External quality assessment demonstrates that PD-L1 22C3 and SP263 assays are systematically different

Andrew Dodson; Suzanne Parry; Birgit Lissenberg-Witte; Alex Haragan; David Allen; Anthony O'Grady; Emma McClean; Jamie Hughes; Keith Miller; Erik Thunnissen

doi:10.1002/cjp2.153

External quality assessment demonstrates that PD-L1 22C3 and SP263 assays are systematically different

J Pathol Clin Res. 2020 Apr;6(2):138-145. doi: 10.1002/cjp2.153. Epub 2019 Dec 17.

Authors

Affiliations

¹ UK National External Quality Assessment Scheme for Immunocytochemistry and In-Situ Hybridisation, London, UK.
² Department of Epidemiology and Biostatistics, Amsterdam UMC, Vrije Universiteit Amsterdam, Amsterdam, The Netherlands.
³ Department of Pathology, Royal Liverpool and Broadgreen University Hospitals, Liverpool, UK.
⁴ HSL-Advanced Diagnostics, London, UK.
⁵ Department of Pathology, Royal College of Surgeons in Ireland, Beaumont Hospital, Dublin, Ireland.
⁶ Oncology, Haematology and Cellular Pathology, Guy's and St Thomas' NHS Foundation Trust, London, UK.
⁷ Department of Pathology, Amsterdam UMC, Vrije Universiteit Amsterdam, Amsterdam, The Netherlands.

Abstract

PD-L1 inhibitors are part of first line treatment options for patients with advanced non-small cell lung cancer. PD-L1 immunohistochemistry (IHC) assays act as either a companion or a complementary diagnostic. The purpose of this study is to describe the experience of external quality assurance (EQA) provider UK NEQAS ICC and ISH with the comparison of different PD-L1 assays used in daily practice. Three EQA rounds (pilot, run A and run B) were carried out using formalin fixed paraffin embedded samples with sample sets covering a range of epitope concentrations, including 'critical samples' near to clinical threshold cut-offs. An expert panel (n = 4) evaluated all returned slides simultaneously and independently on a multi-header microscope together with the participants own in-house control material. The tonsil sample was evaluated as 'acceptable' or 'unacceptable', and for the other samples the percentage of PD-L1 stained tumour cells were estimated in predetermined categories (<1%, 1 to <5%, 5 to <10%, 10 to <25%, 25 to <50%, 50 to <80%, 80 to 100%). In the pilot and the two subsequent runs the number of participating laboratories was 43, 69 and 76, respectively. The pass rate for the pilot run was 67%; this increased to 81% at run A and 82% at run B. For two 'critical samples', in runs A and B, 22C3 IHC had significantly higher PD-L1 expression than SP263 IHC (p < 0.001), whilst the PD-L1 scores for the other six samples were similar for all assays. In run A the laboratory developed tests (LDTs) using 22C3 scored lower than the commercial 22C3 tests (p = 0.01). After the initial testing, improvement in performance of PD-L1 IHC is shown for approved and LDT PD-L1 assays. Equivalency of approved PD-L1 22C3 and SP263 assays cannot be assumed as the scores cross the clinically relevant thresholds of 1% and 50% PD-L1 expression.

Keywords: PD-L1; companion diagnostic assays; external quality assessment; immunohistochemistry; non-small cell lung cancer; predictive testing.

MeSH terms

Antibodies, Monoclonal / therapeutic use*
B7-H1 Antigen / immunology*
B7-H1 Antigen / metabolism
Biomarkers, Tumor / metabolism
Carcinoma, Non-Small-Cell Lung / drug therapy*
Carcinoma, Non-Small-Cell Lung / metabolism
Carcinoma, Non-Small-Cell Lung / pathology
Female
Humans
Lung Neoplasms / drug therapy*
Lung Neoplasms / metabolism
Lung Neoplasms / pathology
Male

Substances

Antibodies, Monoclonal
B7-H1 Antigen
Biomarkers, Tumor
CD274 protein, human