Circulating cKIT and PDGFRA DNA indicates disease activity in Gastrointestinal Stromal Tumor (GIST)

Stefanie Jilg; Michael Rassner; Jacqueline Maier; Silvia Waldeck; Victoria Kehl; Marie Follo; Ulrike Philipp; Andreas Sauter; Katja Specht; Jan Mitschke; Thoralf Lange; Sebastian Bauer; Philipp J. Jost; Christian Peschel; Justus Duyster; Timo Gaiser; Peter Hohenberger; Nikolas von Bubnoff

doi:10.1002/ijc.32282

Circulating cKIT and PDGFRA DNA indicates disease activity in Gastrointestinal Stromal Tumor (GIST)

Stefanie Jilg, Michael Rassner, Jacqueline Maier, Silvia Waldeck, Victoria Kehl, Marie Follo, Ulrike Philipp, Andreas Sauter, Katja Specht, Jan Mitschke, Thoralf Lange, Sebastian Bauer, Philipp J. Jost, Christian Peschel, Justus Duyster, Timo Gaiser, Peter Hohenberger, Nikolas von Bubnoff^*

^*Korrespondierende/r Autor/-in für diese Arbeit

Klinik für Hämatologie und Onkologie

34 Zitate (Scopus)

Abstract

This prospective trial aimed to investigate whether tumor-specific cKIT and PDGFRA mutations can be detected and quantified in circulating tumor (ct)DNA in patients with active GIST, and whether detection indicates disease activity. We included 25 patients with active disease and cKIT or PDGFRA mutations detected in tissue. Mutant ctDNA was detected in the peripheral blood plasma using allele-specific ligation (L-)PCR and droplet digital (d)PCR. CtDNA harboring tumor-specific cKIT or PDGFRA mutations was detected at least once in 16 out of 25 patients using L-PCR (64%) and in 20 out of 25 patients with dPCR (80%). Using dPCR, the absolute numbers of ctDNA fragments (DNA copies/ml) and the mutant allele frequency (MAF; in percent of wild-type control) strongly correlated with tumor size expressed as RECIST1.1 sum of diameter (SOD) in mm (ρ = 0.3719 and 0.408, respectively, p < 0.0001) and response status (ρ = 0.3939 and 0.392, respectively, p < 0.0001 and p < 0.001). Specificity of dPCR for detection of progression was 79.2% with a sensitivity of 55.2% and dPCR discriminated CR from active disease with a specificity of 96% and s sensitivity of 44.7%. With L-PCR, correlations of MAF with tumor size and response status were less prominent. Serial ctDNA measurement reflected individual disease courses over time. Targeted panel sequencing of four patients detected additional driver mutations in all cases and secondary resistance mutations in two cases. Thus, ctDNA indicates disease activity in patients with GIST and should be incorporated as companion biomarker in future prospective trials.

Originalsprache	Englisch
Zeitschrift	International Journal of Cancer
Jahrgang	145
Ausgabenummer	8
Seiten (von - bis)	2292-2303
Seitenumfang	12
ISSN	0020-7136
DOIs	https://doi.org/10.1002/ijc.32282
Publikationsstatus	Veröffentlicht - 15.10.2019

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diagnostic imaging, response to therapy (surgery and/or therapy with a TKI) or relapse or progression of the disease as assessed by diagnostic imaging. Furthermore, the sensitivity of L-PCR and dPCR for specific cKIT or PGDFRA mutations was analyzed. The study was approved by the responsible Institutional Review Board (Technical University of Munich, 5108/11). This trial was registered under Eudra-CTNo. 2011-002544-27 and ClinicalTrials.gov NCT01462994. This trial received financial support by Novartis Pharma (Study Code: CSTI571BDE78T). The authors would also like to acknowledge the support of the Munich Study Center, the University of Freiburg Medical Faculty, the Comprehensive Cancer Center Freiburg (CCCF), the German Cancer Consortium (DKTK; grant no. L665 to NvB), the Bundesministerium für Bildung und Forschung (BMBF; grant no. 13GW0198E to NvB) and Novartis Germany for research support (study no. CSTI5781BDE78T to NvB). We thank Fol-ker Schneller for patient management, Sandra Eckert and Monika Mathew for administrative support, and Amanda Kalman for critical advice. In addition, the authors want to thank Laura-Jane Behl as well as the whole “Genomics and Proteomics Core Facility of the DKFZ Heidelberg (Germany)” for providing excellent sequencing service. The authors would also like to acknowledge the support of the Munich Study Center, the University of Freiburg Medical Faculty, the Comprehensive Cancer Center Freiburg (CCCF), the German Cancer Consortium (DKTK; grant no. L665 to NvB), the Bundesministerium f?r Bildung und Forschung (BMBF; grant no. 13GW0198E to NvB) and Novartis Germany for research support (study no. CSTI5781BDE78T to NvB). We thank Folker Schneller for patient management, Sandra Eckert and Monika Mathew for administrative support, and Amanda Kalman for critical advice. In addition, the authors want to thank Laura-Jane Behl as well as the whole ?Genomics and Proteomics Core Facility of the DKFZ Heidelberg (Germany)? for providing excellent sequencing service.

