Prevention and Nursing of Adverse Reactions of Novel Coronavirus Inactivated Vaccine (Vero Cells)

Objective:To discuss and analyze the causes of adverse reactions caused by the inactivated novel coronavirus vaccine(Vero cells),and to propose methods of prevention and care.Methods:A questionnaire was used to randomly select 229 adults who were vaccinated with the inactivated novel coronavirus vaccine(Vero cells)at Xi’an People’s Hospital(Xi’an Fourth Hospital).The adverse reactions were statistically analyzed.Results:Among the 229 adults vaccinated with the inactivated novel coronavirus vaccine(Vero cells),30 experienced vaccination reactions.The main reaction was local induration at the inoculation site,and dizziness was the primary systemic symptom.Conclusion:To reduce the incidence of adverse reactions to the inactivated novel coronavirus vaccine(Vero cells),it is necessary to effectively evaluate the health status of adults before vaccination,select the correct vaccination site,and strictly implement the rules of 3-inspections,7-checks,and 1-verification.Standardizing the operation process and providing thorough health education after vaccination can effectively reduce the occurrence of adverse reactions.

1株悬浮培养的Vero细胞驯化及其生物学特性研究

目的 将贴壁培养的Vero细胞驯化成悬浮培养细胞,并对其生物学特性进行研究。方法 采用无血清培养和“摇床适应法”对细胞进行培养优化,对其进行成瘤性、短串联重复序列(short tandem repeat,STR)分析、透射电子显微镜形态,以及对流感病毒敏感性检测。结果 成功建立悬浮细胞系Vero-S,Vero-S细胞生长期在24~72 h,平台期在108~144h之间,衰退期在144h以后,细胞PDT为36 h,细胞密度在14.01~14.88×10^(8)个/L之间,细胞平均圆度在0.73~0.75之间,细胞直径在12.12~14.44μm之间。Vero-S细胞在裸鼠皮下形成肿瘤,而悬浮培养前的Vero细胞不具有成瘤性;STR显示为猴源细胞系;电镜下细胞结构完整;Vero-S细胞对流感病毒感染不敏感。结论 悬浮细胞系Vero-S细胞的生长经历与贴壁细胞类似的生长期、平台期、衰退期,且细胞大小均一,建立的悬浮培养基能够支持Vero-S细胞高密度生长。STR结果表明悬浮Vero细胞具有完全的遗传稳定性,透射电镜下与贴壁Vero细胞无明显区别。为细胞悬浮驯化培养技术提供参考价值,并可用于细胞致肿瘤的机理研究。

新型冠状病毒灭活疫苗(Vero细胞)内毒素检查方法比较

目的为新型冠状病毒(简称新冠病毒)灭活疫苗(Vero细胞)的细菌内毒素检查和质量控制提供技术支持和理论基础。方法利用凝胶法、光度测定法[包括动态浊度(TKA)法、微量动态显色(mKCA)法]测定并比较新冠病毒灭活疫苗(Vero细胞)原液和成品中内毒素浓度。结果3种方法测得的供试品内毒素浓度均符合规定(原液为不超过5 EU/600 SU,成品为每剂≤5 EU),且后2种方法既能用于定性检测也能用于定量检测,特别是mKCA法下鲎试剂用量更少。结论mKCA法是检查该疫苗内毒素浓度的最适宜方法,具有灵敏度高、稳定性强、鲎试剂用量少、数据完整和可追溯、人为操作误差较小的特点。

