Literature DB >> 26818831

Doing more with less: fluorescence in situ hybridization and gene sequencing assays can be reliably performed on archival stained tumor tissue sections.

Giuseppe Pelosi1,2, Federica Perrone3, Elena Tamborini3, Alessandra Fabbri3, Maria Adele Testi3, Adele Busico3, Giulio Settanni3, Benedetta Picciani3, Enrica Bovio3, Angelica Sonzogni3, Barbara Valeri3, Marina Garassino4, Filippo De Braud4, Ugo Pastorino5.   

Abstract

Little is known about molecular testing on tumor tissue retrieved from stained sections, for which there may be a clinical need. We retrospectively analyzed 112 sections from 56 tumor patients using either fluorescence in situ hybridization (FISH) with different probes (19 sections from 17 patients) or Sanger or targeted next generation sequencing for detection of BRAF, EGFR, KRAS, C-KIT, and TP53 mutations (93 sections from 39 patients). Tumor tissue sections had been stained by hematoxylin and eosin (H&E) (42 sections) or by immunohistochemistry for cytoplasmic or nuclear/nuclear-cytoplasmic markers (70 sections) with a peroxidase (P-IHC, with 3,3'-diaminobenzidine as chromogen) or alkaline phosphatase label (AP-IHC, with Warp Red™ as chromogen). For FISH analysis, the concordance rate between the original diagnosis and that obtained on H&E- or P-IHC-stained tissue sections (AP-IHC was not on record for this set of patients) was 95% (18 out of 19 tumor sections). Only one tumor sample, diffusely positive for MLH1, did not yield any nuclear hybridization signal. For sequencing analysis, the concordance rate was 100% on negative P-IHC and positive AP-IHC-stained sections, regardless of the subcellular localization of the reaction product. Mutations were detected in only 52% of cases expressing nuclear/nuclear-cytoplasmic markers, regardless of the sequencing technology used (p = 0.0002). In conclusion, stained sections may be a valuable resource for FISH or sequencing analysis, but on cases expressing nuclear markers sequencing results need to be interpreted cautiously.

Entities:  

Keywords:  Direct sequencing; Fish; Immunohistochemistry; Next generation sequencing

Mesh:

Substances:

Year:  2016        PMID: 26818831     DOI: 10.1007/s00428-016-1906-0

Source DB:  PubMed          Journal:  Virchows Arch        ISSN: 0945-6317            Impact factor:   4.064


  30 in total

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Journal:  Lung Cancer       Date:  2012-06-16       Impact factor: 5.705

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7.  DNA interaction with diaminobenzidine studied with optical tweezers and dynamic light scattering.

Authors:  L A Reis; E B Ramos; M S Rocha
Journal:  J Phys Chem B       Date:  2013-11-07       Impact factor: 2.991

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Journal:  Cytopathology       Date:  2014-05-15       Impact factor: 2.073

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Authors:  Samia Mourah; Marc G Denis; Fabienne Escande Narducci; Jérôme Solassol; Jean-Louis Merlin; Jean-Christophe Sabourin; Jean-Yves Scoazec; L'Houcine Ouafik; Jean-François Emile; Remy Heller; Claude Souvignet; Loïc Bergougnoux; Jean-Philippe Merlio
Journal:  PLoS One       Date:  2015-03-19       Impact factor: 3.240

10.  Molecular typing of lung adenocarcinoma on cytological samples using a multigene next generation sequencing panel.

Authors:  Aldo Scarpa; Katarzyna Sikora; Matteo Fassan; Anna Maria Rachiglio; Rocco Cappellesso; Davide Antonello; Eliana Amato; Andrea Mafficini; Matilde Lambiase; Claudia Esposito; Emilio Bria; Francesca Simonato; Maria Scardoni; Giona Turri; Marco Chilosi; Giampaolo Tortora; Ambrogio Fassina; Nicola Normanno
Journal:  PLoS One       Date:  2013-11-13       Impact factor: 3.240

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  1 in total

1.  Thymus neuroendocrine tumors with CTNNB1 gene mutations, disarrayed ß-catenin expression, and dual intra-tumor Ki-67 labeling index compartmentalization challenge the concept of secondary high-grade neuroendocrine tumor: a paradigm shift.

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Journal:  Virchows Arch       Date:  2017-04-27       Impact factor: 4.064

  1 in total

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