Virological
Communication
Biosci. Biotech. Res. Comm. 9(2):
Association of
Priyanka Kashyap*1, Manab Deka1, Sangit Dutta2 and Namrata Kumari1
1Department of Bioengineering and Technology, Laboratory of Molecular Virology & Oncology, Gauhati University, Guwahati, Assam, India
2Department of Medicine, Gauhati Medical College, Guwahati, Assam, India
*Priyanka Kashyap, Department of Bioengineering and Technology, IST, Gauhati University, Guwahati, India
ABSTRACT
Hepatitis A is one of the most common causes of acute viral hepatitis worldwide. Hepatitis A infection can also result in a cholestatic hepatitis or a relapsing course or fulminant liver failure. TLR polymorphisms have been implicated in susceptibility, pathogenesis and progression of viral hepatitis.The aim of the present study was to investigate the role of TLR 2 (rs5743708), TLR7 (rs179009) and TLR9 (rs5743836) polymorphism with association of HAV infection risk in population of Assam. The SNP study was performed by genomic DNA extraction followed by
KEY WORDS: CHOLESTASIS, FULMINANT, HEPATITITS A, POLYMORPHISM, TOLL LIKE RECEPTOR.
ARTICLE INFORMATION:
*Corresponding Author: kashyappriyanka99@gmail.com Received 25th May, 2016
Accepted after revision 28th June, 2016 BBRC Print ISSN:
Thomson Reuters ISI SCI Indexed Journal NAAS Journal Score : 3.48
© A Society of Science and Nature Publication, 2016. All rights289 reserved.
Online Contents Available at: http//www.bbrc.in/
Priyanka Kashyap et al.
INTRODUCTION
Hepatitis A is one of the most common causes of acute viral hepatitis worldwide (MMWR.,1996). Globally, an estimated 1.4 million cases of hepatitis A virus (HAV) infection occur annually. The liver injury from hepatitis A infection is usually mild, mostly in children, where it is frequently subclinical. But in adults, infection with hepatitis A can result in acute or fulminant liver fail- ure. Hepatitis A infection can also result in a choles- tatic hepatitis or a relapsing course (Glikson et al.,1992). The reported overall
TLRs recognize a wide variety of pathogen associ- ated molecular patterns (PAMPs) from a wide range of host like bacteria, viruses, and fungi, as well as some other host molecules (Aderem and Ulevitch.,2000). TLR’s play a key role in the pathophysiology of a range of human diseases, including cancer. TLR2 gene is located on chromosome 4 and recognizes conserved molecular patterns (e.g. lipopolysaccharide (LPS) on bacteria which are major inducers of the inflammatory response. It is involved in the innate immune system (Medzhitov.,2001) and TLR2 is capable of detecting the widest repertoire of
Genetic studies on the TLR2 gene have identified a number of polymorphisms which have been shown to affect host defense and disease progression (Chen et al.,2010; Takeda et al., 2003). TLR 2 SNP rs5743708 is associated with tuberculosis, staphylococcal septic shock, heart restenosis, Lyme disease and cytomegalo- virus (CMV) disease after liver transplantation (Ogus et al., 2004;Lorenz et al., 2000; Schro¨der et al., 2005; Kijpittayarit et al., 2007). Also it correlates with trans- plant rejection and higher mortality of chronic hepatitis C patients (Eid et al., 2007).
TLR7 is mainly expressed in the
ssviral RNA which are released upon phagocytosis when phagocytes take up a virus or
TLR9 is localized intracellularly mostly in the endo- cytic compartments and TLR9 recognizes unmethyl- ated CpG motifs present in bacteria and viruses (Pan- dey et al., 2006). TLR9 functions through the MyD88
dependent pathway leading to
The role of host genetic factors in determining sus- ceptibility to infections has become more evident; some persons may be predisposed to certain infections, whereas others are protected (Hill, 2001). Evidence sug- gests that single nucleotide polymorphisms (SNPs) in the TLR genes impair the ability to respond to different type of infection (Weltzler., 2003). And so we hypothesise that a better understanding of the HAV disease infection may be achieved by studying the TLR2, TLR7 and TLR9 gene polymorphism of the susceptible and resistant persons may contribute to the HAV infection severity. The aim of the present study was to investigate the role of TLR 2 (rs5743708), TLR7 (rs179009) and TLR9 (rs5743836) polymorphism with association of HAV infection risk in population of Assam.
MATERIAL AND METHODS
Study subjects: A total of 179 patients with HAV infec- tion were included in the study between 2012 and 2014 with prior written informed consent. An almost equal number of age- and sex- matched healthy controls (voluntary blood donors) who had no history of hepa- titis, hepatobiliary diseases, negative for HAV IgM and autoimmune hepatitis, were also included in the study. Patients were enrolled from general OPD and Medicine Ward of Gauhati Medical College and Hospital (GMCH), Guwahati, Assam on the basis of clinical investigation, positive for HAV IgM using 3rd generation ELISA kit and confirmed by HAV detection PCR spanning a region of 154 b.p. for VP1 region. Patients who were positive for other hepatotropic virus, HIV, autoimmune hepati- tis, alcoholic and drug abuse were excluded. The study was approved by the institutional ethical committee of Gauhati University, Guwahati.