慢病毒介导稳定表达增强小反刍兽疫病毒复制的山羊Vero/SLAM细胞系的建立

利用Gateway技术和慢病毒表达系统将山羊淋巴细胞信号活化因子SLAM稳定整合在Vero细胞基因组染色体上,建立稳定表达可增强小反刍兽疫病毒(PPRV)复制的SLAM的Vero阳性细胞亚克隆,并验证阳性细胞亚克隆Vero/SLAM表达SLAM的活性、遗传稳定性及其对PPRV复制的增殖效果。分离山羊外周血淋巴细胞,提取基因组Total RNA,一步RT-PCR获得完整ORF的SLAM基因,采用BP及LR位点的基因重组技术,构建入门载体pDONR/SLAM并获得表达骨架pDEST/SLAM,与Packaging Mix pLP1、pLP2及VSV-G共转染293-FT细胞,获得SLAM复制缺陷型慢病毒样粒子,用其感染Vero细胞,杀稻瘟菌素抗性筛选获得阳性细胞克隆,通过靶标基因扩增、间接免疫荧光、激光扫描共聚焦显微技术、Western blot免疫印迹检测技术、致细胞病变效应及Realtime RT-PCR等技术分别验证SLAM基因组整合、转录,SLAM蛋白表达、反应活性以及PPRV在表达SLAM阳性细胞亚克隆上的增殖效果。结果显示:SLAM受体基因被稳定整合在Vero细胞基因组染色体上,该受体蛋白表达于细胞周质,建立的细胞连续传代不丢失,接种病毒后致细胞病变时间由4～7d缩短为3.5d,TCID_(50)·0.1mL^(-1)由4.25增加为5.67,相对于正常Vero细胞,整合有SLAM的Vero细胞,由于表达了PPRV特异的细胞受体使PPRV对其易感性显著增强。成功建立一株稳定表达靶向增强PPRV复制的Vero/SLAM细胞:该细胞表达的SLAM具有明显增强PPRV复制的功能,不仅可以从细胞模型水平阐明增强PPRV复制的关键靶基因,也为PPRV感染引起宿主细胞的变化以及对机体的致病机制等提供研究工具。

稳定表达山羊SLAM受体的Vero细胞系的建立

信号淋巴激活分子(signalling lymphocyte activation molecule,SLAM)又称CD150,是小反刍兽疫病毒(peste des petits ruminants virus,PPRV)和犬瘟热病毒(canine distemper virus,CDV)等麻疹病毒属病毒感染淋巴细胞的主要受体,在病毒侵入细胞中发挥着重要作用。为了建立稳定表达山羊SLAM真核细胞系,本研究将全基因合成的gSLAM基因克隆至真核表达质粒pIRES2-GFP中,构建了重组质粒pIRES2-gSLAM。将该重组质粒转染非洲绿猴肾细胞(Vero),经G418筛选后,筛选到稳定表达gSLAM基因的细胞系Vero-gSLAM,该细胞系在传代至第10代,仍能稳定表达gSLAM基因,PPRV N75/1病毒株可以感染且能形成明显的细胞病变(CPE),相比在Vero细胞上10-4.65 TCID50/0.1mL的毒价,在Vero-gSLAM上为10-5.75 TCID50/0.1mL,其毒价有所提高。该细胞系可用于PPRV强毒分离和致弱机制等相关研究。

稳定表达犬瘟热病毒基质蛋白的细胞系Vero-SLAM-M的构建

为了建立稳定表达犬瘟热病毒基质蛋白(M)的细胞系,从犬瘟热病毒狐狸源分离毒株SD16F中扩增出M基因,将其克隆至真核表达质粒pCI-neo的Xho I/Not I位点处。重组质粒经PCR、Xho I/Not I双酶切及测序鉴定后转染Vero-SLAM细胞,利用G418抗性压力筛选阳性细胞,并采用RT-PCR及间接免疫荧光试验(IFA)鉴定转染细胞中M蛋白的表达情况。结果表明,成功构建了重组质粒pCI-neo-M,瞬时及稳定转染Vero-SLAM细胞后,RT-PCR和IFA能够检测到M基因的转录和表达,且G418筛选后细胞与其亲本Vero-SLAM细胞生长特性基本一致,表明获得1株能稳定表达M蛋白的细胞系,命名为Vero-SLAM-M。

Screening of a High Growth Influenza B Virus Strain in Vero Cells

Due to the insufficient supply of embryonated chicken eggs,the preparation of large quantities of inactivated influenza vaccines will require an alternative virus culture system after the emergence or reemergence of a pandemic influenza virus.The Vero cell is one of the ideal options since it was used for producing many kinds of human vaccines.However,most of the influenza viruses can not grow well in Vero cells.To develop a new influenza vaccine with Vero cells as a substrate,the virus needs to adapt to this cell substrate to maintain high growth characteristics.By serial passages in Vero cells,the B/Yunnan/2/2005va(B)strain was successfully adapted to Vero cells,with the hemagglutination titer(HAT)of the virus reaching 1:512.The high growth characteristic of this strain is stable up to 21 passages.The strain was identified by hemagglutination inhibition (HAI)test and sequencing respectively;the HA1 gene sequence of the virus was cloned and analyzed.The screening and establishment of high growth B virus provides an important tool for influenza vaccine production in Vero cells.

