Next generation sequencing of PD-L1 for predicting response to immune checkpoint inhibitors

Jeffrey M Conroy; Sarabjot Pabla; Mary K Nesline; Sean T Glenn; Antonios Papanicolau-Sengos; Blake Burgher; Jonathan Andreas; Vincent Giamo; Yirong Wang; Felicia L Lenzo; Wiam Bshara; Maya Khalil; Grace K Dy; Katherine G Madden; Keisuke Shirai; Konstantin Dragnev; Laura J Tafe; Jason Zhu; Matthew Labriola; Daniele Marin; Shannon J McCall; Jeffrey Clarke; Daniel J George; Tian Zhang; Matthew Zibelman; Pooja Ghatalia; Isabel Araujo-Fernandez; Luis de la Cruz-Merino; Arun Singavi; Ben George; Alexander C MacKinnon; Jonathan Thompson; Rajbir Singh; Robin Jacob; Deepa Kasuganti; Neel Shah; Roger Day; Lorenzo Galluzzi; Mark Gardner; Carl Morrison

doi:10.1186/s40425-018-0489-5

Next generation sequencing of PD-L1 for predicting response to immune checkpoint inhibitors

J Immunother Cancer. 2019 Jan 24;7(1):18. doi: 10.1186/s40425-018-0489-5.

Authors

Jeffrey M Conroy^{1

2}, Sarabjot Pabla¹, Mary K Nesline¹, Sean T Glenn^{1

2}, Antonios Papanicolau-Sengos¹, Blake Burgher¹, Jonathan Andreas¹, Vincent Giamo¹, Yirong Wang¹, Felicia L Lenzo¹, Wiam Bshara², Maya Khalil², Grace K Dy², Katherine G Madden³, Keisuke Shirai³, Konstantin Dragnev³, Laura J Tafe³, Jason Zhu⁴, Matthew Labriola⁴, Daniele Marin⁴, Shannon J McCall⁴, Jeffrey Clarke⁴, Daniel J George⁴, Tian Zhang⁴, Matthew Zibelman⁵, Pooja Ghatalia⁵, Isabel Araujo-Fernandez⁶, Luis de la Cruz-Merino⁶, Arun Singavi⁷, Ben George⁷, Alexander C MacKinnon⁷, Jonathan Thompson⁷, Rajbir Singh⁸, Robin Jacob⁸, Deepa Kasuganti⁹, Neel Shah⁹, Roger Day¹⁰, Lorenzo Galluzzi^{11

12

13}, Mark Gardner¹, Carl Morrison^{14

15}

Affiliations

¹ OmniSeq, Inc., 700 Ellicott Street, Buffalo, NY, 14203, USA.
² Roswell Park Comprehensive Cancer Center, Elm and Carlton Streets, Buffalo, NY, 14263, USA.
³ Dartmouth-Hitchcock Medical Center, Lebanon, NH, 03756, USA.
⁴ Duke University Medical Center, 905 S. Lasalle Street, Durham, NC, 27710, USA.
⁵ Fox Chase Cancer Center, 333 Cottman Ave, Philadelphia, PA, 19111, USA.
⁶ Hospital Universitario Virgen Macarena, 41009, Sevilla, Spain.
⁷ Medical College of Wisconsin, 8701 W Watertown Plank Rd, Milwaukee, WI, 53226, USA.
⁸ Meharry Medical College, 1005 Dr DB Todd Jr Blvd, Nashville, TN, 37208, USA.
⁹ Community Hospital, Munster, IN, 46321, USA.
¹⁰ University of Pittsburgh, Pittsburgh, PA, 15213, USA.
¹¹ Department of Radiation Oncology, Weill Cornell Medical College, New York, NY, 10065, USA.
¹² Sandra and Edward Meyer Cancer Center, New York, NY, 10065, USA.
¹³ Université Paris Descartes/Paris V, 75006, Paris, France.
¹⁴ OmniSeq, Inc., 700 Ellicott Street, Buffalo, NY, 14203, USA. Carl.Morrison@roswellpark.org.
¹⁵ Roswell Park Comprehensive Cancer Center, Elm and Carlton Streets, Buffalo, NY, 14263, USA. Carl.Morrison@roswellpark.org.

Abstract

Background: PD-L1 immunohistochemistry (IHC) has been traditionally used for predicting clinical responses to immune checkpoint inhibitors (ICIs). However, there are at least 4 different assays and antibodies used for PD-L1 IHC, each developed with a different ICI. We set to test if next generation RNA sequencing (RNA-seq) is a robust method to determine PD-L1 mRNA expression levels and furthermore, efficacy of predicting response to ICIs as compared to routinely used, standardized IHC procedures.

Methods: A total of 209 cancer patients treated on-label by FDA-approved ICIs, with evaluable responses were assessed for PD-L1 expression by RNA-seq and IHC, based on tumor proportion score (TPS) and immune cell staining (ICS). A subset of serially diluted cases was evaluated for RNA-seq assay performance across a broad range of PD-L1 expression levels.

Results: Assessment of PD-L1 mRNA levels by RNA-seq demonstrated robust linearity across high and low expression ranges. PD-L1 mRNA levels assessed by RNA-seq and IHC (TPS and ICS) were highly correlated (p < 2e-16). Sub-analyses showed sustained correlation when IHC results were classified as high or low by clinically accepted cut-offs (p < 0.01), and results did not differ by tumor type or anti-PD-L1 antibody used. Overall, a combined positive PD-L1 result (≥1% IHC TPS and high PD-L1 expression by RNA-Seq) was associated with a 2-to-5-fold higher overall response rate (ORR) compared to a double negative result. Standard assessments of sensitivity, specificity, positive predictive value (PPV), and negative predictive value (NPV) showed that a PD-L1 positive assessment for melanoma samples by RNA-seq had the lowest sensitivity (25%) but the highest PPV (72.7%). Among the three tumor types analyzed in this study, the only non-overlapping confidence interval for predicting response was for "RNA-seq low vs high" in melanoma.

Conclusions: Measurement of PD-L1 mRNA expression by RNA-seq is comparable to PD-L1 expression by IHC both analytically and clinically in predicting ICI response. RNA-seq has the added advantages of being amenable to standardization and avoidance of interpretation bias. PD-L1 by RNA-seq needs to be validated in future prospective ICI clinical studies across multiple histologies.

Keywords: Atezolizumab; Avelumab; Biomarker; Durvalumab; Nivolumab; PD-L1; Pembrolizumab; cancer immunotherapy.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Antineoplastic Agents, Immunological / therapeutic use*
B7-H1 Antigen / antagonists & inhibitors
B7-H1 Antigen / genetics*
B7-H1 Antigen / metabolism
Humans
Immunohistochemistry
Neoplasms / drug therapy*
Neoplasms / genetics*
Neoplasms / metabolism
RNA, Messenger / genetics
RNA-Seq

Substances

Antineoplastic Agents, Immunological
B7-H1 Antigen
CD274 protein, human
RNA, Messenger

Grants and funding

P30 CA014236/CA/NCI NIH HHS/United States