Figures
Abstract
Background
Psoriasis (PsO) is a chronic inflammatory disease with predominantly cutaneous manifestations. Approximately one third of patients with PsO develop psoriatic arthritis (PsA), whereas the remaining proportion of patients has isolated cutaneous psoriasis (PsC). These two phenotypes share common immunology, but with different heredity that might in part be explained by genetic variables.
Methods
Using a candidate gene approach, we studied 53 single nucleotide polymorphisms (SNPs) in 37 genes that regulate inflammation. In total, we assessed 480 patients with PsO from DERMBIO, of whom 151 had PsC for 10 years or more (PsC10), 459 patients with PsA from DANBIO, and 795 healthy controls. Using logistic regression analysis, crude and adjusted for age and gender, we assessed associations between genetic variants and PsO, PsC10, and PsA, as well as associations between genetic variants and development of PsA in PsO.
Results
Eleven polymorphisms in 10 genes were nominally associated with PsO and/or PsC and/or PsA (P < 0.05). After correction for multiple testing with a false discovery rate of 5%, two SNPs remained significant: TNF (rs361525) was associated with PsO, PsC10, and PsA; and IL12B (rs6887695) was associated with PsO.
Citation: Loft ND, Skov L, Rasmussen MK, Gniadecki R, Dam TN, Brandslund I, et al. (2018) Genetic polymorphisms associated with psoriasis and development of psoriatic arthritis in patients with psoriasis. PLoS ONE 13(2): e0192010. https://doi.org/10.1371/journal.pone.0192010
Editor: Giuseppe Novelli, Universita degli Studi di Roma Tor Vergata, ITALY
Received: October 25, 2017; Accepted: January 14, 2018; Published: February 1, 2018
Copyright: © 2018 Loft et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Data Availability: All relevant data are within the paper and its Supporting Information files.
Funding: The work was funded by Psoriasisforeningen, Robert Wehnerts og Kirsten Wehnerts Fonden, Knud og Edith Eriksens Mindefond, Gigtforeningen (A2037, A3570), DERMBIO, and the Novo Nordisk Foundation (NNF15OC0017622). The Novo Nordisk Foundation provided support in form of a scholarship for author NDL, but did not have any role in the study design, data collection and analysis, decision to publish, or preparation of the manuscript. The rest of the Funders supported the study with funding for collection and analysis of biological material. MKA is employed by Zitelap Aps. Zitelap Aps provided support in the form of salary for author MKA and is responsible for management of the DERMBIO and DANBIO databases, but did not have any additional role in the study design, data collection and analysis, decision to publish, or preparation of the manuscript. The specific role of this author is articulated in the ‘author contributions’ section.
Competing interests: Dr. Skov has received consultancy and/or speaker honoraria from Abbvie, Pfizer, Janssen-Cilag, Merck Sharp & Dohme (MSD), and LEO Pharma and is a member of the advisory boards of Abbvie, Pfizer, Janssen-Cilag, MSD, Eli Lilly, Celgene, and Novartis. Dr. Rasmussen has been a paid speaker for Pfizer, AbbVie, Eli Lilly, and LEO Pharma. He has been consulting or serving on expert/advisory boards with Abbvie, Janssen-Cilag, Novartis, and Eli Lilly. He has served as investigator for Eli Lilly. Dr. Gniadecki has received consultancy and speaker honoraria from Abbvie, Janssen-Cilag, and Novartis and is a member of the advisory boards of Abbvie, Amgen, Janssen-Cilag, Eli Lilly, Celgen, Novartis, and Therakos. Dr. Dam has received compensation as a speaker and member of an advisory board for Janssen-Cilag and Abbvie. Dr. Vibeke Andersen has received compensation as a consultant and member of an advisory board for MSD and Janssen-Cilag. Dr. Glintborg has received research grants from Biogen and Abbvie. Dr. Hetland is a member of the advisory board of Celltrion and has received compensation as a speaker for Roche, Pfizer, and Biogen. MKA is employed by Zitelap Aps, which is responsible for management of the DERMBIO and DANBIO databases. This does not alter our adherence to PLOS ONE policies on sharing data and materials.
