Clonal hematopoiesis (CH) is a phenomenon in which somatic mutations originating from hematopoietic progenitors are detected in peripheral blood cells1,2. The prevalence of CH increases with age, and CH can be detected in 10–25% of healthy, elderly individuals1,2,3,4. Very sensitive methods may allow somatic mutation detection in blood cells in 95% of 50–60-year olds5.
CH confers risk for myeloid malignancy and death1,2. In addition, recent data has suggested that CH is also a risk factor for cardiovascular disease1,6,7. In mice, Tet2 loss-of-function in myeloid cells alone promoted atherosclerosis and proinflammatory cytokine production6. Proinflammatory and dysregulated immune responses play roles in the pathogenesis of multiple diseases. As an example, rheumatoid arthritis (RA) is a chronic autoimmune disease which leads to joint destruction. Despite improved disease outcomes with modern treatments, RA patients have increased risk for death and cardiovascular disease. CH has not been studied in the context of RA previously, except for one study containing self-reported disease history of arthritis3.
Aplastic anemia (AA) and hypoplastic myelodysplastic syndrome (hMDS) are characterized by hypocellular bone marrow and peripheral-blood cytopenias, and are difficult to distinguish8. Although T cells cause hematopoietic stem cell destruction in AA, cytogenetic abnormalities occur in 4–11%, and CH occurs in up to 50% of AA cases8. AA confers a substantial risk for hematological malignancy8.
In this project, we aimed to characterize CH in patients with RA. Results were also compared with the data from patients with AA and hMDS, immune-mediated diseases which have established links with CH. In addition, we hypothesized that CH may modulate chronic inflammation or disease activity in RA. Thus, we compared mutation findings with clinical parameters to investigate associations between CH and the clinical phenotype in RA.
We collected peripheral blood samples from 59 RA patients who fulfilled the ACR2010 classification criteria for RA and had been monitored in the Helsinki University Hospital rheumatology outpatient clinic after RA diagnosis. Twelve acquired AA and hMDS patients were recruited from the Helsinki University Hospital hematology clinic. We also used samples from two young healthy controls (aged 18–22) as negative controls. All patients gave written informed consent. The ethical board of our institution approved the study and the declaration of Helsinki principles were followed. Due to descriptive nature of our study, no power calculations were performed.
To detect CH, we designed a custom sequencing panel based on Illumina’s TruSeq Custom Amplicon technology (Illumina, San Diego, CA, USA). The panel was designed as 250 base-pair amplicons with Illumine Design Studio, and it comprised of 583 amplicons. The panel covered not only genes that are commonly mutated in CH in healthy individuals but also typically in AA patients. Coding exons of 34 tumor suppressor genes and/or mutational hotspots were sequenced (Supplementary table 1; exact genomic coordinates provided as Supplementary Data). Sequencing was performed with the Illumina HiSeq2500 system with 150 paired-end reads, and the average coverage for each amplicon is shown in the Supplementary figure 1. Peripheral-blood DNA (250 ng) was used for sequencing, but for AA/hMDS patients, bone-marrow mononuclear cells (MNC) were used, except for one patient (MDS1, sample type was peripheral blood).
Sequencing data was analyzed by previously described methods9. Briefly, sequencing reads were aligned to the Hg19 genome with Bowtie2 and GATK IndelRealigner, but bases with Phred score < 20 were excluded from further analyses. Variants were required to have sequencing depth > 500, variant base count > 20, and comprise over 80% of all variant bases in the position. Mismapped variants and variants within 5 base-pairs of a 5 base-pair homopolymer were also discarded. Variant with a variant-allele frequency > 35%, population variants with a population frequency of over 1%, and variants that occurred in more than ten individuals were discarded as germline variants. The variants were annotated with the Ensembl Variant Effect Predictor. The Supplementary Material contains more detailed information on variant calling and filtering.
Normal distribution of the data was investigated graphically and with the Shapiro–Wilk test. Statistical tests include two-sided Mann–Whitney test and Fisher’s exact test for comparisons between groups. P-values < 0.05 were considered statistically significant. Longitudinal data was analyzed as In-transformed data with a linear mixed model in SPSS using the unstructured covariance type. Sidak correction was used for paired multiple comparisons in the following analyses. Statistical analyses were performed with Graphpad Prism 6 (Graphpad Software, La Jolla, CA, USA) and SPSS Statistics v.23 (IBM, Armonk, NY, USA).
We discovered CH at 17% prevalence in RA and at 33% in AA/hMDS, which are consistent with previous reports1,2,3,4,8. The identified mutations fulfilled the criteria for clonal hematopoiesis of indeterminate potential (CHIP)10. All synonymous and non-coding mutations were discarded along with mutations with < 2% variant allele frequency (VAF), because we defined CH as a process in which mutations provide survival advantage to cells11. The 2% VAF cutoff has also been suggested to define CHIP10. We did not require missense mutations to occur in cancer gene databases or have deleterious prediction scores by in silico tools, because these strategies will cause underreporting of novel variants and over-reporting of known variants.
In RA patients, DNMT3A mutations were the most common, TET2 mutations ranking second (Figure 1a; Table 1 and Supplementary table 2), consistently with the mutational spectrum found previously in healthy controls1,3,4. None of the DNMT3A mutations occurred in the R882 AML/MDS hotspot that has previously been described in CH1,2,7. Frameshift and nonsense mutations comprised 8/12 of all mutations in RA patients (Fig. 1b), and these disruptive mutations had higher VAFs than missense mutations (Fig. 1c; p = 0.0191). This finding suggests that these mutations give survival advantage to the affected clones.
