Detection of hepatitis E virus RNA and genotype in Bangladesh

Background/Aims:  Hepatitis E virus (HEV) in Bangladesh has not been adequately documented. We report HEV RNA and genotype detection in Bangladesh. Methods:  In total, 82 samples were used; 36 sporadic acute hepatitis (AH), 12 fulminant hepatitis (FH), 14 chronic liver disease (CLD) and 20 from an a...

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Published in:Journal of gastroenterology and hepatology 2009-04, Vol.24 (4), p.599-604
Main Authors: Sugitani, Masahiko, Tamura, Akinori, Shimizu, Yohko K, Sheikh, Aleemuzzaman, Kinukawa, Noriko, Shimizu, Kazufumi, Moriyama, Mitsuhiko, Komiyama, Kazuo, Li, Tian-Cheng, Takeda, Naokazu, Arakawa, Yasuyuki, Suzuki, Koyu, Ishaque, Shamsuddin M, Roy, Projesh K, Raihan, ASMA, Hasan, Mahmud
Format: Article
Language:English
Subjects:
Acute Disease
Adolescent
Adult
Aged
Amino Acid Sequence
Bangladesh
Bangladesh - epidemiology
Base Sequence
Biological and medical sciences
Child
Chronic Disease
Female
Gastroenterology. Liver. Pancreas. Abdomen
Genotype
Hepatitis Antibodies - blood
Hepatitis E - diagnosis
Hepatitis E - epidemiology
Hepatitis E - virology
Hepatitis E virus
hepatitis E virus (HEV)
Hepatitis E virus - genetics
Hepatitis E virus - immunology
HEV RNA
Humans
IgM specific anti-HEV
Immunoglobulin G - blood
Immunoglobulin M - blood
Male
Medical sciences
Middle Aged
Molecular Sequence Data
Phylogeny
RNA, Viral - blood
Young Adult
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Summary:Background/Aims:  Hepatitis E virus (HEV) in Bangladesh has not been adequately documented. We report HEV RNA and genotype detection in Bangladesh. Methods:  In total, 82 samples were used; 36 sporadic acute hepatitis (AH), 12 fulminant hepatitis (FH), 14 chronic liver disease (CLD) and 20 from an apparently healthy population (HP) positive for both immunoglobulin (Ig) M and IgG specific anti‐HEV antibodies (anti‐HEV). The male/female ratio was 61/21, ages 12–67 (mean 30.4) years. RNA was extracted, transcribed to cDNA and amplified in nt 6345–6490 (ORF2) of HEV. Nucleic and amino acid sequences were determined. Homology comparison between Bangladesh clones and other representative HEV clones and phylogenetic tree analyses were done. Relations between HEV RNA‐positivity and clinical factors were analyzed. Results:  HEV RNA was positive in 9/36 (25.0%) of AH cases, 4/12 (33.3%) FH, 3/14 (21.4%) CLD and 0/20 (0%) HP samples; total 16/82 (19.5%). Four factors correlated significantly with HEV RNA‐positivity (Mann‐Whitney U test); alanine aminotransferase (ALT) (P = 0.0229), aspartate aminotransferase (AST) (P = 0.0448), and titers of IgG (P = 0.0208) and IgM (P = 0.0095) specific anti‐HEV. The 16 HEV clones were divided mainly into two groups, A and B, including six different cDNA sub‐groups. Conclusion:  HEV RNA was found in sporadic AH and FH and sub‐clinical CLD cases, but not in HP. HEV RNA‐positivity was significantly related to values of ALT and AST and titers of IgG and IgM specific anti‐HEV, with IgM specific anti‐HEV showing the most significant relationship. All clones were genotype I, which is prevalent in South Asia.
ISSN:0815-9319
1440-1746
DOI:10.1111/j.1440-1746.2008.05677.x