Critical Appraisal of Programmed Death Ligand 1 Reflex Diagnostic Testing: Current Standards and Future Opportunities

Humphries, Matthew P.; McQuaid, Stephen; Craig, Stephanie G.; Bingham, Victoria; Maxwell, Perry; Maurya, Manisha; McLean, Fiona; Sampson, James H.; Higgins, Patricia A.; Greene, Christine; James, Jacqueline

doi:10.1016/j.jtho.2018.09.025

Cited by 42 publications

(65 citation statements)

References 30 publications

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“…To better contrast our work with that in previous studies, we used three TPS cut-offs (< 1, 1-49% and ≥ 50%), which were used in the 22C3 assay, to evaluate PD-L1 expression. This decision was carefully considered and was based on the high concordance between the 22C3 and SP263 assays [14,24,27,28]. In our study, the expression rate of PD-L1 with TPS ≥50% as a cut-off for either histology (29.7%) or cytology (37.7%) was EBRT external beam radiotherapy; a different from previous treatments; Specimen 1 obtained earlier than specimen 2 similar to that noted in two previous studies of consecutive sample analyses [23,25].…”

Section: Discussionsupporting

confidence: 67%

“…As mentioned in many studies, PD-L1 evaluation is indeed a challenge for pathologists because it is sometimes difficult to distinguish tumor cells from immune cells, and this challenge is even more pronounced in cytology samples [23,24]. To our knowledge, it has not yet been reported whether IHC double staining for nuclear proteins such as thyroid transcription factor-1 (TTF-1) and PD-L1 can resolve this issue.…”

Section: Introductionmentioning

confidence: 99%

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Cytology cell blocks from malignant pleural effusion are good candidates for PD-L1 detection in advanced NSCLC compared with matched histology samples

Zou

Tang

et al. 2020

BMC Cancer

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Background: Detection of programmed cell death ligand-1 (PD-L1) by immunohistochemistry (IHC) has been commonly used to predict the efficacy of treatment with PD-1/PD-L1 inhibitors. However, there is limited literature regarding the reliability of PD-L1 testing using malignant pleural effusion (MPE) cell blocks. Here, we assess PD-L1 expression in sections from MPE cell blocks and evaluate the value of IHC double staining in the interpretation of PD-L1 expression. Methods: In all, 124 paired formalin-fixed tissues from advanced NSCLC patients, including MPE cell blocks and matched histology samples, were included. PD-L1 expression was assessed using the SP263 assay, and the tumor proportion score (TPS) and the staining intensity were evaluated. PD-L1 staining results were also compared between IHC double and single staining techniques. Results: PD-L1 expression was concordant in most paired cases (86/101, 85.1%) among three TPS cutoffs (<1%, 1-49% and ≥ 50%), with a kappa value of 0.774. Moreover, a significant difference in PD-L1 expression between MPE cell blocks and biopsy samples was observed (p = 0.005). For the 15 discordant pairs, 13 MPE cell block samples showed increased expression of PD-L1. Compared with the standard IHC single PD-L1 assay, double staining with anti-TTF-1 and anti-PD-L1 revealed a negative effect on PD-L1 expression testing and resulted in weaker staining intensity and a lower TPS (p = 0.000). Conclusions: MPE cell block samples are good candidates for PD-L1 expression detection in advanced NSCLC patients. The mechanism and clinical significance of the higher PD-L1 expression rate in MPE cell blocks compared with small biopsy samples remain to be evaluated prospectively.

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Section: Discussionsupporting

confidence: 67%

Section: Introductionmentioning

confidence: 99%

Cytology cell blocks from malignant pleural effusion are good candidates for PD-L1 detection in advanced NSCLC compared with matched histology samples

Zou

Tang

et al. 2020

BMC Cancer

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“…Developing a standardized procedure for cytological samples is undoubtedly challenging, since specimens can be fixed by a variety of methods and processed by different workflows. Moreover, although CBs can be prepared with distinct techniques, 18,30‐32 most studies applying PD‐L1 on cytology (Table 3) provide only few details on laboratory processing and fixation time 6‐9,11‐18 …”

Section: Discussionmentioning

confidence: 99%

“…Interestingly, 22 CBs have been included in the Blueprint (BP) PD‐L1 Immunohistochemistry Comparability Phase 2 Project, which aims to harmonize in real life practice the clinical use of different commercial PD‐L1 IHC assays on 81 routine lung cancer samples 5 . Noteworthy, several studies carried out on matched cytological and histological samples from the same patients have reported comparable results between CBs, surgical resections and small biopsy specimens in terms of adequacy rate, level of PD‐L1 expression, and clinical outcomes 6‐18 . Moreover, CBs also represent a valuable source of diagnostic material even in the early stages of the disease.…”

