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检测人类III型嗜T细胞淋巴细胞病毒/淋巴结病相关病毒逆转录酶的微量方法

Micromethod for assaying reverse transcriptase of human T-cell lymphotropic virus type III/lymphadenopathy-associated virus.

作者信息

Spira T J, Bozeman L H, Holman R C, Warfield D T, Phillips S K, Feorino P M

出版信息

J Clin Microbiol. 1987 Jan;25(1):97-9. doi: 10.1128/jcm.25.1.97-99.1987.

Abstract

A micromethod for assaying the reverse transcriptase enzyme of human T-cell lymphotropic virus type III/lymphadenopathy-associated virus in cocultures of clinical specimens for viral isolation was developed and compared with the macromethod in use. Ultracentrifuged, pelleted, and solubilized viral culture supernatants were transferred into either tubes (macromethod) or microtiter plates (micromethod) and incubated with tritiated enzyme substrate. Trichloroacetic acid-precipitated DNA was collected on individual filter papers with a Millipore filtration manifold (macromethod) or on filter sheets using a semiautomated cell harvester (micromethod). Filters were then placed in scintillation fluid and counted on a beta scintillation counter. Results of the micromethod significantly correlated to those of the macromethod, with a linear relationship between the two. The cutoffs for positivity based on the mean + 2 standard deviations for a set of known negative specimens (n = 19) was 4,973 cpm for the micromethod compared with 5,336 for the macromethod. The intrarun and interrun variations were comparable for both methods. There was a 67% increase in the maximal daily number of specimens which could be run (100 versus 60) as well as a reduction in reagent use. In summary, the micromethod utilizing a semiautomated cell harvester is comparable to the existing macromethod in accuracy and is an improvement due to savings in time and reagents.

摘要

开发了一种用于在临床标本共培养物中检测人类Ⅲ型嗜T细胞淋巴病毒/淋巴结病相关病毒逆转录酶的微量方法以进行病毒分离,并与现行的常量方法进行比较。将超速离心、沉淀并溶解的病毒培养上清液转移至试管(常量方法)或微量滴定板(微量方法)中,与氚化酶底物一起孵育。用密理博过滤歧管在单独的滤纸上收集三氯乙酸沉淀的DNA(常量方法),或使用半自动细胞收集器在滤纸上收集(微量方法)。然后将滤纸置于闪烁液中,用β闪烁计数器计数。微量方法的结果与常量方法的结果显著相关,二者呈线性关系。基于一组已知阴性标本(n = 19)的平均值 + 2个标准差确定的阳性临界值,微量方法为4973 cpm,常量方法为5336 cpm。两种方法的批内和批间变异相当。可检测的每日标本最大数量增加了67%(从60份增加到100份),同时试剂用量减少。总之,使用半自动细胞收集器的微量方法在准确性上与现有的常量方法相当,并且由于节省时间和试剂而有所改进。

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