Unraveling the chromosome 17 patterns of FISH in interphase nuclei: an in-depth analysis of the HER2 amplicon and chromosome 17 centromere by karyotyping, FISH and M-FISH in breast cancer cells

BACKGROUND: In diagnostic pathology, HER2 status is determined in interphase nuclei by fluorescence in situ hybridization (FISH) with probes for the HER2 gene and for the chromosome 17 centromere (CEP17). The latter probe is used as a surrogate for chromosome 17 copies, however chromosome 17 (Chr17)...

Descripción completa

Detalles Bibliográficos
Autores principales: Rondón-Lagos, Milena, Verdun Di Cantogno, Ludovica, Rangel, Nelson, Mele, Teresa, Ramírez-Clavijo, Sandra R, Scagliotti, Giorgio, Marchiò, Caterina, Sapino, Anna
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2014
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4295336/
https://www.ncbi.nlm.nih.gov/pubmed/25481507
http://dx.doi.org/10.1186/1471-2407-14-922
_version_ 1782352829317382144
author Rondón-Lagos, Milena
Verdun Di Cantogno, Ludovica
Rangel, Nelson
Mele, Teresa
Ramírez-Clavijo, Sandra R
Scagliotti, Giorgio
Marchiò, Caterina
Sapino, Anna
author_facet Rondón-Lagos, Milena
Verdun Di Cantogno, Ludovica
Rangel, Nelson
Mele, Teresa
Ramírez-Clavijo, Sandra R
Scagliotti, Giorgio
Marchiò, Caterina
Sapino, Anna
author_sort Rondón-Lagos, Milena
collection PubMed
description BACKGROUND: In diagnostic pathology, HER2 status is determined in interphase nuclei by fluorescence in situ hybridization (FISH) with probes for the HER2 gene and for the chromosome 17 centromere (CEP17). The latter probe is used as a surrogate for chromosome 17 copies, however chromosome 17 (Chr17) is frequently rearranged. The frequency and type of specific structural Chr17 alterations in breast cancer have been studied by using comparative genomic hybridization and spectral karyotyping, but not fully detailed. Actually, balanced chromosome rearrangements (e.g. translocations or inversions) and low frequency mosaicisms are assessable on metaphases using G-banding karyotype and multicolor FISH (M-FISH) only. METHODS: We sought to elucidate the CEP17 and HER2 FISH patterns of interphase nuclei by evaluating Chr17 rearrangements in metaphases of 9 breast cancer cell lines and a primary culture from a triple negative breast carcinoma by using G-banding, FISH and M-FISH. RESULTS: Thirty-nine rearranged chromosomes containing a portion of Chr17 were observed. Chromosomes 8 and 11 were the most frequent partners of Chr17 translocations. The lowest frequency of Chr17 abnormalities was observed in the HER2-negative cell lines, while the highest was observed in the HER2-positive SKBR3 cells. The MDA-MB231 triple negative cell line was the sole to show only non-altered copies of Chr17, while the SKBR3, MDA-MB361 and JIMT-1 HER2-positive cells carried no normal Chr17 copies. True polysomy was observed in MDA-MB231 as the only Chr17 alteration. In BT474 cells polysomy was associated to Chr17 structural alterations. By comparing M-FISH and FISH data, in 8 out of 39 rearranged chromosomes only CEP17 signals were detectable, whereas in 14 rearranged chromosomes HER2 and STARD3 genes were present without CEP17 signals. HER2 and STARD3 always co-localized on the same chromosomes and were always co-amplified, whereas TOP2A also mapped to different derivatives and was co-amplified with HER2 and STARD3 on SKBR3 cells only. CONCLUSION: The high frequency of complex Chr17 abnormalities suggests that the interpretation of FISH results on interphase nuclei using a dual probe assay to assess gene amplification should be performed “with caution”, given that CEP17 signals are not always indicative of normal unaltered or rearranged copies of Chr17.
format Online
Article
Text
id pubmed-4295336
institution National Center for Biotechnology Information
language English
publishDate 2014
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-42953362015-01-16 Unraveling the chromosome 17 patterns of FISH in interphase nuclei: an in-depth analysis of the HER2 amplicon and chromosome 17 centromere by karyotyping, FISH and M-FISH in breast cancer cells Rondón-Lagos, Milena Verdun Di Cantogno, Ludovica Rangel, Nelson Mele, Teresa Ramírez-Clavijo, Sandra R Scagliotti, Giorgio Marchiò, Caterina Sapino, Anna BMC Cancer Research Article BACKGROUND: In diagnostic pathology, HER2 status is determined in interphase nuclei by fluorescence in situ hybridization (FISH) with probes for the HER2 gene and for the chromosome 17 centromere (CEP17). The latter probe is used as a surrogate for chromosome 17 copies, however chromosome 17 (Chr17) is frequently rearranged. The frequency and type of specific structural Chr17 alterations in breast cancer have been studied by using comparative genomic hybridization and spectral karyotyping, but not fully detailed. Actually, balanced chromosome rearrangements (e.g. translocations or inversions) and low frequency mosaicisms are assessable on metaphases using G-banding karyotype and multicolor FISH (M-FISH) only. METHODS: We sought to elucidate the CEP17 and HER2 FISH patterns of interphase nuclei by evaluating Chr17 rearrangements in metaphases of 