In this study, prolonged cholestasis was defined as that with total bilirubin level ≥5 mg/dL lasting for more than 4 weeks after admission (Jung et al., 2010) . Acute liver failure according to the widely accepted definition of acute liver failure that states there would be evidence of coagulation abnormality, usually a prolongation of PT by INR ≥1.5 or prothrombin time >15 seconds, and any degree of mental alteration (encephalopathy) in a patient without
DNA EXTRACTION
Blood samples (5.0 ml) from HAV patients and control subjects were collected in EDTA vials and stored at 4 oC until required. Genomic DNA was extracted from whole blood by standard
GENOTYPING
TLR2 (rs rs5743708), TLR7 (rs179009) and TLR9 (rs5743836) genotypes were determined by a polymer- ase chain reaction (PCR) method, and were genotyped by
The PCR product of 190 b. p. of TLR7 rs179009 was amplified using the set of primers 5’- ATTTGCTGC-
The PCR product of 164 b. p. of TLR9 rs5743836 was amplified using the set of primers
Priyanka Kashyap et al.
on 2.5% agarose gel electrophoresis. A single band of 164 b. p. characterised mutant type T allele, while the presence of three bands at 164, 136 and 28 b.p. or two bands at 136 and 28 b.p. only characterises heterozy- gous and homozygous wild variant respectively (C allele is the wild allele). Positive and negative controls were used in the genotyping protocol and 5% of randomly selected samples were
STATISTICAL ANALYSIS
All statistical analyses were performed by the standard methods using SPSS computer software (Version 13, SPSS Inc., Chicago, IL, USA). Results were expressed as means ± standard deviations (SD). A
0.05was considered statistically significant.
RESULTS AND DISCUSSION
DEMOGRAPHIC DATA OF THE STUDY SUBJECTS
A total of 179 HAV confirmed cases were included in the study. The male and female ratio was found out to be 17:9 for all the HAV cases together and so the male gender was predominant (65%) (Table I). It was seen that the confirmed cases of HAV infection belonged mostly to the young adults in this region and so Hepatitis A frequently occurred in the young adults where mean age was calculated to be 25 years. Fulminant hepatic failure developed in 2.8% of the Hepatitis A patients (Table II). Among the 179 HAV patients, 11.2% patients had pro- longed cholestasis during admission.
Table 1: Clinical and laboratory characteristics of hepatitis A cases (n = 100) [ALT – alanine transaminase; AST
Priyanka Kashyap et al.
Table 2: Stratification of the Hepatitis A cases based on their clinical profile
ASSOCIATION OF TLR2 (RS5743708), TLR7 (RS179009) AND TLR9 (RS5743836) GENE VARIANTS WITH HAV INFECTION RISK
The observed genotype frequencies in the study subjects were in agreement with Hardy Wienberg Equilibrium. To analyse the association between genetic variant with risk of HAV infection, the genotype frequency distribu- tion of TLR2, 7 and 9 in HAV cases and control group was compared and shown in Table III.
The genotype and allele frequencies observed at this rs site 5743708 were in agreement with
overall the heterozygous variant GA was most prevalent in both control and HAV cases (52.9 % and 34 % respec- tively). The mutant variant AA was more prevalent in cases than controls (33% vs 9.5%). The variant allele A was found overall more in HAV cases compared to con- trols (67% vs 62.4 %) (Table III).
The wild variant TT of TLR7 rs179009 frequency was higher in controls compared to HAV cases (68.9% vs 67.6%). The wild allele T was dominant in our study cohort (78% and 74.6% in controls and HAV cases respectively). The mutant variant CC was comparatively less in both HAV cases and controls (18.4% vs 12.9%). There was no significant difference between the allelic and genotypic frequencies among the HAV cases and controls (p=0.9). The presence of mutant genotype CC did not significantly increased the risk of HAV infection compared to controls [OR=1.0(0.5619- 1.864) at 95%CI] (Table III).
The wild variant CC frequency was higher in controls compared to HAV cases (69.4% vs 17.3%). The mutant variant TT prevalence was very high in HAV cases com- pared to controls (76.6% vs 2.4%). There was significant difference between the allelic and genotypic frequencies among the HAV cases and controls (p<0.0001). The pres- ence of mutant genotype TT significantly increased the
Table 3: TLR2, TLR7 and TLR9 gene variants and susceptibility to HAV infection risk [Bold values represent significant risk ; OR Odds ratio; CI confidence interval]
Priyanka Kashyap et al.
