Antibody-Based Detection of ERG Rearrangement-Positive Prostate Cancer

Park, Kyung; Tomlins, Scott A.; Mudaliar, Kumaran; Chiu, Ya Lin; Esgueva, Raquel; Mehra, Rohit; Suleman, Khalid; Varambally, Sooryanarayana; Brenner, J. Chad; MacDonald, Theresa Y.; Srivastava, Abhishek; Tewari, Ashutosh; Sathyanarayana, Ubaradka G.; Nagy, Dea; Pestano, Gary A.; Kunju, Lakshmi P.; Demichelis, Francesca; Chinnaiyan, Arul M.; Rubin, Mark A.

doi:10.1593/neo.10726

Cited by 309 publications

(388 citation statements)

References 25 publications

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“…10 The description of a novel ERG antibody in 2010 highly facilitates detection of ERG genomic fusions in clinical specimens. 9 Nuclear staining by the EPR3864 antibody showed excellent concordance with the presence of TMPRSS2-ERG fusion detected by FISH or QPCR. 9,10 Although crossreactivity of the EPR3864 antibody with ETS family member FLI-1 has been reported by the manufacturer, we demonstrated lack of FLI-1 expression in prostate cancer, indicating that the antibody actually detects ERG protein in this disease.…”

Section: Discussionmentioning

confidence: 66%

“…9 Nuclear staining by the EPR3864 antibody showed excellent concordance with the presence of TMPRSS2-ERG fusion detected by FISH or QPCR. 9,10 Although crossreactivity of the EPR3864 antibody with ETS family member FLI-1 has been reported by the manufacturer, we demonstrated lack of FLI-1 expression in prostate cancer, indicating that the antibody actually detects ERG protein in this disease. 10 In this study, we found concordance of nuclear ERG expression and TMPRSS2-ERG fusion in seven human prostate cancer cell lines and 22 xenografts, with exception of xenografts PC133, PC324 and PC339, which have breakpoint in intron 1 of TMPRSS2.…”

Section: Discussionmentioning

confidence: 66%

“…Nuclear reactivity of the antibody in endothelial cells (ERG) and in stromal cells (androgen receptor) was used as internal control for the staining procedure. 9 In case of staining heterogeneity, the highest level was used for statistical analysis. All cores were scored by two investigators (MH, GvL) in a blinded setting.…”

Section: Immunohistochemistrymentioning

confidence: 99%

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ERG immunohistochemistry is not predictive for PSA recurrence, local recurrence or overall survival after radical prostatectomy for prostate cancer

et al. 2012

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In prostate cancer genomic rearrangements involving genes encoding ETS transcription factors are commonly present, with androgen-regulated transmembrane protease, serine 2 (TMPRSS2)-v-ets erythroblastosis virus E26 oncogen homologue (ERG) gene fusion occurring in 40-70%. Studies on the predictive value of ERG rearrangement as detected by in-situ hybridization or polymerase chain reaction have resulted in varying outcomes. The objective of this study was to correlate immunohistochemical ERG protein expression with clinico-pathological parameters at radical prostatectomy specimens, and to determine its predictive value for postoperative disease recurrence and progression in a prostate cancer screening cohort. Since androgen receptor is downregulated by ERG in cell lines, we also compared the expression of respective proteins. We selected 481 participants from the European Randomized Study of Screening for Prostate Cancer treated by radical prostatectomy for prostate adenocarcinoma. A tissue microarray was constructed containing representative cores of all prostate cancer specimens as well as 22 xenografts and seven cell lines. Immunohistochemical expression of ERG and androgen receptor was correlated with prostate-specific antigen (PSA), Gleason sum, pT-stage, surgical margins, biochemical recurrence, local recurrence, overall death and disease-specific death. ERG expression was detected in 284 patients (65%). Expression occurred significantly more frequent in patients with PSA r10 ng/ml (P ¼ 0.024). There was no significant association between ERG and Gleason sum, pT-stage or surgical margin status. PSA (P ¼ 0.011), Gleason sum (P ¼ 0.003), pT-stage (P ¼ 0.001) and surgical margin status (Po0.001) all had independent value for postoperative biochemical recurrence, while positive surgical margin (P ¼ 0.021) was the only independent predictor for local recurrence. ERG protein expression did not have prognostic value for the clinical end points in uni-and multivariate analyses. A positive correlation existed between ERG and androgen receptor expression in single tissue cores (Po0.001). In conclusion, immunohistochemical ERG expression has no predictive value for prostate cancer recurrence or progression after radical prostatectomy. Increasing ERG levels are associated with the upregulation of androgen receptor expression in clinical specimens.