AA/hMDS patients (Supplementary tables 3–4) were characterized by mutations in genes such as LAMB4, PIGA, and STAG2, which differentiates them from RA patients (Fig. 1a) and healthy controls8. Consistently with RA patients, most AA patients harbored only one CH mutation per patient, but one AA patient harbored two CH mutations (Fig. 1d). Follow-up samples were available from two AA/hMDS patients (AA1 and AA3). One of these patients (AA1) harbored a LAMB4 mutation that occurred in one follow-up sample but disappeared after anti-thymocyte globulin treatment (Supplementary figure 2).
Extremely low VAFs are challenging to detect even with modern sequencing methods. High sequencing coverage is not the only solution to achieve sensitive mutation detection, because sequencing library preparation can induce mutational artifacts, especially C>A transversions, to the library DNA12. With a VAF cutoff at 2%, half of the single-nucleotide changes were C>T mutations (Fig. 1e) in our RA data, supporting the accuracy of mutation calling1,2,3,11.
The prevalence of CH increased with age in RA patients: the overall prevalence of CH was 17% but in 70–79-year olds it increased up to 25% (Fig. 1f). However, patients with CH were not significantly older at sampling (Fig. 1g). Nearly all studied RA patients were treated with anti-rheumatic drugs before sample collection. The patients’ treatment histories included methotrexate in 98%, hydroxychloroquine in 75%, sulfasalazine in 58%, leflunomide in 10%, and biological drugs in 8.5% of cases. No differences in the treatment histories were observed between patients with or without CH (Table 1). Taken together, the signature of CH in RA reflects the ageing hematopoietic system with C>T transitions and mutations in epigenetic regulators11.
As chronic inflammation may cause mutagenesis via DNA damage13, we also aimed to explore if CH is linked with disease severity. In our cohort (n = 59) we could not detect any differences in clinical parameters (such as smoking status, serostatus, disease activity at diagnosis or other autoimmune disease) between RA patients with/without CH (Supplementary figures 3–4; Supplementary tables 5–6). Similarly, during four years of follow-up, no differences emerged in blood cell indices between RA patients with/without CH (neutrophil counts and mean corpuscular volume (MCV) are shown in Fig. 1h, i; Supplementary figure 4; Supplementary tables 7–10). This is in line with previous findings in healthy controls, as CH does not associate with cytopenias in hematologically unselected patients1. However, it should be noted that our dataset may lack statistical power to discover subtle changes.
CH mutations occur mostly in myeloid cells, but mutations in lymphoid cells may also modulate autoimmune responses. We recently discovered CD8+ T cells harboring somatic mutations in immune-related genes in RA patients14. Similarly, AA- and Felty’s syndrome (RA with neutropenia and splenomegaly) patients’ CD8+ T cells harbor somatic mutations9,15. Future research is needed to address the “chicken or the egg” dilemma: does autoimmunity increase mutation formation or do mutations promote inflammation and autoimmunity?
Taken together, CH with a typical mutation profile occurs in RA, but despite of years long systemic inflammation, the rate of CH is not markedly increased. To our knowledge, this is the first report describing the occurrence of CH in RA; one previous study included patients with self-reported disease history but did not find a significant association with self-reported arthritis and CH3. However, this data is preliminary, and conclusive results would require analysis of a larger cohort of patients. In addition, although no associations existed between CH and clinical severity of RA in our data, future studies should assess if a specific mutation or a subset of mutations could impact autoimmunity or treatment responses. This is plausible, as CH shapes immune responses in other disease contexts: it increases the risk for cardiovascular endpoints1,7, and Tet2 deficiency in myeloid cells promotes atherosclerosis and proinflammatory cytokine production in mice6. Thus, understanding the functional consequences of all CH-associated mutations, and their roles in various disease conditions, is warranted in the future.
Availability of data and materials
Due to constraints in the ethical permit, the raw sequencing data of patients is only available from the corresponding author upon reasonable request.
Change history
17 February 2021
A Correction to this paper has been published: https://doi.org/10.1038/s41408-021-00427-1
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Acknowledgements
We would like to acknowledge the personnel at Hematology Research Unit Helsinki for their assistance, and the FIMM Technology Center sequencing unit for their assistance on sequencing and data analysis. This work was supported by the European Research Council (M-IMM project), Academy of Finland, Finnish special governmental subsidy for health sciences, research and training, the Sigrid Juselius Foundation, the Instrumentarium Science foundation, the Finnish Cancer Societies, Finnish Cancer Institute, Biomedicum Helsinki foundation, the Finnish medical foundation, Orion research foundation, Juhani Aho foundation, K. Albin Johansson foundation, and Paulo foundation.
Authors contributions
P.S., S.L., M.A.I.K., P.E., T.K. and S.M. designed the study and experiments. P.S., M.A.I.K. and M.L.-R. recruited the patients. P.S., T.K., S.L. and M.A.I.K. collected the samples. P.S., S.L., P.E. and H.A. analyzed the data. P.S. and S.M. wrote the manuscript. All authors contributed to writing and approved the manuscript.
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S.M. has received honoraria and research funding from Novartis, Pfizer, and Bristol-Myers Squibb (not related to this study). The remaining authors declare no competing interests.
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Savola, P., Lundgren, S., Keränen, M.A.I. et al. Clonal hematopoiesis in patients with rheumatoid arthritis. Blood Cancer Journal 8, 69 (2018). https://doi.org/10.1038/s41408-018-0107-2
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DOI: https://doi.org/10.1038/s41408-018-0107-2
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