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Plaque autoradiography assay for the detection and quantitation of thymidine kinase-deficient and thymidine kinase-altered mutants of herpes simplex virus in clinical isolates.

机译:斑块放射自显影分析法用于检测和定量临床分离株中单纯性疱疹病毒的胸苷激酶缺陷型和胸苷激酶改变的突变体。

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摘要

A plaque autoradiography assay to detect and quantitate thymidine kinase (TK) mutants of herpes simplex virus type 1 (HSV-1) and HSV-2 in clinical samples is described. This method utilizes the selective incorporation of [125I]iododeoxycytidine, a pyrimidine analog selectively phosphorylated by the HSV TK. Only cells infected with TK-competent virus will efficiently incorporate iododeoxycytidine and are the only cells detected by autoradiography. Furthermore, this assay discriminates between TK+ virus (TK competent) and TKA virus (TK altered or reduced). This ability to differentiate TK+ from TKA virus is enhanced when infected cells are labeled with [14C]thymidine in tandem with iododeoxycytidine labeling. Reconstruction experiments with mixtures of TK+ (HSV-1 Patton) virus and TK-deficient (TK-) (B2006) or TKA (IUDRr) mutants were performed to determine the limits of detection of this technique. Ten percent TK- or TKA virus was the lower limit for the detection of TK mutants in a mixed population, whereas 1 in 1,000 TK+ virus revertants could be detected in a TK- virus population. In reconstructed populations and 45 clinical samples, a good correlation existed between the increase in 50% inhibitory dose for acyclovir and the percent TK mutant virus present. Similarly, the results of this technique correlated well with the acyclovir phosphorylating activity of extracts from cells infected with isolates or reconstructed mixtures. Plaque autoradiography with [125I]iododeoxycytidine was able to distinguish mixed populations of TK+ and TK- virus and homogeneous populations of TKA virus. The tandem use of [125I]iododeoxycytidine and [14C]thymidine readily identified TKA virus, which appeared as TK+ virus when labeled with [14C]thymidine alone. This technique provides a sensitive screen for antiviral resistance due to alterations in the viral TK and can be used to analyze clinical samples.
机译:描述和检测临床样本中单纯疱疹病毒1型(HSV-1)和HSV-2的胸苷激酶(TK)突变体的噬菌体放射自显影测定法。该方法利用了由HSV TK选择性磷酸化的嘧啶类似物[125I]碘脱氧胞苷的选择性掺入。只有感染了TK的病毒感染的细胞才能有效地掺入碘脱氧胞苷,并且是放射自显影检测到的唯一细胞。此外,该测定法还可以区分TK +病毒(可胜任TK)和TKA病毒(可改变或减少TK)。当用碘代脱氧胞苷标记的[14C]胸腺嘧啶核苷标记感染的细胞时,增强了将TK +与TKA病毒区分开的能力。进行了TK +(HSV-1 Patton)病毒和TK-缺陷(TK-)(B2006)或TKA(IUDRr)突变体混合物的重建实验,以确定该技术的检测范围。在混合人群中检测TK突变体的下限是TK-或TKA病毒的百分数是下限,而在TK-病毒人群中可以检测到千分之一的TK +病毒回复株。在重建的人群和45个临床样本中,阿昔洛韦50%抑制剂量的增加与所存在的TK突变病毒百分比之间存在良好的相关性。同样,这项技术的结果与被分离株或重组混合物感染的细胞提取物的阿昔洛韦磷酸化活性密切相关。用[125I]碘代脱氧胞苷进行的放射自显影能够区分TK +和TK-病毒的混合种群和TKA病毒的均匀种群。串联使用[125I]碘脱氧胞苷和[14C]胸苷很容易鉴定出TKA病毒,当单独用[14C]胸苷标记时,它以TK +病毒的形式出现。该技术为病毒TK的变化提供了抗病毒耐药性的灵敏筛选,可用于分析临床样品。

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