流感病毒在Vero细胞系与MDCK细胞系增殖条件的比较

目的研究流感病毒H1N1及其他亚型在Vero细胞系和MDCK细胞系高效增殖的最适条件,比较两种细胞系对流感病毒的敏感性差异及影响敏感性差异的条件。方法在培养好的Vero细胞系与MDCK细胞系用不同的病毒感染复数(M.O.I)、胰酶浓度、病毒吸附时间、病毒维持液血清质量浓度等条件进行流感病毒在细胞上的增殖。结果在M.O.I为0.01接种流感病毒,吸附时间为1 h,胰酶质量浓度2μg/mL,血清质量浓度为8%时,流感病毒血凝素在MDCK细胞系可获得较高的滴度。结论 MDCK细胞系是适于流感病毒培养的细胞,它作为生产新型流感病毒疫苗的主要细胞基质需要进一步的研究。     

MDCK细胞微载体培养条件优化研究

研究细胞接种量、搅拌转速和微载体浓度对MDCK细胞微载体培养时的影响,以合理优化MDCK细胞微载体培养最大增殖时期的最优条件,对疫苗和病毒分离具有重要意义,以期达到在疫苗和病毒分离领域提高生产效率。采用微载体培养MDCK细胞,在不同搅拌转速、微载体浓度和细胞接种量进行培养,每隔24 h取样计数,确定最优的培养条件。结果表明,细胞接种量在20个/球、搅拌转速45 r/min和载体浓度在2 g/L时,MDCK细胞的增殖较快,细胞密度较大,细胞的密度最大可达15.6×106个/mL,适合MDCK细胞增殖生长。     

重组胰酶在四价流感病毒裂解疫苗(MDCK细胞)制备中的应用

目的 探究使用重组胰酶(recombinant trypsin, RT)替代N-(对甲苯磺酰基)-L-苯基乙基氯甲基酮(N-p-Tosyl-L-phenylalanine chloromethyl ketone, TPCK)处理的牛源胰蛋白酶(TPCK-trypsin, TT),在基于无血清悬浮细胞培养的四价流感病毒裂解疫苗制备中的可行性。方法 用不同浓度的RT处理无血清悬浮培养的犬肾细胞(madin-darby canine kidney cell,简称MDCK细胞),检测其对细胞密度和细胞活力的影响。在流感病毒感染环节添加不同浓度的RT,在不同时间细胞收获病毒液，检测病毒滴度，确定适合的RT浓度。在2μg/mL RT的条件下，接种不同(亚)型流感病毒毒株，以检测不同时间病毒滴度及细胞密度，并在3 L生物反应器中验证RT对流感病毒扩增的影响。结果 当RT浓度<5μg/mL时，对无血清悬浮培养的MDCK细胞生长密度和细胞活力均无显著影响；在病毒感染与扩增过程中，添加终浓度为2μg/mL RT可保证不同(亚)型流感病毒疫苗株的有效扩增。其中，H1N1、H3N2、B/Vic、B/Ya...     

细胞密度和营养供给对H1N1流感病毒产率的影响

探究细胞培养生产流感病毒过程中,高细胞密度引起低单位细胞病毒产率(Svy)的原因及找到解决方法。通过增加微载体浓度以及换液操作获得较高的细胞密度;考察了感染时细胞密度(CCI)和病毒感染用维持培养基对病毒产量和单位细胞病毒产率的影响。在12.6 g/L微载体培养过程中,通过换液操作,可获得高细胞密度,达到1.47×107 cells/m L。在CCI为1×107cells/m L条件时,选择合适的维持培养基,其Svy最高达到5.14×103 virions/cell,比同等条件下用DMEM维持培养基的Svy值提高了近一倍。高密度培养MDCK细胞生产流感病毒时,充分考虑不同阶段的培养条件和营养需求,可以提高细胞密度和单位细胞病毒产率,进而提高流感病毒的产量。该研究结果为工业化生产流感病毒疫苗提供了基础数据。     