稳定表达SLAM受体的Vero和BHK21细胞系的建立及其对犬瘟热病毒分离效果的比较

旨在构建稳定表达SLAM受体的SLAM-Vero细胞系和SLAM-BHK21细胞系,并比较其对犬瘟热病毒(CDV)野毒株的敏感性,为CDV野毒株的快速分离与研究提供一种有效的工具。将真核表达载体Pcag-SLAM分别转染Vero细胞和BHK21细胞。经G418压力筛选结合有限稀释法筛选阳性克隆株,并通过RT-PCR、间接免疫荧光鉴定(IFA)和Western blot等方法对稳定表达SLAM受体的SLAM-Vero细胞系和SLAM-BHK21细胞系加以验证。应用这两种细胞系对3例临床犬瘟热病例的5种不同组织进行病毒分离,对分离得到的CDV进行RT-PCR及IFA鉴定。结果显示,经RT-PCR和Western blot验证,本研究成功构建出SLAM-Vero细胞系和SLAM-BHK21细胞系,SLAM-Vero细胞接种病毒12~24h即可出现典型的CDV导致的细胞融合体CPE,利用SLAM-Vero细胞从3只CDV阳性犬的肺和脾中分离得到2株CDV,而SLAM-BHK21细胞、亲本Vero细胞及亲本BHK21细胞未能分离出病毒。研究表明,与SLAM-BHK21细胞相比,SLAM-Vero细胞对CDV的分离率较高,并能产生明显的CPE。在分离CDV野毒株时,选择肺和脾更容易在SLAM-Vero细胞系上分离出病毒。

传染性法氏囊病病毒疫苗株B87在DF-1细胞和Vero细胞感染性研究

为比较传染性法氏囊病病毒(Infectious bursal disease virus,IBDV)疫苗株B87对DF-1细胞和Vero细胞易感性,对比了IBDV B87株感染两种细胞后的致细胞病变效应(cytopathic effect,CPE)、病毒基因组dsRNA、半数组织感染量(median tissue culture infective dose,TCID 50)水平、病毒载量及VP2基因表达水平。结果显示,IBDV B87株感染后,DF-1细胞CPE程度高于Vero细胞;DF-1细胞病毒基因dsRNA荧光密度高于Vero细胞;DF-1细胞病毒载量荧光密度高于Vero细胞,且DF-1细胞中病毒滴度(105.423±0.03296 TCID 50/0.1 mL)极显著高于Vero细胞中病毒滴度(102.592±0.03428 TCID 50/0.1 mL,P<0.01),VP2基因表达量显著高于Vero细胞(P<0.05)。说明IBDV B87株对DF-1细胞的感染性高于Vero细胞。

Inhibition of Curcumin-Treated Herpes Simplex Virus 1 and 2 in Vero Cells

The purpose of this study was to investigate the effect of curcumin-treated Herpes simplex virus-1 (HSV-1) and Herpes simplex virus-2 (HSV-2) virions in cultured Vero cells. Previous studies have indicated that curcumin, a polyphenol extracted from the plant Curcuma longa, has demonstrated antiviral properties against a variety of viruses. After establishing the maximum non-cytotoxic concentrations of curcumin on Vero cells, HSV-1 and HSV-2 virions were treated with varying concentrations of curcumin. The effect on infectivity was determined by antiviral assays, using WST-1, plaque assays, adsorption and penetration assays. Treating HSV-1 and HSV-2 viruses with curcumin, at a concentration of 30 μM, reduces the production of infectious HSV-1 and HSV-2 virions in cultured Vero cells by interfering with the adsorption process. These results support the potential of curcumin to be used as a therapeutic agent to reduce the transmission of HSV-1 and HSV-2.

Canine Distemper Virus Utilizes Different Receptors to Infect Chicken Embryo Fibroblasts and Vero cells

Inducing animal viruses to adapt to chicken embryos or chicken embryo fibroblasts(CEF) is a common method to develop attenuated live vaccines with full security.Canine distemper virus(CDV) also does this,but the mechanisms and particular receptors remain unclear.Virus overlay protein blot assays were carried out on CEF membrane proteins,which were extracted respectively with a Mem-PER TM kit,a radioimmunoprecipitation assay buffer or a modified co-immunoprecipitation method,and revealed a common 57 kDa positive band that differed from the 42-kDa positive band in Vero cells and also from those receptors reported in lymphocytes and 293 cells,indicating a receptor diversity of CDV and the possibility of the 57-kDa protein acting as a receptor that is involved in adaptive infection of CDV Kunming strain to CEF.

