Optimization of roller culturing of influenza virus vaccine strains in MDCK and Vero cell cultures using plant origin components

E. I. Isaeva; N. A. Mazurkova; M. O. Skarnovich; G. P. Troshkova; L. N. Shishkina; R. Ya. Podchernyayeva

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Optimization of roller culturing of influenza virus vaccine strains in MDCK and Vero cell cultures using plant origin components

机译：使用植物来源成分优化在MDCK和Vero细胞培养中的流感病毒疫苗菌株的轮式培养

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Roller culturing of MDCK and Vero cells in an experimental nutrient medium based on soy flour hydrolysate, plant material obtained using the bromelain plant enzyme, was studied. The medium supplemented with 2 or 3% fetal calf serum (FCS) had a stronggrowth-stimulating effect on Vero and MDCK and cells, respectively, and did not alter the cell morphology. A/Solomon Islands/03/06 (H1N1) and B/Malaysia/2506/04 influenza vaccine viruses were grown on MDCK and Vero cell cultures obtained as a result of culturing in rollers on media containing soy flour hydrolysate and FCS (2 or 3%, respectively). The titer of the viruses was high in the presence of either trypsin (2 mu g/ml) or bromelain (20 mu g/ml).

机译：研究了在基于大豆粉水解物的实验营养培养基中滚轮培养MDCK和Vero细胞的过程，大豆粉水解物是使用菠萝蛋白酶植物酶获得的植物材料。补充有2％或3％胎牛血清（FCS）的培养基分别对Vero和MDCK和细胞具有强烈的促生长作用，并且不会改变细胞形态。 A / Solomon Islands / 03/06（H1N1）和B / Malaysia / 2506/04流感疫苗病毒在MDCK和Vero细胞培养物中生长，这种培养物是通过在含有大豆粉水解产物和FCS的培养基（2或3）上滚轮培养而获得的％，分别）。在胰蛋白酶（2微克/毫升）或菠萝蛋白酶（20微克/毫升）存在下，病毒的滴度很高。

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《Applied biochemistry and microbiology》 |2011年第8期|共7页
作者
E. I. Isaeva; N. A. Mazurkova; M. O. Skarnovich; G. P. Troshkova; L. N. Shishkina; R. Ya. Podchernyayeva;
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正文语种 eng
中图分类微生物学;
关键词
bromelain; influenza virus; soy flour hydrolysate; cultural vaccine; MDCK and Vero cell cultures; roller;

机译：菠萝蛋白酶;流感病毒;大豆粉水解产物;培养疫苗;MDCK和Vero细胞培养;滚轴;

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1. Optimization of roller culturing of influenza virus vaccine strains in MDCK and Vero cell cultures using plant origin components [J] . E. I. Isaeva, N. A. Mazurkova, M. O. Skarnovich, Applied biochemistry and microbiology . 2011,第8期

机译：使用植物来源成分优化在MDCK和Vero细胞培养中的流感病毒疫苗菌株的轮式培养
2. An MDCK Cell Culture-Derived Formalin-Inactivated Influenza Virus Whole-Virion Vaccine from an Influenza Virus Library Confers Cross-Protective Immunity by Intranasal Administration in Mice [J] . Ahmad M. Haredy, Nobuyuki Takenaka, Hiroshi Yamada, Clinical and vaccine immunology: CVI . 2013,第7期

机译：MDCK细胞培养衍生的福尔马林灭活的流感病毒全病毒疫苗从流感病毒库通过鼻内给药给予小鼠交叉保护性免疫
3. MDCK cell-cultured influenza virus vaccine protects mice from lethal challenge with different influenza viruses [J] . Liu K., Yao Z., Zhang L., Applied Microbiology and Biotechnology . 2012,第5期

机译：MDCK细胞培养的流感病毒疫苗可保护小鼠免受不同流感病毒的致命攻击
4. SINGLE-CELL ANALYSIS OF INFLUENZA A VIRUS-INFECTED CELLS FOR THE OPTIMIZATION OF CELL CULTURE-BASED VACCINE PRODUCTION [C] . Sascha Young Kupke, Bioprocess Engineering, Timo Frensing, Vaccine technology VI . 2016

机译：流感病毒感染细胞的单细胞分析，用于优化基于细胞培养的疫苗生产
5. Replication of neurovirulent and non-neurovirulent human H1N1 influenza A viruses in mouse brain and nerve cell cultures: Virus strain-specific and host cell-dependent variations in progeny virus assembly,mRNA splicing efficiency, and expression of RNA gene segments 7 and 8 [D] . Husak, Paul James 1994

机译：在鼠脑和神经细胞培养物中复制神经毒力和非神经毒力的人类甲型H1N1流感病毒：子代病毒装配，mRNA剪接效率以及RNA基因片段7和8的表达中病毒株特异性和宿主细胞依赖性变异
6. Comparison of Madin-Darby canine kidney cells (MDCK) with a green monkey continuous cell line (Vero) and human lung embryonated cells (MRC-5) in the isolation of influenza A virus from nasopharyngeal aspirates by shell vial culture. [O] . J Reina, V Fernandez-Baca, I Blanco, 1997

机译：通过外壳瓶培养从鼻咽抽吸物中分离甲型流感病毒时将Madin-Darby犬肾细胞（MDCK）与绿猴连续细胞系（Vero）和人肺胚细胞（MRC-5）进行比较。
7. Comparison of Madin-Darby canine kidney cells (MDCK) with a green monkey continuous cell line (Vero) and human lung embryonated cells (MRC-5) in the isolation of influenza A virus from nasopharyngeal aspirates by shell vial culture [O] . J Reina, V Fernandez-Baca, I Blanco, 1997

机译：用绿色猴子连续细胞系（VERO）和人肺胚胎细胞（MRC-5）与壳体小瓶培养的流感病毒分离，将Madin-Darby犬肾细胞（MDCK）与人肺胚胎细胞（MRC-5）进行比较

Optimization of roller culturing of influenza virus vaccine strains in MDCK and Vero cell cultures using plant origin components

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