Abstract
Objective
The aims of the present study were to typify the human leukocyte antigen system (HLA)-A, B (class I) and HLA-DR, DQ (class II) antigens and to assess the frequency of the presence of these antigens in the Turkish population with recurrent aphthous ulceration (RAU) and Behçet's disease (BD) compared to healthy subjects.
Subjects and Methods
Thirty patients with RAU, 30 with BD, and 15 healthy subjects were included in the study. HLA typing was performed by serology with commercial kits for HLA class I and II (One Lambda, Canoga Park, Calif., USA).
Results
The HLA-A23 frequency was 26.7% in the RAU patients, which was significantly higher than the 3.3% frequency in the patients with BD (p < 0.05). The HLA-A24 frequency was 33.3% in the RAU patient group, which was significantly higher (p < 0.05) than the frequency in the healthy subjects (6.7%). Significantly higher frequencies (46.7%) of HLA-A30 were found in the healthy subjects compared to the BD (13.3%) and RAU (3.3%) patients (p < 0.05 and p < 0.01, respectively). A higher frequency of HLA-B13 was observed in the RAU (23.3%) patients compared to the BD (0%) patients (p < 0.01). A decrease was observed in HLA-DR10 and HLA-DR17 in the RAU patients (p < 0.05), while a higher frequency of HLA-DR10 was observed in the BD patients compared to the RAU patients (p < 0.01).
Conclusions
These results showed that RAU and BD were not in the same spectrum and the involvement of other genetic and/or environmental factors might be responsible for the development of these diseases and/or disease progression.
Key Words: Recurrent aphthous ulceration, Behçet's disease, HLA class I, HLA class II, Antigen
Introduction
Recurrent aphthous ulceration (RAU), also known as aphthous stomatitis or canker sores, is the most common inflammatory disease of oral mucosa in children and adults, affecting an estimated 20-25% of the world's population [1,2,3,4]. The disorder is characterized by the appearance of painful and recurrent, single or multiple ulcerations that preferentially affect the nonkeratinized oral mucosa [4,5]. Although RAU is global in distribution, it remains one of the least understood diseases of the oral cavity. Patients with RAU tend to be otherwise healthy, so that even in those with severe disease, the process is generally limited to the oral mucosa [1]. Important considerations regarding the differential diagnosis include complex aphthous stomatitis and variants related to systemic diseases, such as those associated with hematologic, hormonal, nutritional and gastrointestinal alterations [4]. In view of these factors, the clinician needs a detailed history of the patient and a clinical examination is necessary in order to diagnose the clinical conditions that involve RAU and other systems, such as Behçet's disease (BD) [4,5].
BD is a multisystem inflammatory disease with a wide variety of manifestations, including oral and genital ulcers, skin lesions, ocular inflammation, arthritis, cardiovascular disease, and involvement of the central nervous system [6]. In BD, the majority of patients experience RAU as the most common major symptom, and it is often the initial feature. However, it is impossible to predict if a patient with RAU will develop BD, and there is no reliable test to exclude BD. Therefore, RAU in BD presents a diagnostic problem. The etiology and pathogenesis of BD are still uncertain; the onset of BD is believed to be triggered by the involvement of some external environmental factors in individuals with a particular genetic makeup [7]. A strong association of BD with HLA-B51 (one of the split antigens of HLA-B5) has been confirmed in many different ethnic groups from the Middle East to the Far East, and about 40-80% of patients with BD in these populations possess HLA-B5 (B51) [7]. Ohno et al. [8] hypothesized that genes susceptible to BD closely linked to HLA-B51 might have been spread by the old nomadic or Turkish tribes via the ancient Silk Route. The association of major histocompability complex class II antigens with BD has also been studied in different groups, but the results vary [9,10,11,12,13]. Only a few studies on the association of human leukocyte antigen system (HLA) class II antigens with the mucocutaneous type of BD have been reported [14,15].
Chung et al. [16] showed that the phenotype frequency of HLA-DRw8 antigen in 16 Chinese patients with the mucocutaneous type of BD is significantly higher than that in patients with RAU. Jaber et al. [17] observed that there is a close association between HLA-B52 and HLA-B44 in Israeli Arab youths with RAU but long-term follow-up is needed to determine the relationship between RAU and BD. Özbakir et al. [18] found a significantly higher frequency of HLA-DR4 antigen in patients with RAU than in patients with BD. In the present study, HLA-A, B (class I) and HLA-DR, DQ (class II) antigens were analyzed in a group of 30 Turkish RAU and 30 Turkish BD patients.