9 breast cancer cell lines and a primary culture from a triple negative breast carcinoma by using G-banding, FISH and M-FISH. RESULTS: Thirty-nine rearranged chromosomes containing a portion of Chr17 were observed. Chromosomes 8 and 11 were the most frequent partners of Chr17 translocations. The lowest frequency of Chr17 abnormalities was observed in the HER2-negative cell lines, while the highest was observed in the HER2-positive SKBR3 cells. The MDA-MB231 triple negative cell line was the sole to show only non-altered copies of Chr17, while the SKBR3, MDA-MB361 and JIMT-1 HER2-positive cells carried no normal Chr17 copies. True polysomy was observed in MDA-MB231 as the only Chr17 alteration. In BT474 cells polysomy was associated to Chr17 structural alterations. By comparing M-FISH and FISH data, in 8 out of 39 rearranged chromosomes only CEP17 signals were detectable, whereas in 14 rearranged chromosomes HER2 and STARD3 genes were present without CEP17 signals. HER2 and STARD3 always co-localized on the same chromosomes and were always co-amplified, whereas TOP2A also mapped to different derivatives and was co-amplified with HER2 and STARD3 on SKBR3 cells only. CONCLUSION: The high frequency of complex Chr17 abnormalities suggests that the interpretation of FISH results on interphase nuclei using a dual probe assay to assess gene amplification should be performed “with caution”, given that CEP17 signals are not always indicative of normal unaltered or rearranged copies of Chr17. BioMed Central 2014-12-07 /pmc/articles/PMC4295336/ /pubmed/25481507 http://dx.doi.org/10.1186/1471-2407-14-922 Text en © Rondón-Lagos et al.; licensee BioMed Central Ltd. 2014 This article is published under license to BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly credited. The Creative Commons Public Domain Dedication waiver (http://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated.
spellingShingle Research Article
Rondón-Lagos, Milena
Verdun Di Cantogno, Ludovica
Rangel, Nelson
Mele, Teresa
Ramírez-Clavijo, Sandra R
Scagliotti, Giorgio
Marchiò, Caterina
Sapino, Anna
Unraveling the chromosome 17 patterns of FISH in interphase nuclei: an in-depth analysis of the HER2 amplicon and chromosome 17 centromere by karyotyping, FISH and M-FISH in breast cancer cells
title Unraveling the chromosome 17 patterns of FISH in interphase nuclei: an in-depth analysis of the HER2 amplicon and chromosome 17 centromere by karyotyping, FISH and M-FISH in breast cancer cells
title_full Unraveling the chromosome 17 patterns of FISH in interphase nuclei: an in-depth analysis of the HER2 amplicon and chromosome 17 centromere by karyotyping, FISH and M-FISH in breast cancer cells
title_fullStr Unraveling the chromosome 17 patterns of FISH in interphase nuclei: an in-depth analysis of the HER2 amplicon and chromosome 17 centromere by karyotyping, FISH and M-FISH in breast cancer cells
title_full_unstemmed Unraveling the chromosome 17 patterns of FISH in interphase nuclei: an in-depth analysis of the HER2 amplicon and chromosome 17 centromere by karyotyping, FISH and M-FISH in breast cancer cells
title_short Unraveling the chromosome 17 patterns of FISH in interphase nuclei: an in-depth analysis of the HER2 amplicon and chromosome 17 centromere by karyotyping, FISH and M-FISH in breast cancer cells
title_sort unraveling the chromosome 17 patterns of fish in interphase nuclei: an in-depth analysis of the her2 amplicon and chromosome 17 centromere by karyotyping, fish and m-fish in breast cancer cells
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4295336/
https://www.ncbi.nlm.nih.gov/pubmed/25481507
http://dx.doi.org/10.1186/1471-2407-14-922
work_keys_str_mv AT rondonlagosmilena unravelingthechromosome17patternsoffishininterphasenucleianindepthanalysisoftheher2ampliconandchromosome17centromerebykaryotypingfishandmfishinbreastcancercells
AT verdundicantognoludovica unravelingthechromosome17patternsoffishininterphasenucleianindepthanalysisoftheher2ampliconandchromosome17centromerebykaryotypingfishandmfishinbreastcancercells
AT rangelnelson unravelingthechromosome17patternsoffishininterphasenucleianindepthanalysisoftheher2ampliconandchromosome17centromerebykaryotypingfishandmfishinbreastcancercells
AT meleteresa unravelingthechromosome17patternsoffishininterphasenucleianindepthanalysisoftheher2ampliconandchromosome17centromerebykaryotypingfishandmfishinbreastcancercells
AT ramirezclavijosandrar unravelingthechromosome17patternsoffishininterphasenucleianindepthanalysisoftheher2ampliconandchromosome17centromerebykaryotypingfishandmfishinbreastcancercells
AT scagliottigiorgio unravelingthechromosome17patternsoffishininterphasenucleianindepthanalysisoftheher2ampliconandchromosome17centromerebykaryotypingfishandmfishinbreastcancercells
AT marchiocaterina unravelingthechromosome17patternsoffishininterphasenucleianindepthanalysisoftheher2ampliconandchromosome17centromerebykaryotypingfishandmfishinbreastcancercells
AT sapinoanna unravelingthechromosome17patternsoffishininterphasenucleianindepthanalysisoftheher2ampliconandchromosome17centromerebykaryotypingfishandmfishinbreastcancercells

Ejemplares similares