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Basic Characteristics of Mutations
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Mutation Site
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Y206H |
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Mutation Site Sentence
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Table 3 |
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Mutation Level
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Amino acid level |
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Mutation Type
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Nonsynonymous substitution |
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Gene/Protein/Region
|
S |
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Standardized Encoding Gene
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S
|
|
Genotype/Subtype
|
- |
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Viral Reference
|
U87742;M57663;D50522;D23678;D23680;M38636;AF151735;X02496;X75657;AB032431;AB091256;AY090455;X69798;AB064313;AF160501;AY090454;AB059659
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Functional Impact and Mechanisms
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Disease
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Hepatitis B Virus Infection
|
|
Immune
|
Y |
|
Target Gene
|
-
|
|
Clinical and Epidemiological Correlations
|
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Clinical Information
|
Y |
|
Treatment
|
- |
|
Location
|
Nigeria |
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Literature Information
|
|
PMID
|
26148052
|
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Title
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Occult Hepatitis B Virus Infection in Nigerian Blood Donors and Hepatitis B Virus Transmission Risks
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Author
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Oluyinka OO,Tong HV,Bui Tien S,Fagbami AH,Adekanle O,Ojurongbe O,Bock CT,Kremsner PG,Velavan TP
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Journal
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PloS one
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Journal Info
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2015 Jul 6;10(7):e0131912
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Abstract
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BACKGROUND: Occult hepatitis B virus infection (OBI) characterized by the absence of detectable HBsAg remains a potential threat in blood safety. We investigated the actual prevalence, viral factors and genotype of OBI infections in Nigerian blood donors. METHODS: Serum collected from two blood banks were reconfirmed as HBsAg seronegative by ELISA. Forty HBsAg positive samples were employed as controls. HBV-DNA was amplified from all donors and viral loads were determined using quantitative real-time PCR. Antibodies to the HBV core, surface and HBe antigen (anti-HBc,anti-HBs,HBeAg) were measured. The PreS/S and PreC/C regions of the HBV genome were sequenced. RESULTS: Of the 429 blood donors, 72(17%) were confirmed as OBI by DNA detection in different reference labs and excluded the concern of possible contamination. Of the 72 OBI samples, 48(67%) were positive for anti-HBc, 25(35%) positive for anti-HBs, and 2(3%) positive for HBeAg. Of the 72 OBI samples, 31(43%) were seropositive for either anti-HBc, anti-HBs or HBeAg, 21 (30%) positive for both anti-HBc and anti-HBs,one positive for both anti-HBc and HBeAg. None of the OBI samples were positive for all three serological markers. The viral load was <50copies/ml in the OBI samples and genotype E was predominant. The L217R polymorphism in the reverse transcriptase domain of the HBV polymerase gene was observed significantly higher in OBI compared with HBsAg positive individuals (P<0.0001). CONCLUSION: High incidence of OBI is relevant in high endemic areas worldwide and is a general burden in blood safety. This study signifies the high prevalence of OBI and proposes blood donor samples in Nigeria should be pre-tested for OBI by nucleic acid testing (NAT) and/or anti-HBc prior to transfusion to minimize the HBV infection risk.
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Sequence Data
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KT001260-KT001331;KT001332-KT001404
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