Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordoma

Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordoma

Abstract The expression of p16/CDKN2A, the second most commonly inactivated tumour suppressor gene in cancer, is lost in the majority of chordomas. However, the mechanism(s) leading to its inactivation and contribution to disease progression have only been partially addressed using small patient coh...

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Main Authors: Lucia Cottone, Nadia Eden, Inga Usher, Patrick Lombard, Hongtao Ye, Lorena Ligammari, Daniel Lindsay, Sebastian Brandner, Jože Pižem, Nischalan Pillay, Roberto Tirabosco, Fernanda Amary, Adrienne M Flanagan
Format: Article
Language:English
Published: Wiley 2020-04-01
Series:The Journal of Pathology: Clinical Research
Subjects:
chordoma
copy number
p16
CDKN2A
IHC
FISH
Online Access:https://doi.org/10.1002/cjp2.156
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spelling doaj-c87f2065efab49d791810ba88b1748ba2020-11-25T03:28:31ZengWileyThe Journal of Pathology: Clinical Research2056-45382020-04-016211312310.1002/cjp2.156Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordomaLucia Cottone0Nadia Eden1Inga Usher2Patrick Lombard3Hongtao Ye4Lorena Ligammari5Daniel Lindsay6Sebastian Brandner7Jože Pižem8Nischalan Pillay9Roberto Tirabosco10Fernanda Amary11Adrienne M Flanagan12UCL Cancer Institute University College London London UKUCL Cancer Institute University College London London UKUCL Cancer Institute University College London London UKUCL Cancer Institute University College London London UKDepartment of Histopathology Royal National Orthopaedic Hospital Stanmore UKUCL Cancer Institute University College London London UKDepartment of Histopathology Royal National Orthopaedic Hospital Stanmore UKUCL Queen Square Institute of Neurology University College London London UKInstitute of Pathology University of Ljubljana, Faculty of Medicine Ljubljana SloveniaUCL Cancer Institute University College London London UKDepartment of Histopathology Royal National Orthopaedic Hospital Stanmore UKUCL Cancer Institute University College London London UKUCL Cancer Institute University College London London UKAbstract The expression of p16/CDKN2A, the second most commonly inactivated tumour suppressor gene in cancer, is lost in the majority of chordomas. However, the mechanism(s) leading to its inactivation and contribution to disease progression have only been partially addressed using small patient cohorts. We studied 384 chordoma samples from 320 patients by immunohistochemistry and found that p16 protein was lost in 53% of chordomas and was heterogeneously expressed in these tumours. To determine if CDKN2A copy number loss could explain the absence of p16 protein expression we performed fluorescence in situ hybridisation (FISH) for CDKN2A on consecutive tissue sections. CDKN2A copy number status was altered in 168 of 274 (61%) of samples and copy number loss was the most frequent alteration acquired during clinical disease progression. CDKN2A homozygous deletion was always associated with p16 protein loss but only accounted for 33% of the p16‐negative cases. The remaining immunonegative cases were associated with disomy (27%), monosomy (12%), heterozygous loss (20%) and copy number gain (7%) of CDKN2A, supporting the hypothesis that loss of protein expression might be achieved via epigenetic or post‐transcriptional regulatory mechanisms. We identified that mRNA levels were comparable in tumours with and without p16 protein expression, but other events including DNA promoter hypermethylation, copy number neutral loss of heterozygosity and expression of candidate microRNAs previously implicated in the regulation of CDKN2A expression were not identified to explain the protein loss. The data argue that p16 loss in chordoma is commonly caused by a post‐transcriptional regulatory mechanism that is yet to be defined.https://doi.org/10.1002/cjp2.156chordomacopy numberp16CDKN2AIHCFISH
collection DOAJ
language English
format Article
sources DOAJ
author Lucia Cottone
Nadia Eden
Inga Usher
Patrick Lombard
Hongtao Ye
Lorena Ligammari
Daniel Lindsay
Sebastian Brandner
Jože Pižem
Nischalan Pillay
Roberto Tirabosco
Fernanda Amary
Adrienne M Flanagan
spellingShingle Lucia Cottone
Nadia Eden
Inga Usher
Patrick Lombard
Hongtao Ye
Lorena Ligammari
Daniel Lindsay
Sebastian Brandner
Jože Pižem
Nischalan Pillay
Roberto Tirabosco
Fernanda Amary
Adrienne M Flanagan
Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordoma
The Journal of Pathology: Clinical Research
chordoma
copy number
p16
CDKN2A
IHC
FISH
author_facet Lucia Cottone
Nadia Eden
Inga Usher
Patrick Lombard
Hongtao Ye
Lorena Ligammari
Daniel Lindsay
Sebastian Brandner
Jože Pižem
Nischalan Pillay
Roberto Tirabosco
Fernanda Amary
Adrienne M Flanagan
author_sort Lucia Cottone
title Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordoma
title_short Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordoma
title_full Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordoma
title_fullStr Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordoma
title_full_unstemmed Frequent alterations in p16/CDKN2A identified by immunohistochemistry and FISH in chordoma
title_sort frequent alterations in p16/cdkn2a identified by immunohistochemistry and fish in chordoma
publisher Wiley
series The Journal of Pathology: Clinical Research
issn 2056-4538
publishDate 2020-04-01
description Abstract The expression of p16/CDKN2A, the second most commonly inactivated tumour suppressor gene in cancer, is lost in the majority of chordomas. However, the mechanism(s) leading to its inactivation and contribution to disease progression have only been partially addressed using small patient cohorts. We studied 384 chordoma samples from 320 patients by immunohistochemistry and found that p16 protein was lost in 53% of chordomas and was heterogeneously expressed in these tumours. To determine if CDKN2A copy number loss could explain the absence of p16 protein expression we performed fluorescence in situ hybridisation (FISH) for CDKN2A on consecutive tissue sections. CDKN2A copy number status was altered in 168 of 274 (61%) of samples and copy number loss was the most frequent alteration acquired during clinical disease progression. CDKN2A homozygous deletion was always associated with p16 protein loss but only accounted for 33% of the p16‐negative cases. The remaining immunonegative cases were associated with disomy (27%), monosomy (12%), heterozygous loss (20%) and copy number gain (7%) of CDKN2A, supporting the hypothesis that loss of protein expression might be achieved via epigenetic or post‐transcriptional regulatory mechanisms. We identified that mRNA levels were comparable in tumours with and without p16 protein expression, but other events including DNA promoter hypermethylation, copy number neutral loss of heterozygosity and expression of candidate microRNAs previously implicated in the regulation of CDKN2A expression were not identified to explain the protein loss. The data argue that p16 loss in chordoma is commonly caused by a post‐transcriptional regulatory mechanism that is yet to be defined.
topic chordoma
copy number
p16
CDKN2A
IHC
FISH
url https://doi.org/10.1002/cjp2.156
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