This study included 35 dogs referred to the Veterinary Medical Center of the University of Tokyo (VMC-UT) and diagnosed with LCGIL. All of the dogs originated from Japan. The diagnosis of large cell lymphoma was made based on histopathological examinations using endoscopically or surgically obtained tissues or cytological examinations using samples obtained by fine-needle aspiration. PCR for antigen receptor gene rearrangements (PARR) was conducted using a part of DNA derived from tumors as previously described to evaluate clonal rearrangements of the T-cell receptor γ (TCRγ) and the immunoglobulin heavy chain (IgH) genes in all cases (14). Peripheral blood-derived gDNAs (genomic DNA) were available in 21 of the 35 cases and analyzed as normal controls. The signalment and sample information of each case are shown in Supplementary Table S1.

WES analysis was conducted using 4 dogs diagnosed with LCGIL (Dog 1–4). gDNAs (500 ng) obtained from the tumor site sample were mechanically sheared to fragments of approximately 150 bp (Covaris S220, Woburn, MA, USA). Fragment sizes were verified for quality control using Agilent 2,100 Bioanalyzer (Agilent, Santa Clara, CA, USA). SureSelect XT Canine All Exon V2 kit (Agilent, Santa Clara, CA, USA) and AMPure XP beads (Beckman Coulter, CA, USA) were used to prepare libraries for sequence analysis. The library was sequenced using a paired-end 2 × 100 bp read protocol on the NextSeq500 instrument (Illumina, San Diego, CA, USA). Signal captures were converted into FASTQ files using bcl2fastq (v2.18.0.12) and trimmed with trimgalore (v0.6.5) and Cutadapt (v1.15). The alignment of processed reads to a canine reference genome (CanFam 3.1, GenBank assembly accession: GCA_000002285.2), local realignment, and variants calling in each sample were performed using DRAGEN software (v 07.021.572.3.6.3) (Illumina, San Diego, CA, USA) with the standard protocol, and mutations were annotated using SnpEff (v5.0). The information on canine genetic variation, single nucleotide polymorphisms, and insertions and deletions was available from the Ensembl variation database (CanFam3.1, dog release 101). Somatic mutations were called using VarScan2. Somatic mutations whose variant allele frequencies >0.2 and somatic p value <0.05 were regarded as somatic mutations. Extracted mutations in WES were filtered by the following criteria: (1) mutations that were categorized into HIGH and MODERATE by SnpEff, (2) mutations with total read depths of more than 15 and variant read depths of more than 5 in the tumor genome, (3) mutations with total read depths of more than 15 and variant allele frequency of less than 0.03 in the peripheral blood genome. Datasets obtained through WES analyses are available at the DDBJ Sequenced Read Archive repository with accession number PRJDB15563.

The mutations that were extracted based on the results of WES were validated by targeted NGS with the samples used for WES and additional samples from 31 dogs with LCGIL (Dog 5–35, Supplementary Table S1) as a previous study (15). The sequencing libraries for targeted NGS were prepared from each gDNA sample by two-step multiplex PCR; 1st PCR to amplify the target regions using Platinum™ Multiplex PCR Master Mix (Applied Biosystem, CA, USA), and 2nd PCR to add index sequences, which were used to identify individuals, and sequences that were used to bind the flow cell using KOD One PCR Master Mix (TOYOBO, Osaka, Japan). The library was purified using AMPure XP beads (Beckman Coulter, CA, USA). After assessing the quantity and quality using Bioanalyzer (Agilent, Santa Clara, CA, USA) and KAPA Library Quantification Kit (Nippon Genetics, Tokyo, Japan), the library was sequenced on the MiSeq instrument (Illumina, San Diego, CA, USA). FASTQ files were trimmed with Cutadapt (v2.10). The processed reads were mapped to CanFam 3.1 using BWA (v0.7.17) and sorted using Samtools (v1.10). Variants calling in each sample were performed using the Mutect2 tool in GATK (v4.2.6.1). Primer sequences used for targeted NGS are shown in Supplementary Table S2. Variants were evaluated as mutations if the variant allele frequencies were more than 0.1.