Introduction
Psoriasis (PsO) is a chronic inflammatory disease that affects approximately 2–4% of the western world’s population [1]. Approximately one third of patients with PsO develop psoriatic arthritis (PsA) [2], while the remaining patients have isolated cutaneous psoriasis (PsC). PsA and PsC share common immunology, in which the interleukin (IL)-23/IL-17 axis plays a critical pathogenic role [3]. Other important cytokines include tumor necrosis factor alpha (TNF-α), interleukin (IL)-12, IL-22, and interferon gamma (IFN-γ) [4, 5], with NFκB being a crucial mediator in the pathogenesis [6].
Epidemiological studies suggest stronger heritability for PsA than for PsC (9) which indicates that there could be individual risk loci for these two disease entities. Identification of such loci could potentially serve as novel drug targets and possibly improve patient outcomes by facilitating earlier detection of PsA, thereby possibly preventing irreversible joint destruction [7–9]. Indeed genetic differences related to the human leukocyte antigen (HLA) class I region of the major histocompatibility complex (MHC) have been well established. Variants of HLA-B, namely HLA-B*27, have been proven to confer risk of PsA [10], while HLA-C*06 has been demonstrated to hold a specific risk for PsC [10–14].
Only a limited number of studies have evaluated genetic loci specifically associated with PsA, PsC and the differences between PsA and PsC. To date only 15 polymorphisms in twelve genes outside the MHC region have been reported to render differences in susceptibility between the two phenotypes, including IL23R (rs2201841, rs12044149) [11, 12, 15], FBXL19 (rs10782001) [16], IL12B (rs2082412) [11, 17], ZNF816A (rs9304742) [17], CCR2 (rs1799864) [18], CSF2 (rs715285) [19], PTPN22 (rs2476601) [12, 20], IL13 (rs1800925, rs20541, rs848) [21–23], TNFRSF9 (rs4908742) [12], LCE3A (rs10888503) [12], TNFAIP3 (rs9321623) [12], and KIR2DS2 [24]. Among these, only associations to PTPN22 (rs2476601) [12, 20], IL23R (rs2201841, rs12044149) [11, 12, 15], IL12B (rs2082412) [11, 17], and IL13 (rs1800925, rs20541, rs848) [21–23] have been replicated, while a large scale genome wide association study (GWAS) failed to reproduce the associations for the polymorphisms in IL13 and IL12B [12].
In order to potentially add to the number of loci outside of the HLA region that confer risk specific to PsA and PsC, this study examined functional single nucleotide polymorphisms (SNPs) in genes involved in regulation of the NFκB pathway (CD14, LY96, MAP3K14, NFKB1, NFKBIA, SUMO4, TIRAP, TLR1, TLR2, TLR4, TLR5, and TLR9), cytokines regulated by NFκB (IL1B, IL1RN, IL6, and IL10), TNF-α signaling (TNFA, TNFAIP3, and TNFRSF1A), IFN-γ signaling (IFNG, IFNGR1, IFNGR2, JAK2, and TBX21), the IL-23/IL-17 axis (IL12B, IL12RB1, IL17A, and IL23R), and other genes involved in regulation of inflammation (CARD8, IL4R, IL6R, IL18, NLRP1, NLRP3, PPARG, PTPN22, and TGFB1). These were assessed for association with PsO, PsC, and PsA and compared to the general population, and furthermore they were examined for association with development of PsA in PsO.
Materials and methods
Cohort
As described by Loft et al. a Danish cohort comprising 480 patients, registered in the national database DERMBIO, diagnosed with PsO was established [25]. Among these patients, 147 had an additional diagnosis of PsA recorded in DERMBIO [25]. Patients registered in DERMBIO have all received biological therapy in a dermatological setting, thus all patients had moderate-to-severe involvement of skin. We identified a subgroup of 151 patients with PsC who had been retrospectively followed for ≥10 years prior to initiation of biological treatment (PsC10) and who did not have an additional PsA diagnosis in DERMBIO. This group represented a group of patients with isolated cutaneous psoriasis who were unlikely to develop PsA, as the majority of patients with PsO, who develop PsA do so within the first 10 years after diagnosis [26].
