TY - JOUR
T1 - Antibody selection influences the detection of AR-V7 in primary prostate cancer
AU - Kaczorowski, Adam
AU - Chen, Xin
AU - Herpel, Esther
AU - Merseburger, Axel S.
AU - Kristiansen, Glen
AU - Bernemann, Christof
AU - Hohenfellner, Markus
AU - Cronauer, Marcus V.
AU - Duensing, Stefan
N1 - Funding Information:
We are very grateful to the NCT Tissue Bank for procurement of tumor specimens and TMA construction. We would like to thank Jocelyn Céraline for the AR-V7 construct and Constanze Rapp and Christine Geisler for patient data management. This work was supported by the Medical Faculty Heidelberg and the Wilhelm Sander-Stiftung.
Publisher Copyright:
© 2020 The Author(s)
Copyright:
Copyright 2020 Elsevier B.V., All rights reserved.
PY - 2020
Y1 - 2020
N2 - Background: The androgen receptor (AR) splice variant V7 (AR-V7) is an emerging marker to aid clinical decision-making in patients with castration-resistant prostate cancer (CRPC). A number of studies have shown that a subset of patients also express AR-V7 in the primary tumor. These findings have recently been challenged by a study showing that AR-V7 becomes only detectable in CRPC but is virtually absent in castration-naïve prostate cancer. Methods: Herein, we directly compare the two relevant antibodies used for the immunodetection of AR-V7 in the conflicting studies (clones AG10008 and RM7) in a predominantly high-risk prostate cancer patient cohort with primary tumor specimens assembled in a tissue microarray (TMA). Results: The overall rate of AR-V7 positive TMA cores was comparable (AG10008, 24.9%; RM7, 21%). However, the percentage agreement of identical staining intensities of positive cores was only 7%. In contrast, the percentage agreement of negative cores was 62.8%. In approximately 30% of the cores, the antibodies produced discordant staining intensities. Only one of the two antibody stainings (AG10008) conveyed prognostic information and was associated with a shorter progression-free patient survival. Conclusions: Our study underscores that nuclear AR-V7 expression can be detected in primary prostate cancer prior to long-term androgen deprivation and castration resistance. There are staining differences between the two antibodies in tumor tissue, for which we currently have no explanation. Clearly, improvements in the detection of functional AR-V7 in prostate cancer are urgently needed.
AB - Background: The androgen receptor (AR) splice variant V7 (AR-V7) is an emerging marker to aid clinical decision-making in patients with castration-resistant prostate cancer (CRPC). A number of studies have shown that a subset of patients also express AR-V7 in the primary tumor. These findings have recently been challenged by a study showing that AR-V7 becomes only detectable in CRPC but is virtually absent in castration-naïve prostate cancer. Methods: Herein, we directly compare the two relevant antibodies used for the immunodetection of AR-V7 in the conflicting studies (clones AG10008 and RM7) in a predominantly high-risk prostate cancer patient cohort with primary tumor specimens assembled in a tissue microarray (TMA). Results: The overall rate of AR-V7 positive TMA cores was comparable (AG10008, 24.9%; RM7, 21%). However, the percentage agreement of identical staining intensities of positive cores was only 7%. In contrast, the percentage agreement of negative cores was 62.8%. In approximately 30% of the cores, the antibodies produced discordant staining intensities. Only one of the two antibody stainings (AG10008) conveyed prognostic information and was associated with a shorter progression-free patient survival. Conclusions: Our study underscores that nuclear AR-V7 expression can be detected in primary prostate cancer prior to long-term androgen deprivation and castration resistance. There are staining differences between the two antibodies in tumor tissue, for which we currently have no explanation. Clearly, improvements in the detection of functional AR-V7 in prostate cancer are urgently needed.
UR - http://www.scopus.com/inward/record.url?scp=85087390016&partnerID=8YFLogxK
U2 - 10.1016/j.ctarc.2020.100186
DO - 10.1016/j.ctarc.2020.100186
M3 - Journal articles
C2 - 32619831
AN - SCOPUS:85087390016
SN - 2468-2942
VL - 24
JO - Cancer Treatment and Research Communications
JF - Cancer Treatment and Research Communications
M1 - 100186
ER -