| Autor: |
Kaushal Parikh, MD, Faye R. Harris, MS, Giannoula Karagouga, MS, Amy Schrandt, CRA, Jay Mandrekar, PhD, Sarah Johnson, MS, Alexa McCune, BS, Dorsay Sadeghian, MD, Debarshi Roy, PhD, Katarzyna Polonis, PhD, Athanasios Gaitatzes, MS, Aaron O. Bungum, BS, Eric S. Edell, MD, Mitesh J. Borad, MD, Tobias Peikert, MD, Farhad Kosari, PhD, John Cheville, MD, George Vasmatzis, PhD, Aaron S. Mansfield, MD |
| Jazyk: |
angličtina |
| Rok vydání: |
2024 |
| Předmět: |
|
| Zdroj: |
JTO Clinical and Research Reports, Vol 5, Iss 12, Pp 100692- (2024) |
| Druh dokumentu: |
article |
| ISSN: |
2666-3643 |
| DOI: |
10.1016/j.jtocrr.2024.100692 |
| Popis: |
Introduction: The spatially complex nature of mesothelioma and interventions like pleurodesis, surgery, and radiation often complicate imaging-based assessment. Further, cell-free DNA (cfDNA) based monitoring strategies are inadequate for mesothelioma, given the presence of a few recurring nonsynonymous somatic variants. However, patient-specific chromosomal rearrangements are commonly found in mesothelioma. Our study objective was to develop an individualized cfDNA assay to enable blood-based monitoring using circulating tumor DNA (ctDNA) in mesothelioma. We hypothesized that the unique chromosomal rearrangement junctions found in mesothelioma could be employed for individualized ctDNA detection and disease monitoring. Methods: DNA was extracted from tumor specimens for whole genome sequencing. Chromosomal junctions, prioritized by highest allele frequency and low homology to the rest of the genome, were selected for detection. Primers and Taqman probes were designed to span the junctions, forming personalized junction panels. Patient plasma obtained before therapy and at response assessment was tested for the presence of personalized junctions via quantitative polymerase chain reaction. Results: Our study included nine patients, four with peritoneal and five with pleural mesothelioma. 763 chromosomal junctions were identified in the tumors of all cases. We selected three to five junctions per sample for quantitative polymerase chain reaction. We detected 25/30 (83%) of selected junctions in the plasma of seven out of nine patients (78%). Cell-free junction detection at follow-up was concordant with disease status: cfDNA junctions were detected in three patients with persistent disease, and not detected in a patient with no evidence of disease after surgery. Conclusions: With further validation, individualized ctDNA junction assays could supplement imaging for disease monitoring in mesothelioma. |
| Databáze: |
Directory of Open Access Journals |
| Externí odkaz: |
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