Additionally, a PsA cohort was established. This included 459 patients diagnosed with PsA according to their treating rheumatologist in DANBIO, an independent Danish nationwide quality registry for patients treated in a rheumatology setting with disease modifying anti rheumatic drugs (DMARDs) including biological (b)DMARDs [27]. There was no overlap of included patients in DERMBIO and DANBIO.
Patients were identified by linking the unique personal identification number of Danish citizens (CPR number) from blood clot samples, sent for Mycobacterium tuberculosis (TB) screening, with DANBIO and DERMBIO. Screening for TB before the initiation of biological therapy is a routine element of care in Denmark. Blood clot samples were obtained from: the Department of Biochemistry, Hospital of Lillebaelt (Vejle, Denmark); the Department of Biochemistry, Hospital of Slagelse (Slagelse, Denmark); the Department of Clinical Biochemistry, Herlev and Gentofte Hospital (Hellerup, Denmark); the Department of Respiratory Diseases B and the Department of Clinical Microbiology, Aarhus University Hospital (Aarhus, Denmark); and Statens Serum Institut (Copenhagen, Denmark) from September 2009 through July 2015, as described earlier [25, 28–31]. A previously described group of 795 healthy blood donors recruited from Viborg, Denmark was used as control group [32].
Ethical considerations
The study was conducted in accordance with the Declaration of Helsinki and was approved by Regional Ethics Committees of Southern (S-20120113) and Central (M-20100153) Denmark and the Danish Data Protection Agency of Southern (RSD: 2008-58-035) and Central (RM: J. 2010-41-4719) Denmark. The Ethics Committees gave exemption from obtaining written informed consent, because information had no health-related impact.
Genotyping
For the patients, DNA was extracted from cryopreserved blood clots by using the Maxwell 16 Blood purification kit (Promega, Madison, Wisconsin, USA), as described by Bank et al. [33]. DNA from the healthy controls was extracted according to the manufacturers’ instructions from EDTA-stabilized peripheral blood using either a either PureGene (Qiagen, Hilden, Germany) or Wizard Genomic (Promega, Madison, Wisconsin, USA) DNA purification kit [32].
A candidate gene approach was chosen, with focus on genes involved in the NFκB pathway, TNF-α signaling, the IFN-γ pathway, and the IL-23/IL-17 axis, as described earlier [28–30]. In addition, other genes involved in regulation of inflammation including the inflammasome were assessed [34]. In short, relevant genes were identified by searching pathway databases (http://www.genome.jp/kegg/pathway.html and http://www.wikipathways.org/index.php/WikiPathways) and SNP candidates were identified by searching PubMed with “polymorphism AND Gene name AND (reporter gene OR luciferase OR ELISA OR RT-PCR OR flow cytometry OR EMSA)”. The SNPs were selected based on the reported functionality or associated with autoimmune diseases (S1 Table). Additionally, SNPs or genes associated with response to biological treatment of either inflammatory bowel diseases or rheumatoid arthritis were included [28–30].
The polymorphisms were genotyped with Competitive Allele-Specific Polymerase chain reaction (KASP™) by LGC Genomics (LGC Genomics, Hoddesdon, United Kingdom) (http://www.lgcgenomics.com/). Genotype distributions for healthy controls and phenotypes are presented in S2 Table.
Linking disequilibrium (LD) was calculated using SNP Annotation and Proxy Search (SNAP) software (http://archive.broadinstitute.org/mpg/snap/) using as reference the Central Europeans in the 1,000 Genomes [35].
As a quality control, all SNPs were replicated for 94 randomly selected samples, yielding >99% identical genotypes.
Power analysis
At the 5% significance level, and a minor allele frequencies (MAF) of 0.05, 0.25, and 0.45 there is > 80% power for detecting a dominant effect with an odds ratio (OR) of 1.7, 1.4, and 1.5, respectively, for PsO, an OR of 2.0, 1.7, and 1.9, respectively, for PsC10, an OR of 1.7, 1.4, and 1.5, respectively, for PsA, and for PsA in patients diagnosed with PsO an OR of 1.8, 1.5, and 1.6, respectively (Table 1). The Genetic Power Calculator [36] was used for power calculations, setting ‘prevalence’ of PsO to 2%, of PsC10 to 1.4%, of PsA to 0.6%, and of PsA in PsO to 30%, D-prime to 1, type 1 error rate to 0.05, and number of cases and control:case ratio was based on data described in Table 2.
