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Article type: Research Article
Authors: Wang, Xingwei | Chen, Xiaodong | Li, Yuhua | Liu, Hong | Li, Shibo | Zhang, Roy R. | Zheng, Bin
Affiliations: Department of Radiology, University of Pittsburgh, Pittsburgh, PA, USA | Department of Electrical and Computer Engineering, University of Oklahoma, Norman, OK, USA | Department of Pediatrics, University of Oklahoma Health Sciences Center, Oklahoma, OK, USA
Note: [] Corresponding author. Hong Liu, Department of Electrical and Computer Engineering, University of Oklahoma, 202 West Boyd St. Room 219, Norman, OK 73019, USA. Tel.: +1 405 325 4286; Fax: +1 405 325 7066; E-mail: liu@ou.edu
Abstract: Fluorescence in situ hybridization (FISH) tests provide promising molecular imaging biomarkers to more accurately and reliably detect and diagnose cancers and genetic disorders. Since current manual FISH signal analysis is low-efficient and inconsistent, which limits its clinical utility, developing automated FISH image scanning systems and computer-aided detection (CAD) schemes has been attracting research interests. To acquire high-resolution FISH images in a multi-spectral scanning mode, a huge amount of image data with the stack of the multiple three-dimensional (3-D) image slices is generated from a single specimen. Automated preprocessing these scanned images to eliminate the non-useful and redundant data is important to make the automated FISH tests acceptable in clinical applications. In this study, a dual-detector fluorescence image scanning system was applied to scan four specimen slides with FISH-probed chromosome X. A CAD scheme was developed to detect analyzable interphase cells and map the multiple imaging slices recorded FISH-probed signals into the 2-D projection images. CAD scheme was then applied to each projection image to detect analyzable interphase cells using an adaptive multiple-threshold algorithm, identify FISH-probed signals using a top-hat transform, and compute the ratios between the normal and abnormal cells. To assess CAD performance, the FISH-probed signals were also independently visually detected by an observer. The Kappa coefficients for agreement between CAD and observer ranged from 0.69 to 1.0 in detecting/counting FISH signal spots in four testing samples. The study demonstrated the feasibility of automated FISH signal analysis that applying a CAD scheme to the automated generated 2-D projection images.
Keywords: Fluorescence in situ hybridization (FISH), automated FISH signal analysis, computer-aided detection (CAD), molecular imaging biomarker
DOI: 10.3233/ACP-2012-0068
Journal: Analytical Cellular Pathology, vol. 35, no. 5-6, pp. 395-405, 2012
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