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Behcet's disease (BD) was first introduced in 1937 by Hulusi Behçet (1). BD is a chronic and systemic vasculitis with inflammation and dysfunction of various organs and systems including: immune system, central nerve system, heart, gastrointestinal tract and joints. The disease is characterized by the occurrence of recurrent aphthous ulcer in different parts of the body. According to several studies, outbreaks of BD are most commonly reported from Turkey, with a prevalence of 20–421 cases per 100000 population. After Turkey, Iran is the second most prevalent country with about 80/100000, in general population. The prevalence of BS in the Middle East, varies between 17–80/100000, and in the Far East, the prevalence of BS is approximately 2.6–15/100000 among Japanese and Chinese people. On the other hand, the prevalence of BD in western and European countries, e.g. the United Kingdom and the United States is ranged from 0.12–0.66 per 100000 in General population (2-5). The etiology and pathogenesis of Behcet disease are not clear but are assumed to be multifactorial, including the involvement of genetics (human leukocyte antigen (HLA-B51 allele)), infectious agents (bacteria and viruses), and immunological factors (2).
Herpesviridae is a large family of DNA viruses that cause infections in animals and humans. Distinct viruses of the family are associated with several important diseases in humans including Herpes Simplex Virus 1 and 2 (HSV-1,2), Epstein-Barr Virus (EBV), Human Herpes Virus 6 and 7 (HHV-6,7), Kaposi's sarcoma-associated herpesvirus (HHV-8), and Human cytomegalovirus(HCMV) (6, 7). HCMV belongs to betaherpesvirinae subfamily and cytomegalovirus genus (8). The virus often causes asymptomatic primary infection in the first years of life and remains latent in monocytes, bone marrow, and other tissues (9, 10). However, several studies have been conducted about the prevalence of HCMV in the Behcet's, but, Concurrent prevalence of IgG, IgM antibodies against HCMV and virus DNA titers in serum of Behcet's patients has not been studied.
Study Population
This was a cross-sectional study including 103 Behcet's patients (54 male and 49 female). They were referred to hospitals affiliated with Iran University of Medical Sciences in the period between January 2016 and February 2019. Ethical approval for this study was obtained from IUMS’s Medical Ethics Committee (Ethic code number: IR.IUMS.REC 1396.32331). Written informed consent was obtained from all the study patients.
Collection and Preparation of the Samples
About 10 mL of whole blood samples was collected from each patient. Serum was separated by centrifugation and stored at –80℃ and –20℃ for HCMV DNA and serological examinations, respectively.
Serological assays
HCMV serological markers including IgM and IgG were tested by a Vircell ELISA kit according to the
manufacturer’s instructions (Vircell, Spain).
DNA extraction and Polymerase Chain Reaction
HCMV DNA was extracted from 220 µl of the serum using a High Pure Viral Nucleic Acid Kit (Roche Diagnostics GmbH, Mannheim, Germany) with a procedure adapted from the manufacturer’s recommendation. DNA was eluted using 30 µl of the RNAase/DNAase free buffer and stored in -70 °C. For HCMV DNA detection in the serum samples, Real time PCR was performed using TaqMan kit, based to the manufacturer’s instructions. A highly conserved region of the glycoprotein B (UL55) gene was selected for amplification of HCMV DNA. Sequences of the HCMV primers and probe was as follows (11):
HCMV Forward Primer (5´- TGGGCGAGGACAACGAA -3´)
HCMV Reverse Primer (5´- TGAGGCTGGGAAGCTGACAT-3´)
HCMV PROBE (5´- 6- FAM- TCGGCAACCACCGCACTG –BHQ- 3´).
Real-time PCR was performed by TaqMan universal master mix. DNA was added to a 16 mL PCR mixture containing 8 mL of TaqMan universal PCR master mix, 1mL each primer and probe mix. The reaction consisted of 10 minutes at 94°C, followed by 40 cycles of amplification, including 15 s at 94°C and 40 s at 60°C.
Statistical analysis
Statistical analysis was done using IBM SPSS version 20 (IBM Corp., Armonk, NY, USA). Data was reported as mean ± standard deviation. For all comparisons, p-values <0.05 were considered to be statistically significant.