Statistical analysis
Assuming a dominant model, we compared genotype distributions for the following groups: patients with PsO and PsC10 from DERMBIO compared with healthy controls using logistic regression analysis; patients with PsA from DANBIO compared with healthy controls; patients with PsA from DANBIO compared to patients with PsC10 from DERMBIO. Odds ratios unadjusted and adjusted for age and gender are reported (S3 and S4 Tables). Correction for multiple testing by controlling the false discovery rate (FDR) at 5% was performed [37]. Additional computation of FDR-adjusted p-values (q-values) based on all P-values presented in S3 and S4 Tables were performed. Q-values describe the estimated proportion of false positives among associations equal to, or more extreme than, the observed association.
Chi-square test was used to test deviations from Hardy-Weinberg equilibrium among healthy controls. Statistical analyses were performed using Stata version 14 (StataCorp LP, College Station, TX, USA).
Results
Study population
The characteristics of patients and healthy controls are shown in Table 2. The genotype distributions among healthy controls deviated from Hardy-Weinberg equilibrium for TGF-B1 (rs1800469) (P = 0.016), TLR1 (rs4833095) (P = 0.028), TLR2 (rs4696480) (P = 0.018), and TLR4 (rs1554973) (P = 0.032). After correction for multiple testing, none of the deviations remained statistically significant.
Polymorphisms associated with the risk of PsO in the general population
The association of SNPs in patients with PsO was compared with healthy controls using a dominant model for association. Nine SNPs were nominally associated with PsO (P < 0.05) (S3 Table). Two SNPs [TNF (rs361525) and IL12B (rs6887695)] withstood correction for multiple testing (Table 3).
Polymorphisms associated with the risk of PsC10 in the general population
Patients were stratified for phenotype and diseased duration, and the genotype distributions of patients with PsC10 were compared with healthy controls. Five SNPs were nominally associated with PsC10 (S3 Table), among which one SNP [TNF (rs361525)] withstood correction for multiple testing (Table 3).
Polymorphisms associated with the risk of PsA in the general population
Genotype distributions for patients with PsA from DANBIO were compared with those from healthy controls using a dominant model for association. Two SNPs were nominally associated with PsA (S3 Table), with one withstanding correction for multiple testing (Table 3).
Polymorphisms associated with the risk of PsA in patients with PsO
Genotype distributions for patients with PsA from DANBIO were compared with patients with PsC10. Only TNF (rs361525) (OR: 0.59, 95% CI: 0.38–0.92, P = 0.019, q = 0.32) showed nominally evidence of association, but this did not withstand correction for multiple testing (S3 Table).
Discussion
This study evaluated 53 SNPs in 37 genes in 480 Danish patients with moderate-to-severe PsO and in 459 patients with PsA. The polymorphisms were primarily chosen as functional polymorphisms targeting the inflammatory signaling pathways. Eleven polymorphisms in 10 genes were nominally associated with PsO and/or PsC and/or PsA (P < 0.05), among which two withstood correction for multiple testing.
The variant alleles in IL12B (rs6887695) [38–45], IL23R (rs11209026) [39–42, 46, 47], and TNF (rs361525) [48–52] are all well-known polymorphism associated with susceptibility to PsO. We found that the variant allele of IL23R (rs11209026) was nominally associated with decreased risk of PsO, but this did not withstand correction for multiple testing.
In the current study, the variant allele of TNF (rs361525) was the only variant consistently associated with an increased risk of all phenotypes, thus underlining the importance of TNF-α signaling in the development of psoriasis. Conflicting results for the association of TNF (rs361525) and development of PsA in PsO have previously been reported. While some studies have reported a protective role for the variant allele of TNF (rs361525) in development of PsA in PsO [53, 54], other studies have reported increased or no altered risk for development of PsA in PsO [55, 56]. In the current study, the variant allele of TNF (rs361525) was associated with an increased risk of PsA and nominally associated with a decreased risk of developing PsA in PsO. The strong association between PsO and TNF (rs361525), and the increased risk of PsC compared to PsA have been suggested to be due to a high LD between TNF (rs361525) and HLA-CW*6 [54].