In addition, we investigated the mutations of the ZDBF2 gene throughout the whole coding region by targeted NGS analysis that covered all exons using the samples from 31 LCGIL dogs (Dog 5–35). Targeted NGS analysis was performed according to the same method described above using ROS_Cfam_1.0 as a reference genome. Primer sequences are shown in Supplementary Table S3. Variants were evaluated as mutations by the following criteria: (1) mutations with the variant allele frequencies of more than 0.1 and the total read depths of more than 100 in the tumor sample, (2) mutations with the variant allele frequency of less than 0.1 and the total read depths of more than 100 in all peripheral blood samples.

Among 35 lymphoma samples included in this study, 22 samples were collected by endoscopic biopsy, 9 samples by fine-needle aspiration, and 4 samples by surgical resection. The median age of the cases was 11.1 (range: 3.9–13.6) years old. There were 19 males (12 were castrated) and 16 females (15 were spayed). The breeds of these dogs were Miniature Dachshunds (n = 8), Chihuahuas (n = 4), Toy Poodles (n = 4), Shibas (n = 4), Pomeranians (n = 2), Pugs (n = 2), Jack Russell Terriers (n = 2), French Bulldog (n = 2), and 1 each of English Cocker Spaniel, Miniature Schnauzer, Beagle, Norfolk Terrier, Pekingese, Papillon and mixed breed. By PARR analysis, clonal rearrangements of the TCRγ gene were shown in tumor samples of 24 dogs, the IgH gene in those from 2 dogs, and neither in those from 8 dogs. Amplification of the two control genes was verified to assess DNA quality for these 34 samples. In one dog (Dog 28), PARR could not be performed because of insufficient DNA quantity. Clinical information of the 35 dogs including age, sex, breed, and immunophenotype of tumor cells determined by PARR were shown in Supplementary Table S1.

The samples of four dogs (Dogs 1–4) were subjected to WES analysis. Tumor samples were obtained by endoscopic biopsy in three dogs (Dogs 1–3) and by surgical resection in one dog (Dog 4). The lesions of all dogs were localized to the intestinal wall and adjacent lymph nodes. In WES, the mapping rate was more than 99% in each sample, and the average depths were 165× in tumors and 170× in peripheral blood. By comparison with the peripheral blood genome, 1910–4602 somatic mutations were called in each case (Supplementary Table S4). Among these called mutations, 9 mutations in Dog 1, 14 in Dog 2, 2 in Dog 3, and 147 in Dog 4 were extracted based on the filtering criteria described above (Table 1). The mutations in TTBK1 and NACC1 genes were commonly found in Dogs 1, 3, and 4, and Dogs 1 and 4, respectively (Table 2). The same mutation in TTBK1 gene was observed in Dog 3 and 4. However, since the TTBK1 mutation in Dogs 1, 3, and 4 was found to be located in the non-protein-coding region when verified on the CanFam3.1 database, the TTBK1 was excluded from the following analysis. We also extracted the mutations in genes where mutations were commonly identified in human intestinal T-cell lymphoma, and we found the mutations in ASXL3, SOCS3, PRDM1, FYN, TET2, and ZDBF2 genes in Dog 4 (Table 3) (9–11, 16, 17).

We decided to validate the 8 mutations in 7 genes that were extracted based on the results of WES. The NACC1 mutation (c.204dupC), which was found in Dog 1 in WES analysis, could not be analyzed due to GC-rich sequences. Among the remaining 7 gene mutations observed in Dog 4 by WES analysis, those in NACC1, ASXL3, SOCS3, PRDM1, FYN, and TET2 genes were not found in any of the 31 additional cases by targeted NGS analysis. As for the mutation in ZDBF2 gene, the variant allele frequency was more than 0.15 in all tumor samples. Particularly high variant allele frequency was identified in tumor samples of the two dogs: 0.484 in Dog 4 and 0.394 in Dog 30. However, the same mutation was ubiquitously observed in all 17 peripheral blood samples with variant allele frequency ranging from 0.18 to 0.27.

Also, targeted NGS analysis that covered all exons revealed other point mutations in ZDBF2 gene than that detected by WES: a missense mutation (c.485G > A) in Dog 17, two missense mutations (c.5339G > T, c.6731C > T) in Dog 33, and two missense mutations (c.5339G > T, c.7016C > T) in Dog 34 (Table 4).