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横断面评估循环乙型肝炎病毒 RNA 和 DNA:不同准种?

Cross-sectional evaluation of circulating hepatitis B virus RNA and DNA: Different quasispecies?

机构信息

Clinical Biochemistry Research Group, Department of Biochemistry, Vall d'Hebron Institut Recerca-Hospital Universitari Vall d'Hebron, Universitat Autònoma de Barcelona, Barcelona 08035, Spain.

Centro de Investigación Biomédica en Red de Enfermedades Hepáticas y Digestivas, Instituto de Salud Carlos III, Madrid 28029, Spain.

出版信息

World J Gastroenterol. 2021 Nov 7;27(41):7144-7158. doi: 10.3748/wjg.v27.i41.7144.

Abstract

BACKGROUND

Different forms of pregenomic and other hepatitis B virus (HBV) RNA have been detected in patients' sera. These circulating HBV-RNAs may be useful for monitoring covalently closed circular DNA activity, and predicting hepatitis B e-antigen seroconversion or viral rebound after nucleos(t)ide analog cessation. Data on serum HBV-RNA quasispecies, however, is scarce. It is therefore important to develop methodologies to thoroughly analyze this quasispecies, ensuring the elimination of any residual HBV-DNA. Studying circulating HBV-RNA quasispecies may facilitate achieving functional cure of HBV infection.

AIM

To establish a next-generation sequencing (NGS) methodology for analyzing serum HBV-RNA and comparing it with DNA quasispecies.

METHODS

Thirteen untreated chronic hepatitis B patients, showing different HBV-genotypes and degrees of severity of liver disease were enrolled in the study and a serum sample with HBV-DNA > 5 Log IU/mL and HBV-RNA > 4 Log copies/mL was taken from each patient. HBV-RNA was treated with DNAse I to remove any residual DNA, and the region between nucleotides (nt) 1255-1611 was amplified using a 3-nested polymerase chain reaction protocol, and analyzed with NGS. Variability/conservation and complexity was compared between HBV-DNA and RNA quasispecies.

RESULTS

No HBV-DNA contamination was detected in cDNA samples from HBV-RNA quasispecies. HBV quasispecies complexity showed heterogeneous behavior among patients. The Rare Haplotype Load at 1% was greater in DNA than in RNA quasispecies, with no statistically significant differences ( = 0.1641). Regarding conservation, information content was equal in RNA and DNA quasispecies in most nt positions [218/357 (61.06%)]. In 102 of the remaining 139 (73.38%), HBV-RNA showed slightly higher variability. Sliding window analysis identified 4 hyper-conserved sequence fragments in each quasispecies, 3 of them coincided between the 2 quasispecies: nts 1258-1286, 1545-1573 and 1575-1604. The 2 hyper-variable sequence fragments also coincided: nts 1311-1344 and 1461-1485. Sequences between nts 1519-1543 and 1559-1587 were only hyper-conserved in HBV-DNA and RNA, respectively.

CONCLUSION

Our methodology allowed analyzing HBV-RNA quasispecies complexity and conservation without interference from HBV-DNA. Thanks to this, we have been able to compare both quasispecies in the present study.

摘要

背景

已在患者血清中检测到不同形式的前基因组和其他乙型肝炎病毒 (HBV) RNA。这些循环 HBV-RNA 可能有助于监测共价闭合环状 DNA 活性,并预测乙型肝炎 e 抗原血清学转换或核苷(酸)类似物停药后的病毒反弹。然而,关于血清 HBV-RNA 准种的数据很少。因此,开发彻底分析这种准种的方法非常重要,以确保消除任何残留的 HBV-DNA。研究循环 HBV-RNA 准种可能有助于实现 HBV 感染的功能性治愈。

目的

建立一种用于分析血清 HBV-RNA 的下一代测序 (NGS) 方法,并将其与 DNA 准种进行比较。

方法

本研究纳入了 13 名未经治疗的慢性乙型肝炎患者,这些患者具有不同的 HBV 基因型和不同程度的肝病严重程度,从每位患者中采集 HBV-DNA>5 Log IU/mL 和 HBV-RNA>4 Log 拷贝/mL 的血清样本。用 DNAse I 处理 HBV-RNA 以去除任何残留的 DNA,然后使用 3 个嵌套聚合酶链反应方案扩增核苷酸 (nt) 1255-1611 之间的区域,并进行 NGS 分析。比较 HBV-DNA 和 RNA 准种之间的变异性/保守性和复杂性。

结果

从 HBV-RNA 准种的 cDNA 样本中未检测到 HBV-DNA 污染。HBV 准种复杂性在患者之间表现出异质性行为。1%稀有单倍型负荷在 DNA 中大于 RNA 准种,但无统计学差异 ( = 0.1641)。关于保守性,在大多数 nt 位置 [218/357(61.06%)],RNA 和 DNA 准种的信息含量相等。在其余 139 个中的 102 个 (73.38%),HBV-RNA 显示出略高的变异性。滑动窗口分析在每个准种中确定了 4 个超保守序列片段,其中 3 个在 2 个准种中都存在:nt 1258-1286、1545-1573 和 1575-1604。2 个超可变序列片段也吻合:nt 1311-1344 和 1461-1485。nt 1519-1543 和 1559-1587 之间的序列仅在 HBV-DNA 和 RNA 中分别超保守。

结论

我们的方法允许在没有 HBV-DNA 干扰的情况下分析 HBV-RNA 准种的复杂性和保守性。由于这个原因,我们能够在本研究中比较这两种准种。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4417/8613647/f2d0e7959ade/WJG-27-7144-g001.jpg

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