无血清全悬浮培养Vero细胞系的建立及生物反应器培养参数优化

为建立无血清全悬浮培养Vero细胞系,并使其在反应器中高密度生长。从美国典型培养物保藏中心(ATCC)引进贴壁培养型Vero细胞,通过降低血清浓度和改变培养液的方式获得1株无血清全悬浮培养型Vero细胞,扩增培养后液氮冻存,建立相应的细胞库;复苏细胞后对活力、形态、生长曲线、微生物污染、染色体核型等特性进行检定;通过Box-Behnken试验对生物反应器pH、溶氧和搅拌转速等3个培养参数进行优化,确定最优培养参数。结果显示,筛选的Vero悬浮细胞形态呈圆形、饱满、透亮,大小均匀,呈现较好的悬浮生长状态;生长曲线呈S型;细菌、真菌、支原体及外源病毒检查均为阴性;染色体数目为58或60的占75%;用响应面分析法得出的最优培养参数培养Vero细胞,细胞最高密度可达4.5×10^(6)cells/mL。结果表明,成功筛选出了适应无血清悬浮培养的Vero细胞,通过优化培养参数,可在生物反应器中高密度生长。

犬瘟热病毒强毒株在Vero-SLAM细胞上传代后的基因突变分析

为了了解犬瘟热病毒强毒株全基因组序列在Vero-SLAM细胞上传代培养后的突变情况,本试验利用犬瘟热病毒强毒分离株HeBei株第12代细胞毒,通过RT-PCR方法分段扩增犬瘟热病毒全基因,对扩增出的各个片段进行克隆和鉴定,并应用SeqMan程序将所测得的序列进行拼接成Hebei株全长cDNA序列。结果表明,全基因与原始序列相比有24处碱基突变,总突变率为0.15%,其中3处为非编号码区的突变,其余21处在编码区,碱基突变率最高的蛋白基因为F(0.36%),最低为N(无突变)。氨基酸突变率分别为N蛋白0.00%;P蛋白0.39%;M蛋白0.30%;F蛋白0.60%;H蛋白0.50%;L蛋白0.18%。表明犬瘟热病毒强毒株经Vero-SLAM细胞传代培养后基因突变主要发生在F蛋白基因上。

Neurturin gene cloning and expression in Vero cells

BACKGROUND： Transplantation of cell lines expressing neurturin （NTN） has been used to treat animal models of Parkinson＇s disease. However, gone homology between humans and rats varies greatly, so experimental results are not entirely suitable for understanding cellular transplantation in humans. OBJECTIVE： To explore expression of NTN in African green monkey kidney cells （Vero cells）; to obtain a stably NTN expressing cell line. DESIGN, TIME AND SETTING： An observation study of gone engineering and cellular biology was performed at the Institute of Medical Biology, Chinese Academy of Medical Science and Peking Union Medical College between 2005 and 2008. MATERIALS： Human embryonic hepatic tissues, expression vector pcDNA3, and Vero cells were prepared in this laboratory. Primers were synthesized by TaKaRa Biotechnology, Dalian, China; RNA extraction kit and plasmid extraction kit were purchased from Shanghai Watson Bioengineering, China; G418 and MTT were purchased through Sigma, USA; Lipofectamine2000 was a product of Invitrogen, USA; mice anti-human NTN antibody and fluorescent labeling goat anti-mouse IgG antibody were provided by Jingmei Biotech, China. METHODS： Total RNA was harvested from human embryonic hepatic tissues, and NTN cDNA was cloned by RT-PCR method, followed by subcloning into the pcDNA3 eukaryotic expression vector. The obtained pcDNA3/hNTN was stably transfected into Vero cells using Lipofectamine 2000, and stably expressing clones were selected using G418. MAIN OUTCOME MEASURES： NTN mRNA and protein expressions were respectively identified by RT-PCR and immunofluorescence. The morphology of transfected cells was observed under inverted microscopy, and the growth characteristics of those cells were determined using MTT method. RESULTS： A clonal cell line, stably expressing human NTN mRNA and protein, was obtained through stable transfection of pcDNA3/hNTN into Vero cells. The transfected Veto cells exhibited irregular morphology, rather than a spindle shape. The growth retardation phase was prolonged, but the number of cells was identical to non-transfected cells. CONCLUSION： Vero cell lines, which stably expressed human NTN protein, were obtained, and expression patterns of these cell lines were acceptable.