Another SNP investigated, IL12B (rs3212217), is in close LD with two other polymorphisms: IL12B (rs3212227, r2 = 0.95) [38–45, 57] and IL12B (rs2082412, r2 = 0.95) [11, 17], both associated with reduced risk of PsO. Differences in effect size between PsC and PsA for IL12B (rs2082412) have been reported [11, 17] although the associations could not be replicated by a large GWAS that attempted to confirm previously reported associations [12]. In the current study, no statistically significant difference in effect size between PsA and PsC10 for IL12B (rs3212217) was observed. Thus the current study adds to the evidence that suggest that there is no difference in PsA and PsC10 susceptibility for the variants in IL12B.
In a previous study, the variant allele of PPARG (rs1801282) was associated with decreased risk of PsA [58]. Another study demonstrated the same trend, although the findings were not statistically significant [59]. In the current study, the variant allele of PPARG (rs1801282) was nominally associated with decreased risk of PsA, with odds ratios similar to those previously reported, but the association was not statistically significant after correction for multiple testing. In accordance with previous studies [60], we observed no association between PPARG (rs1801282) and uncomplicated psoriasis, PsO or PsC10. Additional studies investigating association of PPARG (rs1801282) with PsA should be performed in order to clarify the role of PPARG (rs1801282) in PsA. PPARG (rs1801282) encodes a Pro to Ala amino acid substitution in PPARG that leads to reduced activity. PPARG (rs1801282) is a variant of notable interest that has, in addition to PsA, been associated with a lower risk of alcohol-related breast cancer [61, 62], but an increased risk of alcohol-related colorectal cancer [63] likely because PPARG inhibits sex hormone synthesis via negative regulation of aromatase [62].
We failed to replicate PTPN22 (rs2476601) as a risk factor of PsA in PsO, probably due to lack of power, since we observed odds ratios similar to those previous reported [12, 20].
The main limitation in this and other studies evaluating risk of PsA in PsO is the potential for phenotype misclassification, which inevitably will lead to a decrease in statistical power. In this study, data on PsA, for the DERMBIO cohort, were retrieved from the DERMBIO database, with patient registration performed by dermatologists. Although dermatologist are experienced and trained in assessing PsA, we cannot rule out the possibility that some patients with PsC may have had undiagnosed or undeveloped PsA. This might bias the effect size towards the null hypothesis of no difference. In order to overcome the possibility of undeveloped PsA and reduce the risk of undiagnosed PsA, a cohort of patients with PsC who had the disease for ≥10 years (PsC10) was established, as proposed by Stuart et al [12]. Similarly, there is risk of potential misclassification in the PsA cohort (e.g. rheumatoid arthritis or osteoarthritis). However, this risk was lowered by only including patients registered in DANBIO, where diagnoses are according to the treating rheumatologist.
In conclusion, this study confirms that two SNPs in the IL12B and TNF genes are associated with susceptibility to psoriasis in Danish patients with moderate-to-severe psoriasis. None of the investigated SNPs were specifically associated with isolated cutaneous psoriasis or psoriatic arthritis.
Supporting information
S1 Table. The chosen polymorphisms and corresponding gene.
https://doi.org/10.1371/journal.pone.0192010.s001
(DOCX)
S2 Table. Genotype distributions for patients with psoriasis, psoriatic arthritis, isolated cutaneous psoriasis for a minimum of 10 years, and healthy controls.
https://doi.org/10.1371/journal.pone.0192010.s002
(DOCX)
S3 Table. Odds ratios (OR) for genotypes studied among healthy controls and patients with psoriasis (PsO), isolated cutaneous psoriasis (PsC10) and psoriatic arthritis (PsA) and comparison of PsA with PsC10, unadjusted.
https://doi.org/10.1371/journal.pone.0192010.s003
(DOCX)
S4 Table. Odds ratios (OR) for genotypes studied among healthy controls and patients with psoriasis (PsO), isolated cutaneous psoriasis (PsC10) and psoriatic arthritis (PsA) and comparison of PsA with PsC10 adjusted for age and gender.
https://doi.org/10.1371/journal.pone.0192010.s004
(DOCX)
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