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      Pulmonary adenocarcinoma with mucin production modulates phenotype according to common genetic traits: a reappraisal of mucinous adenocarcinoma and colloid adenocarcinoma

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          Abstract

          Whether invasive mucinous adenocarcinoma (IMA) and colloid adenocarcinoma (ICA) of the lung represent separate tumour entities, or simply lie within a spectrum of phenotypic variability, is worth investigating. Fifteen ICA, 12 IMA, 9 ALK‐rearranged adenocarcinomas (ALKA), 8 non‐mucinous KRAS‐mutated adenocarcinomas (KRASA) and 9 mucinous breast adenocarcinomas (MBA) were assessed by immunohistochemistry for alveolar (TTF1, cytoplasmic MUC1), intestinal (CDX‐2, MUC2), gastric (membrane MUC1, MUC6), bronchial (MUC5AC), mesenchymal (vimentin), neuroendocrine (chromogranin A, synaptophysin), sex steroid hormone‐related (oestrogen and progesterone receptors), pan‐mucinous (HNF4A) and pan‐epithelial (keratin 7) lineage biomarkers and by targeted next generation sequencing (TNGS) for 50 recurrently altered cancer genes. Unsupervised clustering analysis using molecular features identified cluster 1 (IMA and ICA), cluster 2 (ALKA and KRASA) and cluster 3 (MBA) ( p < 0.0001). Cluster 1 showed four histology‐independent sub‐clusters (S1 to S4) pooled by HFN4A and MUC5AC but diversely reacting for TTF1, MUC1, MUC2, MUC6 and CDX2. Sub‐cluster S1 predominantly featured intestinal‐alveolar, S2 gastrointestinal, S3 gastric and S4 alveolar differentiation. In turn, KRASA and ALKA shared alveolar lineage alongside residual MUC5AC expression, with additional focal CDX2 and diffuse vimentin, respectively. A proximal‐to‐distal scheme extending from terminal (TB) and respiratory (RB) bronchioles to alveolar cells was devised, where S3 originated from distal TB (cellular mucinous adenocarcinoma), S2 from proximal RB (secreting mucinous adenocarcinoma), S1 from intermediate RB (mucin lake‐forming colloid adenocarcinoma), S4 from distal RB (colloid alveolar adenocarcinoma), KRASA from juxta‐alveolar RB (KRAS‐mutated non‐mucinous adenocarcinoma) and ALKA from juxta‐bronchial alveolar cells (ALK‐translocated adenocarcinoma). TNGS analysis showed KRAS, LKB1, TP53, APC and CDKN2A mutation predominance. In conclusion, IMA and ICA are basket categories, which likely originate from distinct domains of stem/progenitor cells spatially distributed along bronchioles upon common molecular features and genetic alterations.

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          MUC1 cell surface mucin is a critical element of the mucosal barrier to infection.

          J. McAuley, C Png, Sara K. Lindén (2007)
          Cell surface mucin glycoproteins are highly expressed by all mucosal tissues, yet their physiological role is currently unknown. We hypothesized that cell surface mucins protect mucosal cells from infection. A rapid progressive increase in gastrointestinal expression of mucin 1 (Muc1) cell surface mucin followed infection of mice with the bacterial pathogen Campylobacter jejuni. In the first week following oral infection, C. jejuni was detected in the systemic organs of the vast majority of Muc1(-/-) mice but never in Muc1(+/+) mice. Although C. jejuni entered gastrointestinal epithelial cells of both Muc1(-/-) and Muc1(+/+) mice, small intestinal damage as manifested by increased apoptosis and enucleated and shed villous epithelium was more common in Muc1(-/-) mice. Using radiation chimeras, we determined that prevention of systemic infection in wild-type mice was due exclusively to epithelial Muc1 rather than Muc1 on hematopoietic cells. Expression of MUC1-enhanced resistance to C. jejuni cytolethal distending toxin (CDT) in vitro and CDT null C. jejuni showed lower gastric colonization in Muc1(-/-) mice in vivo. We believe this is the first in vivo experimental study to demonstrate that cell surface mucins are a critical component of mucosal defence and that the study provides the foundation for exploration of their contribution to epithelial infectious and inflammatory diseases.
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            Evidence for human lung stem cells.

            Mark A Perrella, K Haley, R. Hall-Wilton (2011)
            Although progenitor cells have been described in distinct anatomical regions of the lung, description of resident stem cells has remained elusive. Surgical lung-tissue specimens were studied in situ to identify and characterize human lung stem cells. We defined their phenotype and functional properties in vitro and in vivo. Human lungs contain undifferentiated human lung stem cells nested in niches in the distal airways. These cells are self-renewing, clonogenic, and multipotent in vitro. After injection into damaged mouse lung in vivo, human lung stem cells form human bronchioles, alveoli, and pulmonary vessels integrated structurally and functionally with the damaged organ. The formation of a chimeric lung was confirmed by detection of human transcripts for epithelial and vascular genes. In addition, the self-renewal and long-term proliferation of human lung stem cells was shown in serial-transplantation assays. Human lungs contain identifiable stem cells. In animal models, these cells participate in tissue homeostasis and regeneration. They have the undemonstrated potential to promote tissue restoration in patients with lung disease. (Funded by the National Institutes of Health.).
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              Nkx2-1 represses a latent gastric differentiation program in lung adenocarcinoma.