Vero细胞培养A/Shanghai/CN02/2013(H7N9)Va流感病毒适宜条件研究

目的:优化Vero细胞培养H7N9流感病毒的培养条件,建立细胞培养病毒高产培养系统。方法:采用不同病毒接种MOI、培养温度、pH值和TPCK胰酶等条件优化培养H7N9流感病毒Vero细胞适应株A/Shanghai/CN02/2013(H7N9)Va的条件,并将其连续传代后扩大至细胞工厂大规模培养。结果:Vero细胞高产H7N9流感病毒培养条件为DMEM/F12和MEM以1∶1混合,并添加0.3 mg/mL牛血清白蛋白、1%谷氨酰胺、0.5%双抗和1.5μg/mL TPCK胰蛋白酶,pH为7.4时,连续传代病毒血凝效价保持在512,扩大至细胞工厂大规模培养病毒产量稳定。结论:建立的Vero细胞培养H7N9流感病毒条件,能够持续稳定高产,并适用于细胞工厂大规模培养,有望用于H7N9流感细胞疫苗的大规模制备。     

miR26a和miR939调控H1N1型流感病毒在MDCK细胞中的复制

摘要：【目的】研究发现microRNAs（miRNAs）可以参与调控病毒在宿主细胞内感染和复制的过程。作者研究了两条miRNAs对H1N1型流感病毒在宿主细胞内复制的影响。【方法】构建miR26a和miR939的高效表达载体,并将这两种表达载体转入MDCK细胞中,24 h后用H1N1型流感病毒感染转染后的MDCK (Madin dardy canine kidney) 细胞,接种72 h后,检测流感病毒的复制情况,研究miR26a和miR939对H1N1型流感病毒在MDCK细胞内复制的影响。【结果】实验结果表明,miRNAs的表达载体可以在细胞内高效表达miRNAs,不同的miRNAs对流感病毒在MDCK细胞中复制的调控作用不同, miR26a可以有效抑制流感病毒在MDCK细胞中的复制,而miR939则促进流感病毒在MDCK细胞中的复制的作用。【结论】细胞内miRNAs可以调控H1N1型流感病毒在宿主细胞中的复制过程,本文首次报导miR26a和miR939在流感病毒复制过程中的调控作用。     

禽流感病毒H5N1全基因组克隆与分析

为明确广东地区分离的一株禽流感病毒H5N1的遗传背景,建立流感病毒反向遗传的平台。对该株禽流感病毒进行了空斑纯化与组织细胞培养,检测其在MDCK细胞中的增殖特性;利用H5N1病毒通用引物,通过RT-PCR对该病毒全基因组的8条片段进行全长克隆及测序分析;将H5N1的8条全长基因组片段分别插入反向遗传通用载体中,构建禽流感病毒H5N1的感染性克隆。结果表明,该H5N1毒株在MDCK细胞中可不依赖胰酶进行有效增殖与复制,可使MDCK细胞出现典型细胞病变,具有高致病性禽流感病毒的细胞增殖特征。RT-PCR克隆得到该H5N1毒株的PB2、PB1、PA、HA、NP、NA、M和NS八条全长片段,经测序分析确认该毒株的基因序列,其内部编码序列出现多处突变,其中HA连接肽为多个连续碱性氨基酸,表明该毒株可不依赖胰酶进行有效复制,与细胞培养结果一致,未出现抗药性的遗传突变。PCR与测序证明,插入H5N1八个全长基因组片段的载体序列完全正确,表明成功构建了该毒株的感染性克隆。为明确病毒遗传信息,建立流感病毒反向遗传的平台,为进一步研究禽流感病毒相关疫苗提供了研究基础。     

感染时间对MDCK细胞中H1N1甲型流感病毒扩增过程的影响

为了研究感染时间TOI对MDCK细胞中H1N1甲型流感病毒扩增过程的影响,以期合理优化以MDCK细胞培养技术为基础的H1N1流感病毒生产工艺,从而提高其生产效率。在不同TOI条件下以H1N1流感病毒感染MDCK细胞,考察TOI对MDCK细胞生长与代谢动力学以及H1N1流感病毒扩增过程的影响。结果表明,当TOI为72 h时,H1N1流感病毒产量最高。然而单位细胞病毒产率却随TOI增大而呈现下降趋势,进一步剖析TOI与感染时细胞密度CCI对单位细胞病毒产率的影响可知,该现象是由细胞状态而非高细胞密度所致。上述研究揭示了由TOI不同导致的细胞状态差异对MDCK细胞中H1N1流感病毒生产效率的重要性。     

