Tumor samples from NSCLC patients were obtained from biopsy specimens. A portion of the sample was removed for formalin fixation and paraffin embedding (FFPE). The remainder of the tissue was immediately frozen in aliquots and stored in vapor-phase liquid nitrogen.

PBMCs obtained for immune monitoring or as starting material for the manufacturing process were isolated by Ficoll-Hypaque (Amersham Biosciences) density gradient centrifugation from buffy coats of healthy donors or from peripheral blood samples of NSCLC patients. Immature dendritic cells (DCs) were generated as described previously (18, 19). T2 and H522 cells (ATCC) were cultured under standard conditions. T2 and H522cells were stably transfected with the A2.1/Kb chimeric gene (T2/Kb, H522/Kb) for mice experiments. T2/Kb and H522/kb cells were stable transfectants and express the product of the HLA-A*02:01/Kb chimeric gene (the α1 and α2 domains from HLA-A*0201 and the α3 domain of H-2K^b (20). Cell banks were generated and tested for mycoplasma. The cells were reauthenticated short tandem repeat (STR) profiling at ATCC.

For WES sequencing, DNA from fresh frozen tumor samples or cells was extracted using the DNeasy Blood and Tissue Kit, which was purchased from Qiagen. The genomic DNA was sheared, end-repaired, ligated to barcoded Illumina sequencing adapters, amplified, and size-selected. Whole-exome capture was performed using an Agilent Sure Select Human All Exon 44-Mb version 2.0 bait set (Agilent Technologies) (21). The resulting libraries were then quantified by qPCR, pooled, and sequenced using 76-basepaired-end reads obtained with HiSeq 2000 or 2500 sequencers (Illumina).

For RNA sequencing, RNA from fresh frozen tumor samples was extracted using the RNeasy Mini Kit. RNA-seq libraries were prepared using an Illumina TruSeq Stranded mRNA Library Prep Kit (for cell suspensions). Flow cell cluster amplification and sequencing were performed according to the manufacturer’s instructions using either a HiSeq2500.

The sequencing data have been deposited in the NCBI Sequence Read Archive (SRA) database under the accession code SRP (https://submit.ncbi.nlm.nih.gov/subs/sra/SUB8559404/overview).

All mutanome-related data analysis steps for a single patient were coordinated by a software pipeline implemented in the Python programming language. At least 150× 10⁶and 75× 10⁶ paired-end 50 nt reads were required for the DNA and RNA libraries, respectively. For mutation detection, the DNA reads were aligned to the reference genome hg19 with BWA (22). Duplicate exomes from tumor and matched normal samples were analyzed for single-nucleotide variants. Loci with putative homozygous genotypes in the normal samples were identified and filtered to retain high-confidence calls for single-nucleotide variants. The remaining sites were further inspected for a putative homozygous or heterozygous mutational event. The suspected sites were filtered to remove potential false positives, and replicates were incorporated by testing both the sum of replicates and the replicates separately. The final list of single-nucleotide variants was composed of high-confidence homozygous sites in the normal samples and high-confidence heterozygous or homozygous mutational events in the tumor samples. The genomic coordinates of identified variants were compared with known gene transcript coordinates detailed in the UCSC Genome Browser to determine the association of the variants with genes, transcripts, potential amino acid sequence changes and RNA-seq-derived expression values.

For RNA-seq, RNA reads were aligned to the hg19 reference genome and transcriptome using Bowtie (23), and the gene expression levels were determined by comparison with known gene transcript and exon coordinates detailed in UCSC followed by normalization to RPKM units (16).

A tandem minigene (TMG) was constructed as previously described (30). Minigenes were included in each TMG construct used in this study. Plasmids encoding the minigenes were linearized with the restriction enzyme NsiI, and each linearized plasmid was used as a template for in vitro transcription using the mMESSAGE mMACHINE T7 Transcription Kit (Thermo Fisher Scientific) according to the manufacturer’s instructions.

The autologous PBMCs from the patients were harnessed to evaluate the immunogenicity of the candidate neoantigens in vitro. An established simple and effective culture protocol with a few modifications (31, 32) was applied to detect and monitor the antigen peptide-specific cytotoxic T lymphocyte precursors (CTL-P) in the circulation. Briefly, heparinized blood samples were obtained from patients with relapsed/refractory tumors for the isolation of PBMCs by centrifugation on a Ficoll density gradient, and the isolated PBMCs were suspended in AIM-V medium (Gibco). In each U-bottomed well of a plate, 1 × 10⁵ PBMCs were incubated with a corresponding peptide (25 μM) in 200μl of culture medium, which was applied to facilitate cell-to-cell contact. The culture medium consisted of AIM-V medium, 10% FCS (Gibco), and IL-2 (100 U/ml; PeproTech). For peptide stimulation, half of the culture medium was replaced with fresh medium containing the corresponding peptide (25 μM) and IL-2 (100 U/ml) at 3-day intervals. After three cycles of peptide stimulation followed by overnight re-stimulation, the specific T cell responses to each peptide were evaluated through an ELISPOT assay on day 10. The recognition of each single antigen was tested in comparison with the no-peptide control (medium only), and phytohemagglutinin was used as the positive control. In some cases, the reactivity of T cells was evaluated by peptide pulsing of DCs cocultured with T cells. Mature DCs were pulsed with 10 μM peptide for 4–6 hours at 37°C, washed with prewarmed PBS, and then incubated overnight with T cells at a stimulator/effector ratio of 1:10 in complete AIM-V medium. IFN-γ-secreting cells was determined by IFN-γ ELISPOT assay.