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10.1002/ijc.32282

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Jilg, S., Rassner, M., Maier, J., Waldeck, S., Kehl, V., Follo, M., Philipp, U., Sauter, A., Specht, K., Mitschke, J., Lange, T., Bauer, S., Jost, P. J., Peschel, C., Duyster, J., Gaiser, T., Hohenberger, P., & von Bubnoff, N. (2019). Circulating cKIT and PDGFRA DNA indicates disease activity in Gastrointestinal Stromal Tumor (GIST). International Journal of Cancer, 145(8), 2292-2303. https://doi.org/10.1002/ijc.32282

@article{512b4e372dca4b01bf1c35c2d71f66bf,

title = "Circulating cKIT and PDGFRA DNA indicates disease activity in Gastrointestinal Stromal Tumor (GIST)",

abstract = "This prospective trial aimed to investigate whether tumor-specific cKIT and PDGFRA mutations can be detected and quantified in circulating tumor (ct)DNA in patients with active GIST, and whether detection indicates disease activity. We included 25 patients with active disease and cKIT or PDGFRA mutations detected in tissue. Mutant ctDNA was detected in the peripheral blood plasma using allele-specific ligation (L-)PCR and droplet digital (d)PCR. CtDNA harboring tumor-specific cKIT or PDGFRA mutations was detected at least once in 16 out of 25 patients using L-PCR (64\%) and in 20 out of 25 patients with dPCR (80\%). Using dPCR, the absolute numbers of ctDNA fragments (DNA copies/ml) and the mutant allele frequency (MAF; in percent of wild-type control) strongly correlated with tumor size expressed as RECIST1.1 sum of diameter (SOD) in mm (ρ = 0.3719 and 0.408, respectively, p < 0.0001) and response status (ρ = 0.3939 and 0.392, respectively, p < 0.0001 and p < 0.001). Specificity of dPCR for detection of progression was 79.2\% with a sensitivity of 55.2\% and dPCR discriminated CR from active disease with a specificity of 96\% and s sensitivity of 44.7\%. With L-PCR, correlations of MAF with tumor size and response status were less prominent. Serial ctDNA measurement reflected individual disease courses over time. Targeted panel sequencing of four patients detected additional driver mutations in all cases and secondary resistance mutations in two cases. Thus, ctDNA indicates disease activity in patients with GIST and should be incorporated as companion biomarker in future prospective trials.",

author = "Stefanie Jilg and Michael Rassner and Jacqueline Maier and Silvia Waldeck and Victoria Kehl and Marie Follo and Ulrike Philipp and Andreas Sauter and Katja Specht and Jan Mitschke and Thoralf Lange and Sebastian Bauer and Jost, \{Philipp J.\} and Christian Peschel and Justus Duyster and Timo Gaiser and Peter Hohenberger and \{von Bubnoff\}, Nikolas",

note = "Publisher Copyright: {\textcopyright} 2019 UICC",

year = "2019",

month = oct,

day = "15",

doi = "10.1002/ijc.32282",

language = "English",

volume = "145",

pages = "2292--2303",

journal = "International Journal of Cancer",

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Jilg, S, Rassner, M, Maier, J, Waldeck, S, Kehl, V, Follo, M, Philipp, U, Sauter, A, Specht, K, Mitschke, J, Lange, T, Bauer, S, Jost, PJ, Peschel, C, Duyster, J, Gaiser, T, Hohenberger, P & von Bubnoff, N 2019, 'Circulating cKIT and PDGFRA DNA indicates disease activity in Gastrointestinal Stromal Tumor (GIST)', International Journal of Cancer, Jg. 145, Nr. 8, S. 2292-2303. https://doi.org/10.1002/ijc.32282

TY - JOUR

T1 - Circulating cKIT and PDGFRA DNA indicates disease activity in Gastrointestinal Stromal Tumor (GIST)

AU - Jilg, Stefanie

AU - Rassner, Michael

AU - Maier, Jacqueline

AU - Waldeck, Silvia

AU - Kehl, Victoria

AU - Follo, Marie

AU - Philipp, Ulrike

AU - Sauter, Andreas

AU - Specht, Katja

AU - Mitschke, Jan

AU - Lange, Thoralf

AU - Bauer, Sebastian

AU - Jost, Philipp J.