Section: Introductionmentioning

confidence: 99%

PD‐L1 expression in cell‐blocks of non‐small cell lung cancer: The impact of prolonged fixation

Vigliar

Iaccarino

Campione

et al. 2020

Diagnostic Cytopathology

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Introduction In the selection of non‐small cell lung cancer (NSCLC) patients for immunotherapy, specimen processed as cell blocks (CBs) may be the only available material to assess PD‐L1 expression. Therefore, optimal CB preparation becomes paramount. In this context, here we assessed whether inadequate fixation time might be one of the pre‐analytical factors affecting PD‐L1 expression. Methods Ex vivo CBs from placental (n = 3) and NSCLC (n = 8) resection specimens were obtained. PD‐L1 staining was performed on CBs prepared at increasing fixation times (12 hours, 48 hours, 72 hours, 96 hours, 168 hours and 504 hours) using the companion diagnostic SP263 Assay and a validated 22C3 laboratory developed test (LDT). Staining intensity and percentage of positive cells were evaluated. Results All placental CBs showed moderate to strong PD‐L1 positivity in most cells, regardless of the fixation time. Likewise, the percentage of SP263‐stained NSCLC cells was similar at all fixation times except for one case, which showed less intense SP263 staining at 168 hours. Conversely, in 5/8 cases, the 22C3 LDT percentage of positive cells and staining intensity decreased at 168 hours and 504 hours. Conclusions Our results show that fixation time influences the performance of 22C3 LDT on CBs. Thus, we recommend that the fixation time of cytological materials be carefully checked, especially when PD‐L1 testing is delayed until the oncology request. Indeed, delays in tissue processing and paraffin embedding may lead to sub‐optimal performance of PD‐L1 staining on CBs.

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“…However, the accelerated adoption of these diagnostic tests has highlighted several difficulties in the pathological assessment of PD-L1. We recently reported on the routine challenges faced clinically in assessment of PD-L1 [5]. This is in addition to the myriad of companion diagnostic assays available for PD-L1 and the variation in assessment criteria across tumor types [6][7][8].…”

Section: Introductionmentioning

confidence: 99%

Improving the Diagnostic Accuracy of the PD-L1 Test with Image Analysis and Multiplex Hybridization

Humphries

Bingham

Sidi

et al. 2020

Cancers

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Targeting of the programmed cell death protein (PD-1)/programmed death-ligand 1 (PD-L1) axis with checkpoint inhibitors has changed clinical practice in non-small cell lung cancer (NSCLC). However, clinical assessment remains complex and ambiguous. We aim to assess whether digital image analysis (DIA) and multiplex immunofluorescence can improve the accuracy of PD-L1 diagnostic testing. A clinical cohort of routine NSCLC patients reflex tested for PD-L1 (SP263) immunohistochemistry (IHC), was assessed using DIA. Samples of varying assessment difficulty were assessed by multiplex immunofluorescence. Sensitivity, specificity, and concordance was evaluated between manual diagnostic evaluation and DIA for chromogenic and multiplex IHC. PD-L1 expression by DIA showed significant concordance (R² = 0.8248) to manual assessment. Sensitivity and specificity was 86.8% and 91.4%, respectively. Evaluation of DIA scores revealed 96.8% concordance to manual assessment. Multiplexing enabled PD-L1+/CD68+ macrophages to be readily identified within PD-L1+/cytokeratin+ or PD-L1-/cytokeratin+ tumor nests. Assessment of multiplex vs. chromogenic IHC had a sensitivity and specificity of 97.8% and 91.8%, respectively. Deployment of DIA for PD-L1 diagnostic assessment is an accurate process of case triage. Multiplex immunofluorescence provided higher confidence in PD-L1 assessment and could be offered for challenging cases by centers with appropriate expertise and specialist equipment.

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Critical Appraisal of Programmed Death Ligand 1 Reflex Diagnostic Testing: Current Standards and Future Opportunities

Cited by 42 publications

References 30 publications

Cytology cell blocks from malignant pleural effusion are good candidates for PD-L1 detection in advanced NSCLC compared with matched histology samples

Cytology cell blocks from malignant pleural effusion are good candidates for PD-L1 detection in advanced NSCLC compared with matched histology samples

PD‐L1 expression in cell‐blocks of non‐small cell lung cancer: The impact of prolonged fixation

Improving the Diagnostic Accuracy of the PD-L1 Test with Image Analysis and Multiplex Hybridization

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