Of 103 participated patients, 53% (54/103) were male and 47% (49/103) were female. The mean age was 38.86±8.76 and 39.35±7.50 in males and females, respectively, which had not significant difference between male and female (Table 1). Also, the duration of disease was 20.34±5.87 and 18.82±5.96 in males and females, respectively. HCMV IgG antibody was found in 96% and 94% of males and females, respectively, and IgM antibody was positive only in one male patient. Our Real time PCR assay detected no HCMV DNA in the study patients. Despite the high prevalence of IgG antibody against cytomegalovirus in Behcet's patients, no virus genome was found in these patients (table1).
Table 1. Demographic parameters as well as laboratory data for the studied Behcet patients
Parameters | Sex (n=103) | P-value or Odds ratio (CI95%) | |
---|---|---|---|
Male (54) | Female (49) | ||
Age, mean ± SD | 38.86±8.76 | 39.35±7.50 | 0.89 |
HCMV-IgM | (1) 1.8% | 0 | 0.77 |
HCMV-IgG | (52) 96% | (46) 94% | 0.95 |
HCMV-DNA | 0 | 0 | 0.999 |
Duration (month) | 20.34±5.87 | 18.82±5.96 | 0.81 |
Treatment recipients | 100% | 100% | 0.999 |
Standard deviation (SD)
The exact role of infectious agents, especially viruses, in the pathogenesis of rheumatic diseases is unclear (12). In people with inflammatory diseases, individuals receiving immunosuppressive therapy and with a genetic predisposition, infection with environmental factors such as viruses can lead to immune system disruption (13-16). In this study, we investigated the levels of IgG and IgM antibodies against HCMV as well as the DNA of the HCMV virus in the serum of patients with Behcet's syndrome. Our results showed that the prevalence of IgG antibody against HCMV was 96% and 94% in male and female respectively. However, IgM was positive in one male patient and no DNA virus was detected in the patients. IgG antibodies against CMV are seen in 95% of the general population. However, the absence of the virus genome in a positive IgM person can be due to the Short-term DNAemia. the study by Sulieman showed among 17 patients with positive IgM against CMV, 10 cases have PCR positive, while among 7 cases the CMV-DNA not founded (17).
HCMV causes primary infection in the first years of life and remains mainly latent in monocytes, bone marrow, and other tissues (9, 18). On the other hand, Due to the impaired immune system and the abundant use of immunosuppressive or antimetabolite treatment in Behcet's patients, they are susceptible to viral infection (13, 19). HCMV with transmission to endothelium or fibroblasts cells can negatively affect the prognosis of patients with immune deficiency (20).
Oner et al., Showed that IgG titers against HCMV were positive in 100% of Behcet's patients, but antibody titers were lower than controls (19). Sari's study showed that HCMV colitis develops in Behcet's patients with neurological involvement following TNF inhibitor use (21). Other studies have also shown that use of immunosuppressive drugs in gastrointestinal patients with Behcet's disease due to HCMV virus causes gastrointestinal lesions, but with treatment discontinuation, these lesions return (22). The study by Lee et al. showed that HCMV plays a role in the return of ulcers in Behcet's patients (23). Similar to the Oner study, Seoudi's study also showed that IgG antibody titers were lower in Behcet's patients compared to controls (24). In the present study, unlike previous studies, there was no control group. But IgM antibody and virus genome levels were assessed. IgG positivity and lack of virus genome in the serum may be due to the virus being in the latent stage or the virus being cleared from the body. The results of this study indicated that no infectious HCMV can be detected in serum samples of Behcet's patients by our TaqMan real-time PCR assay. There are some limitations to the explanation of the test results for IgM. The disadvantage, false-positive results due to rheumatoid factor interference. and in immunosuppressed patients, e.g. chronic renal failure, end-stage renal disease and blood diseases (25). In addition, there is a time lag between primary infection and IgM antibody production (IgM level can remain undetectable because of delayed seroconversion owing to immunosuppressive agents). IgM antibodies can also persist for a long time after infection in some healthy individuals (26).
The lack of a control group is the most important limitation of this study.
This project was financially supported by a grant from the Iran University of Medical Sciences (No: IR.IUMS.REC 1396.32331).
Authors declared no conflict of interests.
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