| 核黄素联合紫外线A照射对血浆中伪狂犬病毒的灭活效果 |
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| 引用本文: | 聂咏梅,张晓敏,周豪杰,付涌水,江朝富,汪传喜,陶黎阳,张甜,曹开源,田小东. 核黄素联合紫外线A照射对血浆中伪狂犬病毒的灭活效果[J]. 中国输血杂志, 2007, 20(5): 361-364 |
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| 作者姓名: | 聂咏梅 张晓敏 周豪杰 付涌水 江朝富 汪传喜 陶黎阳 张甜 曹开源 田小东 |
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| 作者单位: | 1. 广州血液中心,广东广州,510095
2. 中山大学临床检验标准化研究中心 |
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| 基金项目: | 广东省医学科学技术研究基金;广东省广州市医药卫生科技基金 |
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| 摘 要: | 目的考察核黄素联合紫外线A对血浆中伪狂犬病毒的灭活效果。方法以伪狂犬病毒为模拟病毒,以Vero细胞为培养细胞,用病毒感染细胞,制备病毒增殖液;分别采用5、10、15及20J/cm2联合核黄素处理血浆,观察处理前后血浆病毒灭活的效果,筛选灭活病毒合适的紫外线剂量;将含有伪狂犬病毒血浆的样本分为实验组:采用上述筛选的紫外线强度照射联合核黄素处理;对照组1:单独采用紫外线A照射;对照组2:单独采用核黄素处理;阴性对照组:未采用紫外线照射和核黄素处理;分别在实验前后采用96孔细胞病变法,对照细胞病变效应,根据Reed-Muench公式计算病毒滴度。结果采用不同强度的紫外线联合核黄素处理血浆,紫外线强度为15及20J/cm2的灭活血浆病毒的效果明显,处理后病毒滴度分别下降4.55和4.39logs;实验组和对照组1病毒滴度分别下降4.55和4.28logs,有统计学意义(P<0.05);对照组2病毒滴度降低1.93logs,没有病毒灭活效果。结论核黄素联合紫外线可灭活血浆中伪狂犬病毒,单独紫外线照射也具有灭活血浆伪狂犬病毒的效果;而仅单独采用核黄素处理而未联合紫外线照射,对血浆中伪狂犬病毒灭活效果不明显。
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| 关 键 词: | 病毒灭活 血浆 核黄素 紫外线A 模拟病毒 伪狂犬病毒 Vero细胞 |
| 文章编号: | 1004-549X(2007)05-0361-04 |
| 收稿时间: | 2006-12-04 |
| 修稿时间: | 2007-09-18 |
Inactivation of pseudorabies virus in plasma using riboflavin and ultraviolet light |
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| Nie Yongmei . Zhang Xiaomin , Zhou Haojie ,et al.. Inactivation of pseudorabies virus in plasma using riboflavin and ultraviolet light[J]. Chinese Journal of Blood Transfusion, 2007, 20(5): 361-364 |
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| Authors: | Nie Yongmei . Zhang Xiaomin Zhou Haojie et al. |
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| Affiliation: | 1. Guangzhou Blood Center, Guangzhou 510095,China 2. Research Center of Clinical Laboratory Standard, Sun Yat-sen University |
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| Abstract: | Objective To study the inactivation efficiency of riboflavin and ultraviolet A light (UV-A. 320 ~ 400nm) on pseudorabies virus in plasma. Methods Pseudorabies virus were cultured with Vero cells, and Riboflavin was added into plasma with a final concentration of 50 μmol/L. and then exposed to ultraviolet A at 5,10,15 and 20J/ cm2 UV-A for 30 minutes, respectively, to chose the optimal dose of UV-A exposure. Then 4 groups, each group with 5ml plasma mixed with 10 μl virus-infected Vero cells, were assigned as follows: experimental group: underwent UV-A exposure at 15J/cm2 for 30 minutes with Riboflavin at a concentration of 50 μmol/Ls control group 1: 15J/cm2 UV-A exposure for 30 minutes without riboflavin; control group 2: use riboflavin of 50 μmol/L only without UV-A exposure; negative control group: neither UV-A exposure nor riboflavin treatment was used. Virus titer was measured by TC1D50, and the changes of the titer throughout the inactivation were analyzed statistically. Results UV-A exposure at 15 and 20J/cm2 for 30 minutes with riboflavin of 50 μmol/L were effective in inactivation, and the virulence of pseudorabies virus drop 4. 55 and 4. 39 logs, respectively. The viral virulence of experimental group was reduced by 4. 55 logs, and control group 1 by 4. 28 logs, while control group 2 didn't achieve the inactivation efficacy expected. Conclusion Both the combination of riboflavin and UV-A light, and UV-A treatment only could effectivelyinactivate pseudorabies virus in plasma. But the use of riboflavin only couldn't achieve effective inactivation. |
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| Keywords: | Riboflavin Ultraviolet A Plasma Pseudorabies virus |
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