The preparation of bone marrow-derived DCs from Tg mice and the vaccination of HLA-A2.1/K^bTg mice (10 mice per group)with peptide-pulsed DCs were performed as described previously (33). On day 7 after the last immunization with peptide-pulsed DCs, all the immune splenocytes from the same group of primed mice were collected, cultured at a density of 1 × 10⁷ cells per well in six-well plates and stimulated with peptides (20 μM) for 7 days in vitro. The bulk populations were functionally tested by enzyme-linked immunospot assay (ELISPOT), enzyme-linked immunosorbent assay (ELISA), intracellular staining assays, and time-resolved fluorescence assays.

ELISPOT kits (Dakewei) was used to determine the amount of cytokine-secreting T cells after overnight activation with a peptide (34). In this study, a multiple culture protocol was used to analyze the T cell response as described above. Briefly, the peptide-stimulated PBMCs or the DC-pulsed peptide coculture with T cells (10⁵ per well) were added to duplicate wells for 18–20 hours. The plates were washed before addition of the diluted detection antibody (1:100 dilution) and then incubated for 1 hour at 37°C. After the plates were washed, streptavidin–HRP (1:100 dilution) was added, and the plates were incubated at 37°C for 1 hour. 3-Amino-9-ethylcarbazole (AEC) solution mix was then added to each well, and the plates were left in the dark for approximately 15–25 minutes at room temperature. Deionized water was then added to stop the reaction, and the plates were subsequently scanned using an ELISPOT CTL Reader (Cellular Technology Inc.). The results were analyzed with ELISPOT software (AID). Spots with a size that were more than twofold greater than that of the no-peptide control (medium only) were considered positive for T cell reactivity.

Cytotoxicity assays were performed using time-resolved fluorescence assay as previously described (35, 36). Briefly, target cells were labeled with a fluorescence enhancing ligand (BADTA)and co-incubated with NRT cells for 2h. The supernatants were then measured by time-resolved fluorometry (EnVision 2014Multilabel reader, PerkinElmer). The percent specific lysis was determined according to the following formula: (experimental release −spontaneous release)/(maximum release −spontaneous release)) × 100% and the percent spontaneous release was calculated from(spontaneous release – background signal)/(maximum release − background signal) × 100%.

Splenocytes from each group of immunized HLA-A2.1/K^b mice were stimulated with 20 μMACAD8-T105I, BCAR1-G23V or PLCG1-M425Lfor 7 days as described in the section detailing the protocol used for the cytotoxicity assay. HLA-A*02:01⁺H522/Kb-minigene tumor cells (5 × 10⁶) were injected s.c. into the flanks of C57BL/6nu/nu mice, which formed homogeneous tumors in 100% of the mice. Three days later (37–41), the mice were intravenously injected with splenocytes (1 × 10⁸ cells per mouse) from each group of immunized HLA-A2.1/K^b mice that were stimulated with 20 μM ACAD8-T105I, BCAR1-G23V and PLCG1-M425L for 7 days as described in the section detailing the protocol used for the cytotoxicity assay. This adoptive transfer was performed twice at 1-week intervals and was followed by the intraperitoneal administration of 2000 U of hIL-2 every 2 days. The control mice received splenocytes from HLA-A2.1/K^b mice immunized with irrelevant peptide -pulsed DCs or only IL-2. The tumor size and body weight were measured in two perpendicular dimensions three times at weekly intervals. The mice were killed 80 days after tumor inoculation.

GraphPad Prism 5.0 (GraphPad Software) was used for all statistical analyses. The data samples were compared using two-tailed Student’s t test, and a P value less than 0.05 was considered significant.

Whole-exome sequencing of tumor specimens and matched normal samples from three NSCLC patients (Clinicopathological characteristics of the subjects were presented in Supplementary Table 3 ) was performed after DNA extraction, and the resulting genetic mutations and HLA typing information were then analyzed ( Supplementary Table 1 ). RNA was also extracted, and transcriptome sequencing was performed to confirm the genetic mutations and identify mutant gene expression level. Patient somatic mutations and RNA expression were analyzed by MuPeXI to identify neoantigen candidates. An average of 184 non-synonymous somatic mutations were detected ( Figure 1A ) and an average of 145MHC I-restricted neoantigens (range of 97-226) and an average of 38 MHC II-restricted neoantigens (range of 32-46) were identified in 3 NSCLC patients ( Supplementary Table 2 ). An average of 34 neoantigens were considered as strong binders with %rank less than 0.5, and an average of 150 neoantigens were considered as weaker binders with %rank larger than 0.5 ( Figure 1B ). Ten putative mutation-associated long peptides (27 aa) with strong HLA affinity were selected from each patient and produced by chemosynthesis ( Table 1 ).