Subjects and Methods
Selection of the Study Group
Thirty patients (12 men and 18 women) with RAU, another 30 patients (15 men and 15 women) with BD, and 15 healthy subjects (9 men and 6 women) participated in the study. The diagnosis of RAU was made according to the criteria of Lehner [19], and all were diagnosed with minor or major RAU in the Department of Oral Diagnosis and Radiology, Faculty of Dentistry, Marmara University. The RAU patients had aphthous ulcerations that recurred at least once in 2 months during a 1-year period prior to this study. Subjects with herpetiform ulceration or those in whom the diagnosis was not clear were excluded from the study. Thirty patients with BD who fulfilled the International Study Group criteria were selected from the Rheumatology Out-Patient Clinic by an expert rheumatologist (Melek Özer) [20]. For the patients with RAU and BD, the duration of aphthous ulcers was recorded. Fifteen healthy subjects comprising faculty personnel participated after having given informed consent. All healthy subjects were questioned about the absence of recurrent oral aphthous ulcers or other BD-related manifestations or a family history of BD. Similarly, the RAU and BD patients were requested to sign a written informed consent. The study was carried out according to the recommendations of the Helsinki Declaration. The study protocol was approved by the Local Committee of Research and Ethics of Marmara University. All patients and healthy subjects were of Turkish origin and not related to one another.
Analysis of HLA Typing
For HLA, serology typing was performed using commercial kits for HLA class I and II (One Lambda, Canoga Park, Calif., USA). For HLA-A, B (major histocompability complex I) and HLA-DR, DQ (major histocompability complex II) Terasaki HLA tissue typing trays were used.
Mononuclear cells were obtained from whole blood samples drawn into heparin tubes by density centrifugation with Lympho-Kwik® Isolation Reagents (One Lambda). T and B lymphocytes were separated using EasySep® Cell Isolation System (Stem Cell Technologies, Canada). Isolated cells were pipetted into 96-well plates. Before seeding, the cells’ viability was controlled by staining with trypan blue solution (Sigma, USA) and counting viable cells under light microscopy (Leica, Germany). Cells that had more than 90% viability were processed. The cell concentration was adjusted to 2 × 106 cells/ml. Cells were incubated in the presence of a complement binding antibody (One Lambda). After this incubation period, the complement was added into the wells. FluoroQuench™ (One Lambda) was used to stain and fix lymphocytes in the microcytotoxicity assay since a quenching reagent can significantly reduce background fluorescence. Ethylenediaminetetraacetic acid was used to stop complement-dependent cell lysis. Ethidium bromide was used to stain dead cells while acridine orange was used to stain live cells. Live lymphocytes (nonreactive) stained green, while for positive reactions lymphocytes stained orange/red. For each patient sample, amounts of live and dead cells were evaluated with a fluorescence microscope (Olympus, Japan). Each plate was evaluated by two independent observers (G.Y.D., Mustafa Aslan).
Statistical Analysis
The data were analyzed with NCSS (Number Cruncher Statistical System) 2007 and PASS 2008 Statistical Software (Kaysville, Utah, USA). The age, gender, clinical characteristics, and HLA typing between patients with BD or RAU and controls were analyzed by means of the χ2 test. p values <0.05 were interpreted as significant, and the level of confidence intervals was 95%.
Results
The mean age of the patients with RAU was 37.03 ±13.8 years (range 17-64) while that of those with BD was 38.06 ± 8.55 years (range 15-54) and that of the healthy control subjects was 30.26 ± 8.98 years (range 23-51). The differences were not statistically significant.
Frequencies of HLA-A, B (class I) and HLA-DR, DQ (class II) are shown in table 1. The HLA-A23 antigen frequency was 26.7% in the RAU patient group compared to the 3.3% in the BD patients (p = 0.05). The HLA-A24 antigen frequency was 33.3% in the RAU patient group compared to the 6.7% in the healthy subjects (p < 0.05). A significantly higher frequency of HLA-A30 was found in the healthy subjects compared to the RAU patients (p < 0.01). A higher frequency of HLA-B13 was observed in the RAU patients (0%) compared to the BD patients (23.3%; p < 0.05). A lower frequency of HLA-DR10 and HLA-DR17 in the RAU patients was observed compared to the healthy subjects (p < 0.05). A statistically higher frequency of HLA-DR10 was observed in the BD patients compared to the RAU patients (p < 0.01). A significantly higher frequency of HLA-A30 was found in the healthy subjects compared to the BD patients (p < 0.05). The differences among all the other HLA-A, B (class I) and HLA-DR, DQ (class II) antigens were not statistically significant in the patients with RAU and BD and the healthy subjects (table 1).
