Abstract 17P
Background
Early CD8+ T cell responses to PD-1 blockade are well-characterised. However, an understanding of the long-term clonal and transcriptomic signatures of complete response (CR) to Immune Checkpoint Blockade (ICB) is currently lacking. We aimed to identify and describe CD8+ T cell clonal and transcriptomic changes post complete response to PD-1 blockade in metastatic melanoma (MM).
Methods
We performed single-cell RNA sequencing (scRNAseq) of both the T cell receptor (TCR) and transcriptomes of PBMCs and sorted peripheral CD8+ T cells in patients with MM with a complete response to PD-1 blockade (n=10), patients with progressive disease (PD, n=6) and healthy donors (HD, n=2). Blood was sampled at multiple time points, including a median of 3.2 years following cessation of PD-1 blockade for CR.
Results
Following a CR and cessation of ICB, there is increased abundance of a subtype of CD8+ T cell characterised by high expression of NK-associated genes, termed a killer-like subset. Using the top 25 genes upregulated by this subset to generate a ‘Killer Score’, we show that patients with CR to anti-PD-1 demonstrate a broad increase in killer gene expression over time absent in those with PD and HDs. By tracking key clones through TCR usage, we identify those which are stable/expanding from pre-treatment to post treatment, occupy >0.5% of the repertoire and are persistent post-cessation of ICB, terming these large expanding persistent clones. These clones have a predominantly cytotoxic, effector, gene expression profile and display surface markers consistent with a recently-described ‘Long-lived Effector Cell’ subtype.
Conclusions
CR to PD-1 blockade is associated with persistence of highly-cytotoxic effector CD8+ T cells that circulate years after cessation of treatment. Whilst similar subsets have been implicated with chronic viral infection, these observations are novel in the cancer setting and have important implications for mechanisms of durable disease control.
Clinical trial identification
Editorial acknowledgement
Legal entity responsible for the study
The authors.
Funding
The Wellcome Trust, Cancer Research UK, National Institute for Health Research.
Disclosure
All authors have declared no conflicts of interest.
Resources from the same session
78P - Peroxiredoxin-1 knockout negatively affects the viability of ph+ B-cell acute lymphoblastic leukemia cells and sensitizes them to tyrosine kinase inhibitors
Presenter: Jaromir Hunia
Session: Poster session 09
79P - Co-delivered crizotinib and gefitinib based on nanoparticle for synergically overcoming resistance lung adenocarcinoma treatment
Presenter: Haiyu Zhou
Session: Poster session 09
80P - Steroidal oximes: A new potential therapeutic approach for cancer treatment
Presenter: Mafalda Laranjo
Session: Poster session 09
81P - miR-23b and -133a role on TRAIL-induced apoptosis pathway components expression and TRAIL sensitization in lung adenocarcinoma cells
Presenter: Denise Leite
Session: Poster session 09
83P - Impact of VHL-associated tumor treatment on mental health: An international patient survey
Presenter: Othon Iliopoulos
Session: Poster session 09
84P - Microenvironment immune differences between sexes in multiple myeloma
Presenter: Maria de los Angeles Clavo
Session: Poster session 09
85P - In silico evaluation of the transcriptomic and immunologic profile of lung adenocarcinomas with deletions or disruptive mutations of SMARCA4
Presenter: Ester Garcia Lorenzo
Session: Poster session 09
86P - Effect of chemotherapy-induced autophagic secretome on natural killer cell activity
Presenter: Ayfer Karlitepe
Session: Poster session 09
87P - WIP1 phosphatase promotes etoposide induced autophagy in medulloblastoma and neuroblastoma
Presenter: Hatice Pilevneli
Session: Poster session 09
88P - PPM1D/WIP1 phosphatase mediates basal and genotoxic stress-induced autophagy via ULK-1 de-phosphorylation
Presenter: Ceylan Ak
Session: Poster session 09