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用于检测阿昔洛韦耐药单纯疱疹病毒的改良DNA杂交方法

Improved DNA hybridization method for detection of acyclovir-resistant herpes simplex virus.

作者信息

Swierkosz E M, Scholl D R, Brown J L, Jollick J D, Gleaves C A

机构信息

Department of Pediatrics/Adolescent Medicine, St. Louis University School of Medicine, Missouri.

出版信息

Antimicrob Agents Chemother. 1987 Oct;31(10):1465-9. doi: 10.1128/AAC.31.10.1465.

Abstract

A simplified DNA hybridization method was developed to detect acyclovir-resistant isolates of herpes simplex virus. Herpes simplex virus-infected cell cultures in microtiter plates were treated with concentrations of acyclovir ranging from 8 to 0.015 micrograms/ml. At 48 h postinfection, infected cells were lysed by a one-step procedure and lysates were absorbed to membranes. Without further treatment, membranes were hybridized by using a herpes simplex virus-specific radioiodinated probe. The membranes were then washed and counted in a gamma counter. The elapsed time for assay performance was 4 h. Parallel plaque reduction assays were performed for comparison. The mean 50% inhibitory dose of in vivo- and in vitro-derived acyclovir-resistant, thymidine kinase-negative isolates was greater than 2 micrograms/ml by DNA hybridization. The 50% inhibitory dose of acyclovir-susceptible, thymidine kinase-positive isolates ranged from 0.01 to 1.1 micrograms/ml. This assay is simple and objective and should facilitate antiviral susceptibility testing in diagnostic laboratories.

摘要

开发了一种简化的DNA杂交方法来检测单纯疱疹病毒的阿昔洛韦耐药株。微量滴定板中感染单纯疱疹病毒的细胞培养物用浓度范围为8至0.015微克/毫升的阿昔洛韦处理。感染后48小时,通过一步法裂解感染细胞,裂解物吸附到膜上。无需进一步处理,使用单纯疱疹病毒特异性放射性碘化探针进行膜杂交。然后洗涤膜并在γ计数器中计数。测定过程的耗时为4小时。进行平行蚀斑减少试验以作比较。通过DNA杂交,体内和体外获得的阿昔洛韦耐药、胸苷激酶阴性分离株的平均50%抑制剂量大于2微克/毫升。阿昔洛韦敏感、胸苷激酶阳性分离株的50%抑制剂量范围为0.01至1.1微克/毫升。该检测方法简单且客观,应有助于诊断实验室进行抗病毒药敏试验。

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Phosphorylation of acyclovir diphosphate by cellular enzymes.阿昔洛韦二磷酸被细胞酶磷酸化。
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