In order to identify the neoantigen with high immunogenicity, an established simple and effective polypeptide immunogenicity assay with a few modifications (31) was applied to test the immunogenicity of the synthesized neoantigen polypeptides based on NSCLC patient-derived PBMCs. The neoantigens GPM6B-C94F, DMXL1-L2124F,TPBG-P57L,HACE1-T20S and COQ3-T91A from HLA-0206⁺ Patient 01 (P01), OPLAH-G890D, BCAR1-V64L,GBF1-D1478Y,SNX16-C318Y and UPF3A-R380T fromHLA-0207⁺ and HLA-3303⁺ Patient 02(P02) andACAD8-T105I, BCAR1-G23V,SCLC7A1-A349S, SSH1-R470C and PLCG1-M425L from HLA-0201⁺ Patient 03(P03) elicited more obvious peptide-specific T-cell responses than the no-peptide control (medium only) or the irrelevant peptide control (VSV-NP43-69, STKVALNDLRAYVYQGIKSGNPSILHI), as shown by ELISPOT assay ( Figures 2A–C ). GPM6B-C94F and TPBG-P57L from P01, OPLAH-G890D, BCAR1-V64L, GBF1-D1478Y and UPF3A-R380Tfrom P02, and ACAD8-T105I, BCAR1-G23V, and PLCG1-M425Lfrom P03manifestedparticularly distinct peptide-specific T-cell responses.

In order to explore the role of NRT in patients with NSCLC.DCs from P03 (HLA-A*02:01⁺) loaded with ACAD8-T105I, BCAR1-G23V and PLCG1-M425L were cocultured with PBLs to generate mutated peptide-specific NRTs in vitro, and the immune responses were compared with the WT peptide-induced NRTs. As shown by ELISPOT assay, the means spots of IFN-γ-producing T cells were significantly greater in NRTs elicited by the aberrant peptides than in those induced by the WT peptides ( Figures 3A, B ).

Mutant peptide-pulsed HLA-A*02:01⁺ T2 cells and minigene-nucleofected H522 cells (HLA-A*02:01⁺, H522-minigene) were used as peptide-specific targets to further examine the cytotoxic effect of the corresponding NRTs. The killing activity of NRTs at different ratios of effective cells to target cells is shown in Figures 3C–E . Bulk NRTs against ACAD8-T105I, BCAR1-G23V and PLCG1-M425L, particularly NRTs against BCAR1-G23V and PLCG1- M425L, exerted significant cytotoxic effects toward target cells expressing corresponding antigens. No significant cytotoxic effect was detected with T2 cells that did not pulse any peptides or pulsed irrelevant peptides (VSV-NP43-69) and H522 cells that did not express any mutant peptides.

To evaluate the immunogenicity of the candidate polypeptides in vivo, the polypeptides ACAD8-T105I, BCAR1-G23V and PLCG1-M425L from P03 (HLA-A*02:01⁺), whose immunogenicity was previously proven in vitro, were selected for the immunization of HLA-A2.1/k^b mice. On days 0 and 7, ACAD8-T105I, BCAR1-G23V and PLCG1-M425L (100 μg per peptide) were mixed with 50 μg of poly (I:C), and the mixture was subcutaneously injected into transgenic mice for immunization. Splenocytes were collected 7 days after the last immunization. Some of the splenocytes were used for IFN-γ, TNF-αand IL-2 ELISPOT assay. The rest of the splenocytes were cultured for another 7 days with the corresponding peptides, and T cells were then isolated for cytotoxicity detection. NRTs against ACAD8-T105I, BCAR1-G23V and PLCG1-M425L from HLA-A2.1/K^b mice contained more IFN-γ, TNF-α and IL-2-producing T cells than those obtained using the WT epitopes, as demonstrated by ELISPOT assay ( Figures 4A–D ). The no-peptide control (culture medium only) and the irrelevant peptide control (VSV-NP43-69) only induced baseline-level secretory responses. In the cytotoxicity assay, the neoantigen-induced NRTs, particularly those induced with BCAR1-G23V and PLCG1-M425L, presented higher cytotoxicity against T2/Kb cells and H522/Kb-minigene cells carrying or expressing the corresponding mutant peptides. No significant cytotoxicity was detected in T2/Kb cells that were not loaded with the peptide or were loaded with irrelevant peptides or H522/Kb cells that did not express mutant peptides ( Figures 4E–G ).