Tumor mutational burden and purity adjustment before and after treatment with temozolomide in 27 paired samples of glioblastoma: a prospective study

Dorte Schou Nørøxe; Aidan Flynn; Christina Westmose Yde; Olga Østrup; Finn Cilius Nielsen; Jane Skjøth-Rasmussen; Jannick Brennum; Petra Hamerlik; Joachim Weischenfeldt; Hans Skovgaard Poulsen; Ulrik Lassen

doi:10.1002/1878-0261.13015

Tumor mutational burden and purity adjustment before and after treatment with temozolomide in 27 paired samples of glioblastoma: a prospective study

Mol Oncol. 2022 Jan;16(1):206-218. doi: 10.1002/1878-0261.13015. Epub 2021 Jun 25.

Authors

Dorte Schou Nørøxe^{1

2}, Aidan Flynn^{3

4}, Christina Westmose Yde⁵, Olga Østrup⁵, Finn Cilius Nielsen⁵, Jane Skjøth-Rasmussen⁶, Jannick Brennum⁶, Petra Hamerlik⁷, Joachim Weischenfeldt^{3

4}, Hans Skovgaard Poulsen^{1

2}, Ulrik Lassen²

Affiliations

¹ Department of Radiation Biology, Rigshospitalet, Copenhagen, Denmark.
² Department of Oncology, Rigshospitalet, Copenhagen, Denmark.
³ Biotech Research and Innovation Centre (BRIC), University of Copenhagen, Denmark.
⁴ Finsen Laboratory, Rigshospitalet, Copenhagen, Denmark.
⁵ Center for Genomic Medicine, Rigshospitalet, Copenhagen, Denmark.
⁶ Department of Neuro Surgery, Rigshospitalet, Copenhagen, Denmark.
⁷ Danish Cancer Society, Copenhagen, Denmark.

Abstract

Treatment of glioblastoma (GBM) remains a challenging task, with limited treatment options, none offering a cure. Immune therapy has proven effective across different cancers with remarkable response rates. Tumor mutational burden (TMB) is a marker of response, but technical and methodological differences in TMB estimates have made a proper assessment and comparison challenging. Here, we analyzed a prospective collection of paired samples from 35 patients with newly diagnosed GBM, all of whom were wild-type (WT) for isocitrate dehydrogenase, before and after treatment with radiotherapy and temozolomide. Seven patients (20%) had O6-methylguanine-DNA methyltransferase-methylated tumors. Six patients (17%) had two relapse surgeries, and tissue from all three surgeries was collected. We found that accurate evaluation of TMB was confounded by high variability in the cancer cell fraction of relapse samples. To ameliorate this, we developed a model to adjust for tumor purity based on the relative density distribution of variant allele frequencies in each primary-relapse pair. Additionally, we examined the mutation spectra of shared and private mutations. After tumor purity adjustment, we found TMB comparison reliable in tumors with tumor purity between 15% and 40%, resulting in 27/35 patients (77.1%). TMB remained unchanged from 0.65 mutations per megabase (Mb) to 0.67/Mb before and after treatment, respectively. Examination of the mutation spectra revealed a dominance of C > T transitions at CpG sites in both shared and relapse-private mutations, consistent with cytosine deamination and the clock-like mutational signature 1. We present and apply a cellularity correction approach that enables more accurate assessment of TMB in paired tumor samples. We did not find a significant increase in TMB after correcting for cancer cell fraction. Our study raises significant concerns when determining TMB. Although a small sample size, corrected TMB can have a clinical significance when stratifying patients to experimental treatment, for example, immune checkpoint therapy.

Keywords: glioblastoma; immune therapy; paired samples; temozolomide; tumor mutational burden; tumor purity.

MeSH terms

Biomarkers, Tumor / genetics
Glioblastoma* / drug therapy
Glioblastoma* / genetics
Humans
Mutation / genetics
Neoplasm Recurrence, Local
Prospective Studies
Temozolomide / pharmacology
Temozolomide / therapeutic use
Tumor Burden / genetics

Substances

Biomarkers, Tumor
Temozolomide