Table 1.
Frequencies of HLA-A and B and HLA-DR and DQ antigens in patients with BD and RAU and in healthy controls
| HLA antigens | Patients |
p | Odds ratio (95% CI) | ||
|---|---|---|---|---|---|
| with BD (n = 30) | with RAU (n = 30) | Healthy controls (n = 15) | |||
| A23 | 1 (3.3) | 8 (26.7) | 0.026* | 0.095 (0.011–0.815) | |
| A24 | 10 (33.3) | 1 (6.7) | 0.049* | 7.000 (0.802–61.070) | |
| A30 | 4 (13.3) | 7 (46.7) | 0.026* | 0.176 (0.041–0.759) | |
| A30 | 1 (3.3) | 7 (46.7) | 0.001** | 0.039 (0.004–0.369) | |
| B13 | 0 (0) | 7 (23.3) | 0.011* | 2.304 (1.694–3.134) | |
| DR10 | 10 (33.3) | 1 (3.3) | 0.006* | 14.500 (1.718–122.395) | |
| DR10 | 1 (3.3) | 5 (33.3) | 0.012* | 0.069 (0.007–0.664) | |
| DR17 | 1 (3.3) | 5 (33.3) | 0.012* | 0.069 (0.007–0.664) | |
The values for patients and controls are given as number with the percentage in parentheses. Fisher's exact test.
p < 0.05
p < 0.01.
Discussion
Although the immunopathogenic mechanisms of RAU and BD are not clear, infectious agents, immune mechanisms and genetic factors are thought to be involved in the onset of the diseases [7,21], immunogenetic factors seem to play an important role in susceptibility and resistance. Nevertheless, the correlation between HLA antigens and pathogenesis is still obscure. It is hard to predict whether RAU will eventually become BD or not, especially because the relationship between RAU and BD is still controversial [14,15,18].
In this study, HLA-A23 and HLA-B13 had a higher frequency in patients with RAU compared to BD while HLA-DR10 had a higher frequency in BD patients compared to RAU patients. These findings suggest that RAU and BD are not in the same spectrum as has been observed in other studies [18,22,23,24], and that the involvement of other genetic and/or environmental factors may be responsible for the development and/or progression of these diseases. Nevertheless, Lehner et al. [14] had suggested that BD and RAU may be in the same spectrum; however, Sun et al. [15] observed that there is no significant difference in the frequencies of HLA-DR and DQ antigens between patients with BD and those with RAU. Our findings seem to indicate that HLA-A30 might be considered a marker of low specificity of RAU and BD in Turkish people and that it may be a protector HLA antigen. But this assumption needs to be confirmed by further studies.
BD is strongly associated with HLA-B51 in many different ethnic groups [8,11,12], although it is still unclear whether the susceptibility to BD is influenced by HLA-B51 itself or by some other non-HLA antigen [7,23]. Our results did not reveal any remarkable influence of HLA-B51 on the severity of BD. However, this does not answer the question of whether the susceptibility antigen related to the disease is the HLA-B51 itself or another non-HLA antigen in linkage disequilibrium with the HLA-B51.
