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    Evaluation of interleukin 8 +2767 A/T polymorphism in visceral leishmaniasis

    2016-11-24 11:34:30AlirezaAhmadiMehrdadHajilooiGhasemSolgiMohammadAbasiAhadBazmaniAlirezaKhalilianMohammadMatiniKhosroSardarian

    Alireza Ahmadi, Mehrdad Hajilooi, Ghasem Solgi, Mohammad Abasi, Ahad Bazmani, Alireza Khalilian, Mohammad Matini, Khosro Sardarian?

    1Department of Internal Medicine, School of Medicine, Hamadan University of Medical Sciences, Hamadan, Iran

    2Department of Immunology, Faculty of Medicine, Hamadan University of Medical Sciences,Hamadan, IR Iran

    3Department of Internal Medicine, School of Medicine, Hamadan University of Medical Sciences, Hamadan, Iran

    Evaluation of interleukin 8 +2767 A/T polymorphism in visceral leishmaniasis

    Alireza Ahmadi1, Mehrdad Hajilooi2, Ghasem Solgi2, Mohammad Abasi1, Ahad Bazmani2, Alireza Khalilian1, Mohammad Matini3, Khosro Sardarian3?

    1Department of Internal Medicine, School of Medicine, Hamadan University of Medical Sciences, Hamadan, Iran

    2Department of Immunology, Faculty of Medicine, Hamadan University of Medical Sciences,Hamadan, IR Iran

    3Department of Internal Medicine, School of Medicine, Hamadan University of Medical Sciences, Hamadan, Iran

    ARTICLE INFO

    Article history:

    Accepted 16 August 2016

    Available online 20 November 2016

    Interleukin 8

    Polymorphism

    Visceral leishmaniasis.

    Objective: To evaluated the relationship between the genetic variations at IL-8 +2767 position with VL pathogenesis among Iranian patients. Methods: Three groups including patients with VL clinical presentation and leishmania seropositive(n=124), patients seropositive but without clinical presentation(n=82) and healthy controls(n=63) were selected to conduct this cross-sectional study. Polymorphism at +2767 position of IL-8 was investigated using PCR-RFLP techniques. Anti-leishmania antibody titration was evaluated by the immunoflorescence technique. Results: We observed higher significant frequencies +2767 A/A and A/T genotypes in groups 1 compared to group 2 and healthy controls (P=0.001). Also, patients in Group 1 carriyng A/A genotype showed higher titer of antileshmania antibody than patients with A/T and T/T genotypes (P=0.05). The validity of the data was analyzed using Hardy-Weinberg equilibrium and one way analysis of variance (ANOVA), as well as χ2tests. Conclusions: Our findings indicate that the IL-8 +2767 polymorphism is significantly involved in impaired immune responses against VL and it could be considered as a risk factor for the VL progress.

    1. Introduction

    Leishmaniasis, a serious public health problem, is a protozoan disease with multiple clinical features which manifests predominantly in cutaneous, diffuse cutaneous, mucocutaneous and visceral clinical forms [1]. Visceral Leishmaniasis (VL) infections or Kala Azar result in the most severe forms of the disease [2], causing death if left untreated, and are endemic in tropical and sub-tropical regions [3]. It can be undiagnosed or develop into clinical manifestations, including fever, weight loss, pancytopenia, febrile splenomegaly and hepatomegaly [4]. Although VL infection is a protozoan disease, immunologic dysfunctions play a vital role in VL pathogenesis. A main aspect of the disease is a deficit in immune response to leishmania antigen and lymphokine production [5,6].

    Interleukin 8 (IL-8), a proinflammatory cytokine, is produced by leukocytes as well as many types of tissues upon inflammatory conditions and neutrophils are considered to be major specific targets for IL-8 action [7]. Therefore, genetic variations in IL-8 gene resulting in IL-8 expression levels may affect immune responses and leishmaniasis phenotype [8]. It has been implicated that the functional polymorphism at +2767 (rs1126647) position located within 3`UTR of IL-8 gene may influence the level of IL-8 expression [9]. This study aimed to evaluate whether the progress of VL can be associated with IL-8 +2767 polymorphism in the seropositive VL patients with and without clinical presentation. Theprimer sequences for detection of IL-8 +2767 A/T polymorphism were F:5`-CCAGTTAAATTTTCATTTCAGGTA-3`, R:5`-CAACCAGCAAGAAATTACTAA-3`.

    2. Materials and methods

    This cross-sectional research was carried out on 124 VL seropositive patients with clinical presentation (Group 1), 82 seropositive patients without clinical presentation (Group 2) and 63 healthy controls (Group 3) to evaluate IL-8 +2767 A/T polymorphism. An expert infectious diseases specialist diagnosed VL in participants based on medical history, clinical presentations and laboratory findings [10]. The VL patients and participants in Group 2 and 3 were from East Azarbaijan where the Leishmania infantum is endemic [11]. The participants filled out an informed consent form and the ethical approval for this study was obtained from Hamadan University of Medical Sciences.

