False‐negative programmed death‐ligand 1 immunostaining in ethanol‐fixed endobronchial ultrasound‐guided transbronchial needle aspiration specimens of non‐small‐cell lung cancer patients

False‐negative programmed death‐ligand 1 immunostaining in ethanol‐fixed endobronchial ultrasound‐guided transbronchial needle aspiration specimens of non‐small‐cell lung cancer patients

Aims Programmed death‐ligand 1 (PD‐L1) immunostaining is used to predict which non‐small‐cell lung cancer (NSCLC) patients will respond best to treatment with programmed cell death protein 1/PD‐L1 inhibitors. PD‐L1 immunostaining is sometimes performed on alcohol‐fixed cytological specimens instead...

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Veröffentlicht in:Histopathology 2021-10, Vol.79 (4), p.480-490
Hauptverfasser: Koomen, Bregje M, Vreuls, Willem, Boer, Mirthe, Ruiter, Emma J, Hoelters, Juergen, Vink, Aryan, Willems, Stefan M
Format: Artikel
Sprache:eng
Schlagworte:
22C3 antibody
Apoptosis
B7-H1 Antigen - analysis
Biomarkers, Tumor - analysis
Carcinoma, Non-Small-Cell Lung
Cell death
cytology
Endoscopic Ultrasound-Guided Fine Needle Aspiration - methods
Ethanol
False Negative Reactions
Formaldehyde
Humans
immunohistochemistry
Immunohistochemistry - methods
immunotherapy
Ligands
Lung cancer
Lung Neoplasms
Non-small cell lung carcinoma
Organ Preservation Solutions
Original
Paraffin
Patients
PD-1 protein
PD-L1 protein
programmed cell death‐ligand 1
SP263 antibody
tissue fixation
Tissue Fixation - methods
Ultrasonic imaging
Ultrasound
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Zusammenfassung:Aims Programmed death‐ligand 1 (PD‐L1) immunostaining is used to predict which non‐small‐cell lung cancer (NSCLC) patients will respond best to treatment with programmed cell death protein 1/PD‐L1 inhibitors. PD‐L1 immunostaining is sometimes performed on alcohol‐fixed cytological specimens instead of on formalin‐fixed paraffin‐embedded (FFPE) biopsies or resections. We studied whether ethanol prefixation of clots from endobronchial ultrasound‐guided transbronchial needle aspiration (EBUS‐TBNA) results in diminished PD‐L1 immunostaining as compared with formalin fixation. Methods and results FFPE cell blocks from EBUS‐TBNA specimens of 54 NSCLC patients were identified. For each case, paired samples were available, consisting of clots directly immersed in formalin and clots prefixed in Fixcyt (50% ethanol). Serial sections were immunostained for PD‐L1 by use of the standardised SP263 assay and the 22C3 antibody as a laboratory‐developed test (LDT). PD‐L1 positivity was determined with two cut‐offs (1% and 50%). Concordance of PD‐L1 positivity between the formalin‐fixed (gold standard) and ethanol‐prefixed material was assessed. When the 22C3 LDT was used, 30% and 36% of the ethanol‐prefixed specimens showed false‐negative results at the 1% and 50% cut‐offs, respectively (kappa 0.64 and 0.68). When SP263 was used, 22% of the ethanol‐prefixed specimens showed false‐negative results at the 1% cut‐off (kappa 0.67). At the 50% cut‐off, concordance was higher (kappa 0.91), with 12% of the ethanol‐prefixed specimens showing false‐negative results. Conclusion Ethanol fixation of EBUS‐TBNA specimens prior to formalin fixation can result in a considerable number of false‐negative PD‐L1 immunostaining results when a 1% cut‐off is used and immunostaining is performed with SP263 or the 22C3 LDT. The same applies to use of the 50% cut‐off when immunostaining is performed with the 22C3 LDT.
ISSN:0309-0167
1365-2559
1365-2559
DOI:10.1111/his.14373