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Section: Discussionmentioning

confidence: 66%

Section: Discussionmentioning

confidence: 66%

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ERG immunohistochemistry is not predictive for PSA recurrence, local recurrence or overall survival after radical prostatectomy for prostate cancer

et al. 2012

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“…By IHC using a rabbit ERG-MAb, Park et al and van Leenders et al have provided a comprehensive data showing that virtually all ERG rearranged PCa exhibit an ERG overexpression on the transcriptional and translational level. 20,21 He et al 22 confirmed the feasibility of the ERG IHC on an independent cohort containing a broader spectrum of prostatic lesions.…”

Section: Introductionmentioning

confidence: 87%

“…IHC was conducted with the Ventana Discovery XT automated staining system (Ventana Medical Systems, Tucson, AZ, USA) using Ventana reagents. The following clones and primary antibodies were used: anti-ERG rabbit monoclonal antibody (1:100 dilution, clone EPR3864, Abcam, Cambridge, MA, USA) 21 and anti-ERG mouse monoclonal antibody (1:1000 dilution, CPDR ERG-MAb, clone 9FY, CPDR, Rochville, MD, USA). 19 Dilution was Figure 1.…”

Section: Ihcmentioning

confidence: 99%

ERG protein expression and genomic rearrangement status in primary and metastatic prostate cancer—a comparative study of two monoclonal antibodies

Braun

Goltz

Shaikhibrahim

et al. 2012

Prostate Cancer Prostatic Dis

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BACKGROUND: Overexpression of the ERG protein is highly prevalent in prostate cancer (PCa) and commonly results from gene fusions involving the ERG gene. Recently, N-terminal epitope-targeted mouse and a C-terminal epitope-targeted rabbit monoclonal anti-ERG antibody (ERG-MAbs) have been introduced for the detection of the ERG protein. Independent studies reported that immunohistochemistry (IHC) with both ERG-MAbs highly correlates with the underlying ERG gene rearrangement status. However, comparative studies of both antibodies are lacking. Here, we are among the first to compare the mouse ERGMAb with the rabbit ERG-MAb for their concordance on the same PCa cohort. Furthermore, we assessed whether the ERG protein expression is conserved in lymph node and distant PCa metastases. METHODS: We evaluated tissue microarrays of 278 specimens containing 265 localized PCa, 29 lymph node, 30 distant metastases and 13 normal prostatic tissues. We correlated ERG protein expression with ERG rearrangement status using an ERG break-apart fluorescence in-situ hybridization assay and IHC of both ERG-MAbs. RESULTS: ERG expression and ERG rearrangement status were highly concordant regardless of whether the mouse or rabbit ERG-MAb was used (97.8% versus 98.6%, respectively). Of interest, both ERG antibodies reliably detected the ERG expression in lymph node and distant PCa metastases, of which a subset underwent decalcification. Lymphocytes only revealed immunoreactivity using the rabbit ERG-MAb. If ERG protein expression was present in localized PCa, we observed the same pattern in the corresponding lymph node metastases. CONCLUSIONS: By demonstrating a broad applicability of IHC to study ERG protein expression using either antibody, this study adds an important step toward a facilitated routine clinical application. Further, we demonstrate that the clonal nature of the ERG rearrangement is not restricted to the genomic level, but proceeds in the proteome. Together, our results simplify future efforts to further eliucidate the biological role of ERG in PCa.

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