    2.1. DNA extraction and polymorphism detection

    Genomic DNA was extracted from peripheral blood using a commercial kit (Bioneer, South-Korea) based on the manufacturer's instructions.

    The IL-8 +2767 A/T gene polymorphism was evaluated using RFLP techniques. To amplify the regions containing this site, PCR was performed in a final volume of 20 μL containing 1.5 mM MgCl2, 0.2 mM of each dNTP [(dATP, dCTP, dGTP, dTTP), 10 pM of each primer (25 ng/μL), 0.5 of Taq DNA polymerase, 100 ng of prepared DNA template and 1x PCR buffer. The forward and reverse primers sequencing for amplification of the IL-8 +2767 A/T (222 bp) containing position are shown in the Table 1. The PCR condition was as follows: 1 cycle of 95 ℃ for 5 min (denaturation) then 35 cycles of 30 Sec at 95 ℃, 53 ℃ for 30 Sec and 72 ℃ for 40 Sec using a thermal cycler (Bioneer, South Korea). The PCR product was digested with BstZ17I ( Fermentase Company, Finland) in the case of T allele into 198 bp and 24 bp sub-fragments. Thereafter, the PCR product was separated on an ethidium bromide pretreated 2.5% agarose gel in parallel with a 50 bp ladder (Cinnaclon, Iran).

    2.2. Immunoflorescence assay

    Anti-leishmania antibody titration was performed with a commercial kit from Qiagen Company, USA, based on the manufacturer's instructions.

    2.3. Statistical analysis

    The validity of data was evaluated using Hardy-Weinberg equilibrium and the One Way ANOVA as well as χ2tests were used to determine the differences between groups by using the SPSS software version 13. A P value less than 0.05 was considered as significant.

    3. Results

    The results from polymorphism analysis showed that the polymorphism at +2767 (P= 0.001) was significantly associated with VL. We found that +2767 A/A genotype significantly increased in group 1 compared to groups 2 and 3 (Table 1). The statistical analysis demonstrated a significant difference between groups regarding +2767 A and T alleles (P< 0.001, Table 1). Antileishmania antibody levels among VL patients with the +2767 A/A genotype was higher than A/T and T/T genotypes (P=0. 05, Table 2). As shown in Table 2, the anti-Leishmania antibody titration among participants in group 2 with various genotypes within IL-8 +2767 positions was not statistically different.

    Table 1 The status of IL-8 +2767 A/T polymorphism in patients with clinical presentation of VL and seropositive for the leishmania (Group 1), without clinical presentation but seropositive (Group 2) and healthy controls (Group 3) [n(%)].

    Table 2 Anti-leishmania antibody titration in group 1 and 2 with various IL-8 +2767 A/T polymorphism.

    4. Discussion

    Our investigation provides the first evidence that genetic polymorphisms in IL-8 +2767 position among an Iranian population may be involved in impaired immune responses against visceral leishmaniasis. Since IL-8 plays a crucial role in the induction of immune responses against leishmaniasis, genetic variations that influence IL-8 expression or function may contribute to clinically observed leishmaniasis phenotypes and impaired immune response [12]. T cell-mediated immune response predominantly plays significant roles in human leishmaniasis through secretion ofcytokines including IL-4 and IL-10, which induce Th1 and Th2 differentiation or IL-12, which promotes Th1 development[12,13]. These observations prompted us to investigate the clinical relevance between IL-8 genetic variation +2767 position and leishmaniasis progress. We found that genotypes and alleles within IL-8 +2767 position might be involved in the VL development in Iranian population. In addition, our results depicted that the IL-8 +2767 A/A genotype was significantly raised in group 1 compared with Groups 2 and 3. Therefore, it is suggested that this genotype may be associated with VL pathogenesis in Iranian populations. Our hypothesis was verified by several studies focusing on IL-8 relationship with induction of immune responses against leishmania[8,14]. Additionally, it has been shown that contact with Leishmania major results in IL-8 release by monocytes and functions as a neutrophil chemotactic factor [15,16]. It has been reported that Keratinocyte-derived cytokine (also known as CXCL1), the functional murine homologues of human IL-8, is rapidly produced in the skin during Leishmania major infection [17]. On the other hand, Kumar et al. found that IL-8 expression levels were high in cutaneous leishmaniasis patients′ sera [15]. Since +2767 A/A genotype is associated with VL, it is suggested that this genotype may be involved up-regulation of IL-8 in VL patients and further studies using luciferase assays can be helpful to clarify this issue.

    Finally, introducing this IL-8 genetic variation will help us to understand the nature of VL and to design novel chemotherapies or vaccine-based therapies which requires further studies on immune modulations in VL patients [3].

    Conflict of interest statement

    The authors declare that they have no conflicts of interest.