Sensitivity of Different Cytotoxic Responses of Vero Cells Exposed to Organic Chemical Pollutants and their Reliability in the Bio-toxicity Test of Trace Chemical Pollutants

Objective To find a sensitive cytotoxic response to reflect the bio-toxicity of trace organic pollutants, the sensitivity and reliability of morphological change and proliferation inhibition of Vero cells exposed to 2, 4, 6-trichlorophenol （TCP） and the leachate from products related to drinking water （PRDW） were compared, and the mechanism of the morphological change in Vero cells exposed to chemical pollutants was studied. Methods Vero cells were treated by different concentration of TCP and the leachate from PRDW. Methylthiazol-2-yl-2, 5-diphenyl tetrazolium bromide （MTT） assay was carried out for proliferation inhibition. Bioluminescence method was carried out as another method to test the toxicity of TCP. Flow Cytometry assay was used to test cell Apoptosis and damage of cell-membrane. Results 0.25 mg/L TCP had an effect on cell morphology, and the proportion of morphologically changed cells increased with increasing TCP concentration. At low TCP concentrations, inhibition of cell proliferation did not seem to correlate to TCP concentration, and was negative when TCP concentration was 〈1.0 mg/L. After exposure to leachate from PRDW extracted at different temperatures, the percentage of morphologically changed cells increased with extracting temperature, but the inhibition of cell proliferation failed to reflect the correlation between extracting temperature and proliferation inhibition of Vero cells. Although the Sensitivity of bioluminescence method seems to be similar to morphological change in Veto cells, the bacterial in this method is not homologous enough with human body cells to reflect the toxicity to human body. These imply cell morphological change is a more sensitive and reliable method to reflect bio-toxicity of organic pollutants than proliferation inhibition. Flow cytometry analysis and cell rejuvenation experiments indicated cell membrane damage, which results in cell morphological change, was an early and sensitive cytotoxic response comparing with necrosis. Conelusion These results indicated that the cell membrane toxicity represented by morphological changes is a more sensitive and reliable method to indicate the composite bio-toxicity of trace chemicals than proliferation inhibition, inhibition on bioluminescence and necrosis. Nevertheless, the quantification of morphological change should be studied further.

Study on the Purification of OPV Produced on Vero Cells with Q-Sepharose F.F.

Q Sepharose Fast Flow(Q Sepharose F.F.) was adopted to purify the suspensions of type Ⅰ,Ⅱ,Ⅲ oral poliovaccine (OPV), which is prepared from Vero cells. After clarification and concentration by ultrafiltration,the recovery of virus infected titre may attain above 85%.Using column chromatography on Q Sepharose F.F. to purify the concentrated virus suspensions,the purified viruses attain 100% recovery of virus infectivity. Dot membrane hybrization was used to detect DNA with the probe of Vero cell genome DNA which was labeled with α P 32 dATP,the contents of residual substrate DNA was less than 100 Pg/dose. The process of downstream had no significant influence on some biological characters of purified viruses,such as virus morphology ,tumorigenicity, rct/40 character and capsid protein.This downstream reseach indicates that Q Sepharose F.F. is an ideal chromatography material for purifying OPV prepared from Vero cells.

Study on Propagation of Chicken Infectious Bursal Disease Virus on Vero Cells Using Microcarriers in Fermentor

It was in flask optimization tests proved that 2% serum, pH 7.0, 5:10 000 inoculation concentration of infectious bursal disease virus (IBDV) and 108 hours cultivation for IBDV harvest after its inoculation were the optimal conditions when IBDV was propagated on Vero cells. 250 ml self-made spinner bottle and 5 L stirring fermentor tests proved that IBDV could maintain higher liters for a long time and the highest liters of IBDV in a spinner bottle and a fermentor were 8.875 and 8.58 ( - lgTCID50/0.1 ml) respectively when IBDV was proliferated on Vero cells using 2 g/L microcarriers in a spinner bottle and a fermentor and was cultivated under the optimum conditions obtained from flask tests after Vero cells had developed a confluent monolayer on microcarriers, which were at least one titer higher than the highest titer in the traditional rolling bottle. All these results suggested that this technology could be applied to large scale production for IBDV.