AU - Peschel, Christian

AU - Duyster, Justus

AU - Gaiser, Timo

AU - Hohenberger, Peter

AU - von Bubnoff, Nikolas

PY - 2019/10/15

Y1 - 2019/10/15

N2 - This prospective trial aimed to investigate whether tumor-specific cKIT and PDGFRA mutations can be detected and quantified in circulating tumor (ct)DNA in patients with active GIST, and whether detection indicates disease activity. We included 25 patients with active disease and cKIT or PDGFRA mutations detected in tissue. Mutant ctDNA was detected in the peripheral blood plasma using allele-specific ligation (L-)PCR and droplet digital (d)PCR. CtDNA harboring tumor-specific cKIT or PDGFRA mutations was detected at least once in 16 out of 25 patients using L-PCR (64%) and in 20 out of 25 patients with dPCR (80%). Using dPCR, the absolute numbers of ctDNA fragments (DNA copies/ml) and the mutant allele frequency (MAF; in percent of wild-type control) strongly correlated with tumor size expressed as RECIST1.1 sum of diameter (SOD) in mm (ρ = 0.3719 and 0.408, respectively, p < 0.0001) and response status (ρ = 0.3939 and 0.392, respectively, p < 0.0001 and p < 0.001). Specificity of dPCR for detection of progression was 79.2% with a sensitivity of 55.2% and dPCR discriminated CR from active disease with a specificity of 96% and s sensitivity of 44.7%. With L-PCR, correlations of MAF with tumor size and response status were less prominent. Serial ctDNA measurement reflected individual disease courses over time. Targeted panel sequencing of four patients detected additional driver mutations in all cases and secondary resistance mutations in two cases. Thus, ctDNA indicates disease activity in patients with GIST and should be incorporated as companion biomarker in future prospective trials.

AB - This prospective trial aimed to investigate whether tumor-specific cKIT and PDGFRA mutations can be detected and quantified in circulating tumor (ct)DNA in patients with active GIST, and whether detection indicates disease activity. We included 25 patients with active disease and cKIT or PDGFRA mutations detected in tissue. Mutant ctDNA was detected in the peripheral blood plasma using allele-specific ligation (L-)PCR and droplet digital (d)PCR. CtDNA harboring tumor-specific cKIT or PDGFRA mutations was detected at least once in 16 out of 25 patients using L-PCR (64%) and in 20 out of 25 patients with dPCR (80%). Using dPCR, the absolute numbers of ctDNA fragments (DNA copies/ml) and the mutant allele frequency (MAF; in percent of wild-type control) strongly correlated with tumor size expressed as RECIST1.1 sum of diameter (SOD) in mm (ρ = 0.3719 and 0.408, respectively, p < 0.0001) and response status (ρ = 0.3939 and 0.392, respectively, p < 0.0001 and p < 0.001). Specificity of dPCR for detection of progression was 79.2% with a sensitivity of 55.2% and dPCR discriminated CR from active disease with a specificity of 96% and s sensitivity of 44.7%. With L-PCR, correlations of MAF with tumor size and response status were less prominent. Serial ctDNA measurement reflected individual disease courses over time. Targeted panel sequencing of four patients detected additional driver mutations in all cases and secondary resistance mutations in two cases. Thus, ctDNA indicates disease activity in patients with GIST and should be incorporated as companion biomarker in future prospective trials.

UR - https://www.scopus.com/pages/publications/85065159590

U2 - 10.1002/ijc.32282

DO - 10.1002/ijc.32282

M3 - Journal articles

C2 - 30882891

AN - SCOPUS:85065159590

SN - 0020-7136

VL - 145

SP - 2292

EP - 2303

JO - International Journal of Cancer

JF - International Journal of Cancer

IS - 8

ER -

Circulating cKIT and PDGFRA DNA indicates disease activity in Gastrointestinal Stromal Tumor (GIST)

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