    Acknowledgement

    This project was supported by a grant from the Tabriz University of Medical Sciences (No. 91-20). The project was implemented in the Hamedan University of Medical Sciences, and approved by the ethics committee of both universities.

    References

    [1] Herrador Z, Gherasim A, Jimenez BC, Granados M, San Martin JV, Aparicio P. Epidemiological changes in leishmaniasis in Spain according to hospitalization-based records, 1997-2011: raising awareness towards leishmaniasis in non-HIV patients. PLoS Negl Trop Dis 2015;9(3):e0003594.

    [2] Vilas VJDR, Maia-Elkhoury AN, Yadon ZE, Cosivi O, Sanchez-Vazquez MJ. Visceral leishmaniasis: a One Health approach. Vet Rec 2014;175(2):42-44.

    [3] Araujo Adc, Gon?alves Nnvm, Dantas-Torres F, Ferreira F, Horta Mc. Visceral leishmaniasis in Petrolina, State of pernambuco, Brazil, 2007-2013. Rev Inst Med Trop Sao Paulo 2016;58;29.

    [4] Adel A, Boughoufalah A, Saegerman C, De Deken R, Bouchene Z, Soukehal A, et al. Epidemiology of visceral leishmaniasis in Algeria: an update. PloS one 2014;9(6):e99207.

    [5] Das A, Ali N. Vaccine development against Leishmania donovani. Front Immunol 2012;3:99.

    [6] Singh OP, Gidwani K, Kumar R, Nylén S, Jones SL, Boelaert M, et al. Reassessment of immune correlates in human visceral leishmaniasis as defined by cytokine release in whole blood. Clin Vaccine Immunol 2012;19(6): 961-966.

    [7] Jundi K, Greene CM. Transcription of interleukin-8: how altered regulation can affect cystic fibrosis lung disease. Biomolecules 2015;5(3):1386-1398.

    [8] Hajilooi M, Abasi M, Bazmani A, Ahmadi A, Matini M, Solgi G, et al. Evaluation of interleukin-8 251 T/A polymorphisms in visceral leishmaniasis. J Res Health Sci 2014;15(1):59-61.

    [9] Koensgen D, Bruennert D, Ungureanu S, Sofroni D, Braicu E, Sehouli J, et al. Polymorphism of the IL-8 gene and the risk of ovarian cancer. Cytokine 2015;71(2):334-338.

    [10] Boelaert M, Verdonck K, Menten J, Sunyoto T, van Griensven J, Chappuis F, et al. Rapid tests for the diagnosis of visceral leishmaniasis in patients with suspected disease. Cochrane Database Syst Rev 2014;(6):CD009135.

    [11] Mohebali M. Epidemiological status of visceral leishmaniasis in Iran: experiences and review of literature. J Clinic Experiment Pathol 2013; S3:003.

    [12] Carvalho EM, Carvalho LP, Passos S, Schriefer A. Protective and pathologic immune responses in human tegumentary leishmaniasis. Front Immunol 2012;3:301.

    [13] Dembic Z. Cytokines of the immune system: interleukins. In: Versteeg-Buschman L.(ed.). The cytokines of the immune system the role of cytokines in disease related to immune response. San Diego: Mica Haley; 2015, p. 143-239.

    [14] Menezes-Souza D, Guerra-Sa R, Carneiro CM, Vitoriano-Souza J, Giunchetti RC, Teixeira-Carvalho A, et al. Higher expression of CCL2, CCL4, CCL5, CCL21, and CXCL8 chemokines in the skin associated with parasite density in canine visceral leishmaniasis. PLoS Negl Trop Dis 2012;6(4):e1566.

    [15] Kumar A. Invade and survival strategy of leishmania. Leishmania and leishmaniasis. New York: Springer 2013,p. 29-35.

    [16] Singh JK, Sim?es BM, Howell SJ, Farnie G, Clarke RB. Recent advances reveal IL-8 signaling as a potential key to targeting breast cancer stem cells. Breast Cancer Res 2013; 15(4):210.

    [17] Karam MC, Merckbawi R, Salman S, Mobasheri A. Atenolol reduces leishmania major-induced hyperalgesia and TNF-without affecting IL-1β or keratinocyte derived chemokines (KC). Front Pharmacol 2016; 7:22.

    Document heading 10.1016/j.apjtm.2016.09.010

    4 June 2016

    in revised form 8 August 2016

    Alireza ahmadi, Department of Internal Medicine, School of Medicine, Hamadan University of Medical Sciences, Hamadan, Iran.

    E-mail: dralzahmadi@umsha.ac.ir

    ? Khosro Sardarian (MSc), Department of Parasitology and Mycology, School of Medicine, Hamadan University of Medical Sciences, Hamadan, Iran.

    Postal Code: 65178-3-8736

    Tel: +98-8138380574

    Fax: +98-8138383208

    E-mail: khsardarian@gmail.com

    Foundation project: This project was supported by a grant from the Tabriz University of Medical Sciences (No. 91-20).

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