两种传代细胞系对轮状病毒D36株(P[4]G2)敏感性的比较

目的探讨轮状病毒D36株在MDCK细胞和Vero细胞上培养的适应性,确定其培养的最佳细胞基质及培养条件。方法将D36株以MOI 1.0按不同培养瓶分组接种MDCK细胞和Vero细胞,补充含有不同浓度胰酶的维持液,于不同时间观察两种细胞病变的情况,同时抽样检测病毒滴度,分析两种细胞对D36株的敏感性。结果D36株病毒感染MDCK细胞后第6天病毒滴度达到最高,为(5.00～5.50)lgCCID50/mL;而D36株病毒感染Vero细胞后病毒滴度于第8天达高峰,为(4.50～4.75)lgCCID50/mL。另外,在两种细胞维持液中加入约0.8μg/mL的胰酶均可提高病毒滴度。结论两种细胞系在同等条件下感染D36株病毒后,MDCK细胞比Vero细胞出现病变的时间早,每一批MDCK细胞培养物病毒滴度高于同批次试验的Vero细胞培养物。     

MDCK单克隆细胞库的建立及检定

目的:建立甲型H1N1流感病毒疫苗株高适应MDCK单克隆细胞库,用于培养生产流感病毒疫苗,为细胞代替鸡胚制备流感病毒疫苗提供保证。方法:用有限稀释法将MDCK细胞进行单克隆化,通过血凝和TCID50筛选甲型H1N1流感病毒疫苗株的高适应性单克隆化细胞株,扩大培养建立细胞库并进行检定。结果:共制备了97株单克隆化MDCK细胞,筛选到甲型H1N1流感病毒疫苗株高适应性MDCK单克隆细胞株,扩大培养建立了细胞库,经检定符合《中华人民共和国药典.三部》(2010版)对细胞库的要求。结论:建立了甲型H1N1流感病毒疫苗株高适应性MDCK单克隆细胞库,为细胞培养生产流感病毒疫苗奠定了基础。     

Properties of reassortants of human and avian influenza viruses. Reproduction in MDCK cells at suboptimum temperatures

A series of reassortants has been constructed by crossing of UV-inactivated avian influenza virus of H3N8 subtype and live human influenza virus of H1N1 subtype, adapted to growth in continuous canine kidney cell line (MDCK). The analysis of RNA duplexes has shown that the reassortants contain HA gene of avian influenza virus whereas the other genes belong to human parent virus. The reassortants were efficiently reproduced in MDCK cells at low temperature (limiting for the avian parent virus). The data suggest that the avian virus HA gene does not hamper the reproduction of reassortant viruses in mammalian cells under the conditions unfavorable for the multiplication of avian influenza subtype H3N8 viruses.     

Evaluation of MDCK Cell-Derived Influenza H7N9 Vaccine Candidates in Ferrets

Avian-origin influenza A (H7N9) viruses emerged as human pathogens in China in early 2013 and have killed >100 persons. Influenza vaccines are mainly manufactured using egg-based technology which could not meet the surging demand during influenza pandemics. In this study, we evaluated cell-based influenza H7N9 vaccines in ferrets. An egg-derived influenza H7N9 reassortant vaccine virus was adapted in MDCK cells. Influenza H7N9 whole virus vaccine antigen was manufactured using a microcarrier-based culture system. Immunogenicity and protection of the vaccine candidates with three different formulations (300μg aluminum hydroxide, 1.5μg HA, and 1.5μg HA plus 300μg aluminum hydroxide) were evaluated in ferrets. In ferrets receiving two doses of vaccination, geometric mean titers of hemagglutination (HA) inhibition and neutralizing antibodies were <10 and <40 for the control group (adjuvant only), 17 and 80 for the unadjuvanted (HA only) group, and 190 and 640 for the adjuvanted group (HA plus adjuvant), respectively. After challenge with wild-type influenza H7N9 viruses, virus titers in respiratory tracts of the adjuvanted group were significantly lower than that in the control, and unadjuvanted groups. MDCK cell-derived influenza H7N9 whole virus vaccine candidate is immunogenic and protective in ferrets and clinical development is highly warranted.     

