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终末(干热)热处理对凝血因子浓缩物中非包膜病毒的影响。

Effect of terminal (dry) heat treatment on non-enveloped viruses in coagulation factor concentrates.

作者信息

Hart H F, Hart W G, Crossley J, Perrie A M, Wood D J, John A, McOmish F

机构信息

Protein Fractionation Centre, Scottish Blood Transfusion Service, Edinburgh, UK.

出版信息

Vox Sang. 1994;67(4):345-50. doi: 10.1111/j.1423-0410.1994.tb01271.x.

Abstract

Terminal dry heat treatment effectively inactivated hepatitis A virus (HAV) and canine parvovirus added to high-purity factor VIII. After 24 h at 80 degrees C, HAV infectivity was reduced by > or = 4.3 log10 TCID50, as measured in a newly developed infectivity assay. The same reduction in virus titer was achieved after 2 h and before 6 h at 90 degrees C. Inactivation of hepatitis A virus was also seen in the freeze-drying step prior to heat treatment with an approximately 2.0 log10 reduction in titer. Similar results were obtained with a high-purity factor IX concentrate. Canine parvovirus was also inactivated at both temperatures, with residual infectivity being undetected after 48 h at 80 degrees C or 10 h at 90 degrees C. Canine parvovirus was not affected by lyophilisation. Canine parvovirus measurements by PCR did not reflect the levels of infectivity measured by the tissue-culture-based method. The addition of the terminal dry heat treatment to solvent/detergent could effectively eliminate the potential contamination of solvent/detergent-treated coagulation factor concentrates by non-lipid-enveloped viruses. However, careful evaluation for any increased induction of non-antigens for factor VIII, as a consequence of such treatment, is needed before use in patients can be recommended.

摘要

终末干热处理能有效灭活添加到高纯度凝血因子 VIII 中的甲型肝炎病毒(HAV)和犬细小病毒。在 80℃下处理 24 小时后,通过一种新开发的感染性测定法测得,HAV 感染力降低了≥4.3 log10 TCID50。在 90℃下处理 2 小时至 6 小时后,病毒滴度也有相同程度的降低。在热处理前的冻干步骤中也观察到甲型肝炎病毒的灭活,滴度降低约 2.0 log10。高纯度凝血因子 IX 浓缩物也得到了类似结果。犬细小病毒在这两个温度下也被灭活,在 80℃下处理 48 小时或 90℃下处理 10 小时后未检测到残留感染力。犬细小病毒不受冻干影响。通过 PCR 检测犬细小病毒无法反映基于组织培养法测得的感染性水平。在溶剂/去污剂处理基础上增加终末干热处理,可有效消除溶剂/去污剂处理的凝血因子浓缩物被非包膜病毒污染的可能性。然而,在推荐用于患者之前,需要仔细评估这种处理是否会增加 VIII 因子非抗原的诱导。

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