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针对丙型肝炎病毒2-6型与丙型肝炎病毒国际标准品96/790(1型)进行校准的协作研究。

Collaborative study to calibrate hepatitis C virus genotypes 2-6 against the HCV International Standard, 96/790 (genotype 1).

作者信息

Saldanha J, Heath A

机构信息

Division of Virology, National Institute for Biological Standards and Control, South Mimms, Herts., UK.

出版信息

Vox Sang. 2003 Jan;84(1):20-7. doi: 10.1046/j.1423-0410.2003.00260.x.

Abstract

BACKGROUND AND OBJECTIVES

A major requirement of a hepatitis C virus (HCV) RNA nucleic acid amplification technology (NAT) assay validation is the ability of the assay to detect the six major genotypes of HCV with equivalent sensitivities. The aim of this study was to characterize and calibrate an HCV genotype panel for use in such studies.

MATERIALS AND METHODS

Panels consisting of the first International Standard (IS) for HCV RNA NAT assays (96/790; HCV genotype 1a) and isolates of genotypes 2-6 were sent to 17 laboratories worldwide which use a variety of NAT tests, both qualitative and quantitative. The HCV RNA content of each panel member was determined and the mean titre calculated in International Units/ml (IU/ml).

RESULTS

The calculated mean titres (calibrated against the HCV International Standard), in log10 IU/ml, of the genotype 2-6 samples were 3.99, 3.81, 4.14, 4.18 and 4.61, respectively.

CONCLUSIONS

An HCV genotype panel, calibrated in IU/ml, has been established and should be valuable for assay validation. All the genotypes were detected by all the assays used, but it was not possible to demonstrate that the genotypes were detected with equal efficiencies.

摘要

背景与目的

丙型肝炎病毒(HCV)RNA核酸扩增技术(NAT)检测方法验证的一项主要要求是该检测方法能够以同等灵敏度检测HCV的六种主要基因型。本研究的目的是鉴定和校准用于此类研究的HCV基因型标准品。

材料与方法

由首个HCV RNA NAT检测国际标准品(96/790;HCV 1a基因型)以及2至6型基因型分离株组成的标准品被送往全球17个实验室,这些实验室使用各种定性和定量的NAT检测方法。测定每个标准品成员的HCV RNA含量,并计算以国际单位/毫升(IU/ml)表示的平均滴度。

结果

2至6型基因型样本以log10 IU/ml为单位计算的平均滴度(相对于HCV国际标准品校准)分别为3.99、3.81、4.14、4.18和4.61。

结论

已建立了以IU/ml校准的HCV基因型标准品,这对于检测方法验证应具有重要价值。所有使用的检测方法都能检测到所有基因型,但无法证明各基因型的检测效率相同。

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