Analytical Validation of a Next-Generation Sequencing Assay to Monitor Immune Responses in Solid Tumors

被引:60
|
作者
Conroy, Jeffrey M. [1 ,2 ]
Pabla, Sarabjot [1 ]
Glenn, Sean T. [1 ,3 ]
Burgher, Blake [1 ]
Nesline, Mary [1 ]
Papanicolau-Sengos, Antonios [1 ]
Andreas, Jonathan [1 ]
Giamo, Vincent [1 ]
Lenzo, Felicia L. [1 ]
Hyland, Fiona C. L. [6 ]
Omilian, Angela [4 ]
Bshara, Wiam [4 ]
Qin, Moachun [1 ]
He, Ji [1 ]
Puzanov, Igor [5 ]
Ernstoff, Marc S. [5 ]
Gardner, Mark [1 ]
Galluzzi, Lorenzo [7 ,8 ,9 ]
Morrison, Carl [1 ,2 ]
机构
[1] OmniSeq Inc, 700 Ellicott St, Buffalo, NY 14203 USA
[2] Roswell Pk Canc Inst, Ctr Personalized Med, Buffalo, NY 14263 USA
[3] Roswell Pk Canc Inst, Ctr Canc Genet & Genom, Buffalo, NY 14263 USA
[4] Roswell Pk Canc Inst, Dept Pathol, Buffalo, NY 14263 USA
[5] Roswell Pk Canc Inst, Dept Med, Buffalo, NY 14263 USA
[6] Thermo Fisher Sci, Clin Next Generat Sequencing Div, San Francisco, CA USA
[7] Weill Cornell Med Coll, Dept Radiat Oncol, New York, NY USA
[8] Sandra & Edward Meyer Canc Ctr, New York, NY USA
[9] Univ Paris Descartes Paris V, Paris, France
来源
JOURNAL OF MOLECULAR DIAGNOSTICS | 2018年 / 20卷 / 01期
关键词
CANCER-THERAPY; CHEMOTHERAPY; INFILTRATE; QUALITY;
D O I
10.1016/j.jmoldx.2017.10.001
中图分类号
R36 [病理学];
学科分类号
100104 ;
摘要
We have developed a next-generation sequencing assay to quantify biomarkers of the host immune response in formalin-fixed, paraffin-embedded (FFPE) tumor specimens. This assay aims to provide clinicians with a comprehensive characterization of the immunologic tumor microenvironment as a guide for therapeutic decisions on patients with solid tumors. The assay relies on RNA-sequencing (seq) to semi-quantitatively measure the levels of 43 transcripts related to anticancer immune responses and 11 transcripts that reflect the relative abundance of tumor-infiltrating lymphocytes, as well as on DNA-seq to estimate mutational burden. The assay has a clinically relevant 5-day turnaround time and can be conducted on as little as 2.5 ng of RNA and 1.8 ng of genomic DNA extracted from three to five standard FFPE sections. The standardized next-generation sequencing workflow produced sequencing reads adequate for clinical testing of matched RNA and DNA from several samples in a single run. Assay performance for gene-specific sensitivity, Linearity, dynamic range, and detection threshold was estimated across a wide range of actual and artificial FFPE samples selected or generated to address preanalytical variability linked to specimen features (eg, tumor-infiltrating lymphocyte abundance, percentage of necrosis), and analytical variability linked to assay features (eg, batch size, run, day, operator). Analytical precision studies demonstrated that the assay is highly reproducible and accurate compared with established orthogonal approaches.
引用
收藏
页码:95 / 109
页数:15
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