Using the SELDI ProteinChip System to Detect Changes in Protein Expression in Vero Cells after Infection

人的疱疹单一的病毒(HSV-1 ) 1 引起美容，眼睛，并且 encephalitic 疾病并且与潜伏的感染和癌症被联系。这里，我们开发了由使用 SELDI 蛋白质薄片在在 vitro 有教养的 Vero 房间检测蛋白质表示的变化在蛋白质水平学习 HSV-1 感染的致病的一个工具。在有为 12， 24 或 48 h 的 HSV-1 和文化的感染以后，房间被收获并且 lysed。IMAC3 数组被用于 SELDI-TOF-MS 在感染前后检测 proteomic 差别。薄片检测了一系列差别表示蛋白质山峰。有趣地，在 16 912 Da 的山峰和 17 581 Da 与 ISG15 的分子的团精确相应，它可以在感染的过程期间参予抗病毒的活动。因此，我们获得了的结果能用作一个基础学习在病毒和它的主人之间的 HSV-1 和相互作用的致病。另外，他们能为 HSV-1 感染的治疗在新治疗学的目标的发现帮助。关键词 SELDI 蛋白质薄片 - Vero 房间 - HSV-1 - 蛋白质表达式 CLC 数字 R373 基础项目：中国(30540075 ) 的国家自然科学基础；

Comparative Efficacy of Different Inactivated Hydro-Pericardium Syndrome Vaccines Prepared from Infected Liver and Vero Cell Line Adapted Adeno Type 4 Virus

Hydro-Pericardium Syndrome (HPS) is viral problem of commercial poultry caused by aviadeno virus type-4. In Pakistan the problems have been controlled by administering inactivated infected liver homogenate vaccine (ILHV). The use of liver based HPS vaccines remained potential threat for having hypersensitivity reactions in poultry. The current study was carried out to compare the serological potency of HPS ILHV to vero cell line adopted vaccine in term of anti HPS-ELISA antibody titers. 14 HPS virus vaccines were prepared based on different concentration of antigen, type of adjuvants and source of virus substrate. Total of 160 birds were divided into 16 groups each containing 10 birds. At day of 14th age each bird of every group was injected with 0.3 ml dose of respective vaccine. It was observed that HPS infected liver based vaccine having 1 × 105.6, 1 × 105.6 and 1 × 103.6 bird lethal dose 50 induced 1092.10, 875.25 and 702.2 anti-HPS ELISA antibody titer respectively. The 20, 25 and 30 doses/gm HPS infected liver vaccine induced 110.4, 1071.9 and 1037.8 anti-HPS ELISA antibody titer respectively. Montanide based tissue culture HPS vaccine showed significantly higher 1148.45 anti-HPS ELISA antibody titer to aluminium hydroxide based vaccine (137.2) (P 5.6 TCID50 is serological potent against field infection. The vaccines based on such formulation could be prepared in future for effective immuno-prophylaxis against HPS virus.

The Growth Study of Vero Cells in Different Type of Microcarrier

The fact of microcarrier (MC) culture introduces new possibilities and makes possible the practical high-yield culture of anchorage-dependent cells has generated a considerable focus in this study. The objective of this research was to study the comparison of Vero cell growth on different types of commercial microcarriers;Cytodex-1, Cytodex-3, Hil-lex? II and Plastic Plus in spinner vessel and two liters bioreactor cultured for 96 hours. Biological performance of the microcarrier in RPMI media showed the preference of Vero cell grew on Cytodex 3 microcarriers with highest maximum viable cell number (2.4 × 105 cells/ml) followed by Cytodex 1, Hillex and Plustic Plus. Vero cell on Cyto-dex-3 data in spinner flask was compared in bioreactor and result showed higher viable cell number in biorector. Thus, this dextran-crosslink gelatin microcarrier (Cytodex 3) provided the best surface for cell attachment and fast proliferation. At the end of this cell growth improvement will be used for virus transfection producing a vaccine in bioreactor.