              Charles A Whittaker, Nicole L. Snyder, Lin Wang (2013)
              Tissue-specific differentiation programs become dysregulated during cancer evolution. The transcription factor Nkx2-1 is a master regulator of pulmonary differentiation that is downregulated in poorly differentiated lung adenocarcinoma. Here we use conditional murine genetics to determine how the identity of lung epithelial cells changes upon loss of their master cell-fate regulator. Nkx2-1 deletion in normal and neoplastic lungs causes not only loss of pulmonary identity but also conversion to a gastric lineage. Nkx2-1 is likely to maintain pulmonary identity by recruiting transcription factors Foxa1 and Foxa2 to lung-specific loci, thus preventing them from binding gastrointestinal targets. Nkx2-1-negative murine lung tumors mimic mucinous human lung adenocarcinomas, which express gastric markers. Loss of the gastrointestinal transcription factor Hnf4α leads to derepression of the embryonal proto-oncogene Hmga2 in Nkx2-1-negative tumors. These observations suggest that loss of both active and latent differentiation programs is required for tumors to reach a primitive, poorly differentiated state. Copyright © 2013 Elsevier Inc. All rights reserved.
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                Author and article information

                Contributors
                Giuseppe Pelosi: giuseppe.pelosi@unimi.it
                Journal
                Journal ID (nlm-ta): J Pathol Clin Res
                Journal ID (iso-abbrev): J Pathol Clin Res
                Journal ID (doi): 10.1002/(ISSN)2056-4538
                Journal ID (publisher-id): CJP2
                Title: The Journal of Pathology: Clinical Research
                Publisher: John Wiley and Sons Inc. (Hoboken )
                ISSN (Electronic): 2056-4538
                Publication date (Electronic): 22 March 2017
                Publication date Collection: April 2017
                Volume: 3
                Issue: 2 ( doiID: 10.1002/cjp2.v3.2 )
                Pages: 139-152
                Affiliations
                [ 1 ] Department of Pathology and Laboratory MedicineFondazione IRCCS Istituto Nazionale Tumori MilanItaly
                [ 2 ] Institute for Stem‐Cell Biology, Regenerative Medicine and Innovative Therapies (ISBreMIT)IRCCS Casa Sollievo della Sofferenza San Giovanni RotondoItaly
                [ 3 ] Division of Anatomic PathologyRegional Hospital Umberto Parini AostaItaly
                [ 4 ] Department of Oncology and Advanced TechnologyOperative Unit of Pathologic Anatomy, IRCCS Azienda Arcispedale S. Maria Nuova Reggio EmiliaItaly
                [ 5 ] Division of Thoracic SurgeryFondazione IRCCS Istituto Nazionale Tumori MilanItaly
                [ 6 ] Department of Oncology and Hemato‐OncologyUniversità degli Studi MilanItaly
                [ 7 ] Inter‐Hospital Pathology DivisionScience & Technology Park, IRCCS MultiMedica Group MilanItaly
                Author notes
                [*] [* ]Correspondence to: Giuseppe Pelosi, Servizio Interaziendale di Anatomia Patologica, Polo Scientifico e Tecnologico, Via Gaudenzio Fantoli 16/15, 20138 Milan, Italy. E‐mail: giuseppe.pelosi@ 123456unimi.it
                Article
                Publisher ID: CJP267
                DOI: 10.1002/cjp2.67
                PMC ID: 5402180
                PubMed ID: 28451462
                SO-VID: 7c9f6e64-65c2-469e-9992-c6fb6c1900f6
                Copyright © © 2017 The Authors The Journal of Pathology: Clinical Research published by The Pathological Society of Great Britain and Ireland and John Wiley & Sons Ltd
                License:

                This is an open access article under the terms of the Creative Commons Attribution‐NonCommercial‐NoDerivs License, which permits use and distribution in any medium, provided the original work is properly cited, the use is non‐commercial and no modifications or adaptations are made.

                History
                Date received : 17 November 2016
                Date accepted : 20 February 2017
                Page count
                Figures: 4, Tables: 2, Pages: 14, Words: 7868
                Categories
                Subject: Original Article
                Subject: Original Articles
                Custom metadata
                source-schema-version-number 2.0
                component-id cjp267
                cover-date April 2017
                details-of-publishers-convertor Converter:WILEY_ML3GV2_TO_NLMPMC version:5.0.9 mode:remove_FC converted:24.04.2017

                Keywords: adenocarcinoma,lung,mucinous,colloid,immunohistochemistry,next generation sequencing,reappraisal,cluster analysis
                Data availability:
                Keywords: adenocarcinoma, lung, mucinous, colloid, immunohistochemistry, next generation sequencing, reappraisal, cluster analysis

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