anna Spiegel Center of Translational Research
[4] TUM School of Medicine,Institute of Pathology
[5] Technical University of Munich,undefined
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Here, we describe a novel approach that allows pathologists to three-dimensionally analyse malignant tissues, including the tumour-host tissue interface. Our visualization technique utilizes a combination of ultrafast chemical tissue clearing and light-sheet microscopy to obtain virtual slices and 3D reconstructions of up to multiple centimetre sized tumour resectates. For the clearing of tumours we propose a preparation technique comprising three steps: (a) Fixation and enhancement of tissue autofluorescence with formalin/5-sulfosalicylic acid. (b) Ultrafast active chemical dehydration with 2,2-dimethoxypropane and (c) refractive index matching with dibenzyl ether at up to 56 °C. After clearing, the tumour resectates are imaged. The images are computationally post-processed for contrast enhancement and artefact removal and then 3D reconstructed. Importantly, the sequence a–c is fully reversible, allowing the morphological correlation of one and the same histological structures, once visualized with our novel technique and once visualized by standard H&E- and IHC-staining. After reverting the clearing procedure followed by standard H&E processing, the hallmarks of ductal carcinoma in situ (DCIS) found in the cleared samples could be successfully correlated with the corresponding structures present in H&E and IHC staining. Since the imaging of several thousands of optical sections is a fast process, it is possible to analyse a larger part of the tumour than by mechanical slicing. As this also adds further information about the 3D structure of malignancies, we expect that our technology will become a valuable addition for histological diagnosis in clinical pathology.
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