Despite the well-established association of HLA-B51 with BD in many ethnic groups, different results of the association between HLA class II antigen and BD-RAU have been reported [15,16,18]. According to Lehner et al. [14], the immunogenetic basis of BD and RAU based on the HLA-A and B loci has been extended to the HLA-DR locus. Therefore, in this study, we investigated whether HLA class II antigens are associated with BD and RAU. In our analysis of HLA class II antigen in BD and RAU, the frequency of HLA-DR10 and HLA-DR17 was found to be relatively low in Turkish patients with RAU compared to healthy control subjects and the frequency of HLA-DR10 was found to be relatively low in Turkish patients with RAU compared to those with BD (table 1). These results suggest that some specific HLA-DR antigens may play important roles in the development of BD and RAU. On the other hand, according to Pirim et al. [7], in their genotyping of HLA class II alleles, HLA-DRB104 and HLA-DRB107 were the predominant alleles in BD Turkish patients. An association of BD with HLA-DRw52 in Japanese people [8], with HLA-DR7, HLA-DRw52, and HLA-DRw53 in British people [14] and with HLA-DRw52 in Italian people has been reported [25]. Sun et al. [6] demonstrated a strong association of the HLA-DRw8 antigen as well as HLA-DRw8/DQw1, DRw8/DQw5(w1), DRw12(5)/DQw1, DRw12(5)/DQw6(w1), and DRw52/DQw1 haplotypes with BD in Chinese people. In addition, they showed no significant association in the frequencies of HLA-DR and DQ antigens in Chinese patients with BD compared to those in healthy control groups [15]. In their genotyping of HLA class II alleles, Pirim et al. [7] found that HLA-DRB104 and HLA-DRB107 were the predominant alleles in BD patients. Although there were different HLA class allele distributions within the groups, the results were not significant. They showed that there is a lack of an association of class II alleles with BD. Kera et al. [26] reported similar results; the frequency of HLA-DR5 was found to be relatively high in BD patients compared to that in healthy controls but was not statistically significant. In contrast, in another study by Balboni et al. [27], the same HLA-DR5 and the DQ3 frequency was found as well when Italian patients with BD were studied. Similar to our study, these authors [26,27] analyzed HLA class II association with BD in Italian patients only by the serological method and reported a significant increase of the DR5-DQ3 haplotype. Lehner et al. [14] suggested that the immunogenetic basis of BD and RAU based on the HLA-A and B loci be extended to the HLA-DR locus. Gallina et al. [28] found a statistically increased value for the HLA-DR7 frequency for a sample of 26 Sicilian patients with RAU. The frequency of HLA-DR7 antigen increased significantly in RAU-affected persons, whereas the B5 antigen frequency decreased significantly. In another study [18], data showed an increased frequency of HLA-DR4 antigen in patients with RAU compared to that in patients with BD. In our analysis of HLA class II antigen in BD and RAU, the frequency of HLA-DR10 and HLA-DR17 was found to be relatively low in Turkish patients with RAU compared to healthy control subjects, and the frequency of HLA-DR10 was found to be relatively low in Turkish patients with RAU compared to those with BD (table 1). These results suggest that some specific HLA-DR antigens may play important roles in the development of BD and RAU. Numerous studies found that the HLA class II antigen frequencies for BD and RAU were different from those found in our study probably because populations of different ethnic origins were studied (British, Italian, or Chinese).
Several reports from different countries showed a genetic correlation of RAU with HLA antigens, but the results of these studies are controversial [6,14,28,29]. In our study, HLA-A24 and B13 had a higher frequency for RAU, while HLA-DR10 and DR17 had a lower frequency (table 1). In agreement with other studies [8,12], this finding supports the hypothesis that a specific antigen may possibly be responsible for RAU. In an English population, Challacombe et al. [29] found that the HLA-B12 frequency was associated with patients with RAU. In groups of patients of a different ethnic origin, a significant association between HLA-DR2 and RAU was noticed [9,14]. Wilhelmsen et al. [30] observed that the HLA frequencies that had the highest rates of patients with RAU were HLA-A33, HLA-B35, and HLA-B81. Gallina et al. [28], with a sample of 26 Sicilian patients with RAU, found a statistically increased value for HLA-DR7 frequency. Sun et al. [6] stated that the HLA-DRw9 frequency can be considered to be a genetic marker for RAU in the Chinese population. Other previous cross-sectional studies from the United Kingdom and Greece have suggested that certain HLA antigens are linked to RAU, notably the class I antigens A2 and B12 [14] and the class II antigen DR5 [9]. In our study, HLA-A24 and B13 were associated with an increased risk of RAU, while HLA-DR10 and DR17 were associated with a decreased risk (table 1). In agreement with other studies [8,12], this finding supports the hypothesis that a specific antigen may possibly be responsible for RAU. Finally, further studies could be mapped to the possible genetic factors involved in the genesis of RAU for each population.
Conclusion
Our findings showed that BD and RAU were not in the same spectrum; there were no differences of HLA-B51 among BD, RAU, and healthy subjects. The presence of HLA-A30 is useful as a determiner for subjects at risk of developing BD and RAU. We recommend that a more advanced method such as single specific primer-polymerase chain reaction should be used to obtain more specific results as well. We aim to further our studies with more advanced methods in the near future.
Acknowledgement
This research was supported by the Marmara University Scientific Research Project Council (project No. SAG-DKR-200407-0078). Authors would like to thank Biologist. Mustafa Aslan, PhD for his technical assistance, Centro Laboratories for providing the use of laboratory equipment, and expert rheumatologist, Dr. Melek Özer.
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