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污泥处理过程中病毒灭活的测定方法。

Method for determining virus inactivation during sludge treatment processes.

作者信息

Traub F, Spillmann S K, Wyler R

出版信息

Appl Environ Microbiol. 1986 Sep;52(3):498-503. doi: 10.1128/aem.52.3.498-503.1986.

Abstract

A simple and reliable method is described which allows determination of virus inactivation rates during sludge treatment processes in situ. Bacteriophage f2 was adsorbed onto an electropositive membrane filter which was then sandwiched between two polycarbonate membranes with pores smaller than the virus diameter. The resulting sandwich was fixed in an open filter holder, and several such devices were connected before being exposed in sludge-digesting tanks. The device described prevented uncontrolled virus escape, but allowed direct contact of the various inactivating or stabilizing substances present in the environment tested with the virus adsorbed to the carrier membrane. After exposure to an environment, the surviving fraction of virus was eluted from the inner filter and determined by plaque counting. By using polycarbonate membranes without pores for sandwiching, the influence of temperature alone on virus inactivation could be measured. Thermophilic fermentation at 60 degrees C and at 65 kPa pressure led to a bacteriophage f2 titer reduction of 3.5 log10 units per h, whereas during thermophilic digestion at 54.5 degrees C titers decreased 1.2 log10 units per h. During mesophilic digestion an inactivation rate of only 0.04 log10 units per h was observed. Under these latter conditions, temperature had only a minor effect (19%) on virus inactivation, whereas at 54.5 degrees C during thermophilic digestion heat accounted for 32% of the total inactivation, and during thermophilic fermentation at 60 degrees C temperature and pressure were 100% responsible for virus denaturation.

摘要

本文描述了一种简单可靠的方法,可原位测定污泥处理过程中的病毒灭活率。将噬菌体f2吸附到带正电的膜过滤器上,然后将其夹在两个孔径小于病毒直径的聚碳酸酯膜之间。将所得的夹层固定在开放式过滤器支架中,连接几个这样的装置后再暴露于污泥消化池中。所描述的装置可防止病毒不受控制地逸出,但能使测试环境中存在的各种灭活或稳定物质与吸附在载体膜上的病毒直接接触。暴露于某一环境后,从内部过滤器中洗脱存活的病毒部分,并通过噬菌斑计数进行测定。通过使用无孔的聚碳酸酯膜进行夹层,可以测量仅温度对病毒灭活的影响。在60℃和65kPa压力下进行嗜热发酵,导致噬菌体f2滴度每小时降低3.5个对数单位,而在54.5℃进行嗜热消化时,滴度每小时降低1.2个对数单位。在中温消化过程中,观察到的灭活率仅为每小时0.04个对数单位。在后者这些条件下,温度对病毒灭活的影响较小(19%),而在54.5℃嗜热消化过程中,热占总灭活量的32%,在60℃嗜热发酵过程中,温度和压力对病毒变性的贡献率为100%。

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