Detection of hepatitis B virus genotypes in a group of hepatitis B virus-infected patients in central and northern Sri Lanka.

Access microbiology Pub Date : 2024-10-03 eCollection Date: 2024-01-01 DOI:10.1099/acmi.0.000838.v3
T T Pattiyakumbura, K G K Malkanthi, W K H Dheerasekara, A Manamperi, M A R V Muthugala
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Abstract

Introduction. Hepatitis B infection causes a spectrum of clinical diseases varying from asymptomatic infection to severe or fulminant acute hepatitis, chronic liver disease, cirrhosis and hepatocellular carcinoma. Hepatitis B virus (HBV) genotypes appear to influence transmission dynamics, clinical outcomes and responses to antiviral therapy. However, hepatitis B genotyping has been poorly investigated in Sri Lanka. This study intended to determine hepatitis B genotypes in a group of HBV-infected people in central and northern Sri Lanka. Methodology. The study was a laboratory-based descriptive cross-sectional study. Initial detection of HBV DNA in 100 EDTA blood samples was done by using a commercially validated quantitative real-time PCR kit. Hepatitis B genotyping was performed by in-house conventional semi-nested multiplex PCR using genotype-specific primers (for genotypes A-F). The serological profile was determined using a commercially validated ELISA/chemiluminescence immunoassay. The results were evaluated for genotype prevalence, viral load association and hepatitis B e antigen (HBeAg) expression in the study population. Results and conclusion. The study detected that genotype C (n=38) is most prevalent and infections with multiple genotypes (n=52, 52%) were commoner than mono-genotype (n=23, 23%) infections. In total, 25% of patients had no detectable genotype among genotypes A-F. The mean viral load in asymptomatic patients with a single genotype was 3.28 log10 copies ml-1 and in multiple genotypes was 4.18 log10 copies ml-1 before treatment. Statistical significance was not detected in mean viral loads and HBeAg expression in these two groups. In the future, chronic HBV infection may be effectively treated and managed according to the infected genotype.

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在斯里兰卡中部和北部一组乙型肝炎病毒感染者中检测乙型肝炎病毒基因型。
导言。乙型肝炎感染会导致一系列临床疾病,从无症状感染到严重或暴发性急性肝炎、慢性肝病、肝硬化和肝细胞癌。乙型肝炎病毒(HBV)基因型似乎会影响传播动态、临床结果和对抗病毒治疗的反应。然而,斯里兰卡对乙型肝炎基因分型的调查却很少。本研究旨在确定斯里兰卡中部和北部一组乙型肝炎病毒感染者的乙型肝炎基因型。研究方法。本研究是一项基于实验室的描述性横断面研究。使用经过商业验证的定量实时 PCR 试剂盒对 100 份 EDTA 血液样本中的 HBV DNA 进行初步检测。乙型肝炎基因分型是通过使用基因型特异性引物(针对基因型 A-F)的内部常规半嵌套多重 PCR 技术进行的。血清学特征采用经商业验证的 ELISA/化学发光免疫测定法进行测定。对研究人群的基因型流行率、病毒载量相关性和乙肝 e 抗原(HBeAg)表达进行了评估。结果和结论。研究发现,基因型 C(38 人)最为流行,多基因型感染(52 人,占 52%)比单基因型感染(23 人,占 23%)更为常见。在 A-F 基因型中,共有 25% 的患者检测不到基因型。治疗前,单基因型无症状患者的平均病毒载量为 3.28 log10 copies ml-1,多基因型患者的平均病毒载量为 4.18 log10 copies ml-1。这两组患者的平均病毒载量和 HBeAg 表达均无统计学意义。未来,慢性 HBV 感染可根据感染的基因型得到有效的治疗和管理。
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