Table 4: Genotypic frequency of TLR2 gene variants and susceptibility to different HAV complications [Bold values represent significant risk;OR Odds ratio;CI confidence interval].
Table 5: Genotypic frequency of TLR7 gene variants and susceptibility to different HAV complications [Bold values represent significant risk; OR Odds ratio;CI confidence interval].
risk of HAV infection compared to controls [OR=10.2 (5.30- 20.29) at 95%CI] by several folds (Table III).
ASSOCIATION OF TLR2(RS5743708), TLR7(RS179009) AND TLR9(RS5743836)
GENE POLYMORPHISM WITH DIFFERENT HAV COMPLICATIONS
The genotypic frequencies of the TLR2, TLR7 and TLR9 SNP’s were correlated with the two HAV case groups ie HAV with cholestasis and HAV caused FHF to investigate whether any possible association is implicated between the polymorphisms and the HAV complications.
In case of different HAV case groups, the presence of variant allele A of TLR2 rs5743708 significantly increased the risk of cholestasis compared to controls (p=0.004) [OR=2.5 (1.328- 4.808) at 95%CI] and non significantly compared to Acute HAV (p=0.6) [OR=1.1(0.6296- 2.005) at 95% CI) and HAV caused FHF (p<0.0001) [OR=0 at 95% CI) . The variant allele was most prevalent in FHF cases (100%) compared to controls and other HAV case groups (Table IV).
When the distribution of TLR7 rs179009 was studied in the different HAV case groups, the data showed that
presence of the wild variant TT was higher in acute HAV cases (70.1%) compared to the controls (68.9%) and HAV with cholestasis (65%), but was not found in the FHF cases (0%) . The mutant variant allele C was most preva- lent in FHF cases (90% vs 22%) compared to controls. The mutant variant CC was associated significantly with HAV caused FHF (p<0.0001) and was not found to be a risk factor (OR=0) . This polymorphism is also not signif- icantly associated with acute HAV (p=0.8) and HAV with cholestasis (p=0.5), and did not significantly increase the risk of acute HAV [OR=0.9 (0.52- 1.749) at 95%CI] and HAV with cholestasis [OR= 1.1 (0.6589- 2.162) at 95% CI] (Table V).
The distribution of TLR9 rs5743836 in the differ- ent HAV case groups showed that presence of the wild variant CC was higher in controls (69.4%) compared to the acute HAV (17.5%) and HAV with cholestasis (30%), and FHF cases (20%) . The heterozygous mutant variant CT was most prevalent in FHF cases (80% vs 28.2%) compared to controls and other case groups. The overall mutant variant (CT+TT) was more prevalent in the HAV case groups rather than the controls. The presence of the mutant allele T significantly increased the risk of acute HAV [p<0.0001; OR=10.07 (5.242- 19.97) at 95%CI] ,
Priyanka Kashyap et al.
HAV with cholestasis [p<0.0001; OR=5.05 (2.784- 9.324) at 95% CI] and FHF (P<0.0001; OR=8.5(4.542- 16.64) at 95% CI) (Table VI).
There is ever increasing evidence suggesting the role of host genetic factors on the different outcomes of hep- atitis infection (Thurz., 2001; Lin et al., 1989). The TLR pathways have been implicated to play important roles in innate immunity against different types of pathogens in humans (Isogawa et al., 2005; Hoebe et al., 2003;
Understanding the host immune factors and its inter- action with the virus may improve the Hepatitis A dis- ease management. Genetic studies on the TLR2 gene have identified a number of polymorphisms which have been shown to affect host defense and disease progres- sion (Chen et al., 2010; Takeda et al., 2003).
Studies have shown the possible involvement of TLR9 in the pathogenesis of human hepatitis (Jiang et al., 2009). The TLR7 gene is located on the
This is the first study of its kind in this region which shows that TLR2 rs5743708 mutant allele A was signi- ficantly associated with Hepatitis A infection and the mutant variant ’A’ was prevalent in our study cohort ie in the polpulation of this region (both control and patient groups).The genotypic variants AA and GA+AA was also found to be risk factor for HAV caused chole- stasis. The mutant variants (TT+CT) was most prevalent for TLR9 rs5743836 in our study cohort and the mutant variant T was found to be a significant risk factor for HAV infection and was significantly associated with acute HAV, Cholestasis and FHF. TLR7 rs179009 mutant variant CC was highly prevalent in the study and patient groups and the mutant genotypes CC and TC was not significantly associated with HAV infection and was not a risk factor for the same.
There was certain limitation in our study that needs to be addressed. The sample number in this study was mod- erate and so other large
ACKNOWLEDGEMENTS
This first author thanks the Dept of Science and Tech- nology (DST) for INSPIRE Fellowship.
The authors declare that they have no conflict of interest.
CONFLICT OF INTEREST
All authors declare that they have no conflict of interest and also no financial interests relevant to the subject of the manuscript.
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