重组细胞高产型H3N2猪流感病毒株的拯救

为拯救出一株能够在动物传代细胞中高水平复制的H3N2亚型猪流感疫苗株,利用反向遗传操作技术,将A/Goose/Dalian/3/01(H9N2)毒株的PB1、PA、NP、M、NS基因和A/PR/8/34毒株的PB2基因作为内部基因与猪流感病毒A/Swine/Henan/S4/01(H3N2)毒株的HA、NA基因进行重组,成功拯救出了具有高度细胞适应性毒株rH3N2株,该毒株接毒MDCK细胞60h后,血凝价可以达到1∶512,表明该毒株具有高度适应细胞繁殖特性,为H3N2亚型猪流感病毒细胞培养型疫苗的研制奠定了基础。     

转谷氨酰胺酶2抑制H1亚型流感病毒在MDCK细胞中的增殖

组织转谷酰胺酶(transglutaminase 2,TGM2)是一种普遍存在的多功能蛋白,与不同细胞的粘附和肿瘤形成有关.有证据表明,TGM2参与了宿主细胞与病毒间的相互作用,但是对于流感病毒在细胞内增殖的影响还未有报道.为了探究MDCK细胞中TGM2对H1N1亚型流感病毒增殖的影响,本研究构建了TGM2过表达和敲除...     

Production of inactivated influenza H5N1 vaccines from MDCK cells in serum-free medium

Background

Highly pathogenic influenza viruses pose a constant threat which could lead to a global pandemic. Vaccination remains the principal measure to reduce morbidity and mortality from such pandemics. The availability and surging demand for pandemic vaccines needs to be addressed in the preparedness plans. This study presents an improved high-yield manufacturing process for the inactivated influenza H5N1 vaccines using Madin-Darby canine kidney (MDCK) cells grown in a serum-free (SF) medium microcarrier cell culture system.

Principal Finding

The current study has evaluated the performance of cell adaptation switched from serum-containing (SC) medium to several commercial SF media. The selected SF medium was further evaluated in various bioreactor culture systems for process scale-up evaluation. No significant difference was found in the cell growth in different sizes of bioreactors studied. In the 7.5 L bioreactor runs, the cell concentration reached to 2.3×10⁶ cells/mL after 5 days. The maximum virus titers of 1024 Hemagglutinin (HA) units/50 µL and 7.1±0.3×10⁸ pfu/mL were obtained after 3 days infection. The concentration of HA antigen as determined by SRID was found to be 14.1 µg/mL which was higher than those obtained from the SC medium. A mouse immunogenicity study showed that the formalin-inactivated purified SF vaccine candidate formulated with alum adjuvant could induce protective level of virus neutralization titers similar to those obtained from the SC medium. In addition, the H5N1 viruses produced from either SC or SF media showed the same antigenic reactivity with the NIBRG14 standard antisera.

Conclusions

The advantages of this SF cell-based manufacturing process could reduce the animal serum contamination, the cost and lot-to-lot variation of SC medium production. This study provides useful information to manufacturers that are planning to use SF medium for cell-based influenza vaccine production.     

N-乙酰半胱氨酸体外对流感病毒H1N1的抑制作用

目的探讨N-乙酰半胱氨酸（N—acetylcysteine,NAC）在体外对流感病毒H1N1的抑制作用。方法采用MTT法、鸡胚接种法和免疫荧光法,观察NAC对流感病毒HlM的抑制作用。采用血球凝集试验、神经氨酸酶活性抑制试验和透射电镜负染技术,初步探讨NAC对流感病毒HlM的抑制机制。结果NAC在MDCK细胞上的最大无毒剂量是6．25mg／mL;流感病毒H1Nl在MDCK细胞上的半数致死感染浓度（TCID-50）为1012-2.25／100μ;在三种作用途径下（治疗性给药、预防性给药和直接灭活后给药）,NAC明显抑制了流感病毒HlNl对MDCK细胞的感染,细胞存活率分别为91．88％、93．21％、94．67％,在对照组,流感病毒H1N1感染后的细胞存活率为28．32％,两者相比差异有统计学意义（P〈0．05）;免疫荧光结果显示,与病毒对照组形成的强特异性荧光相比,三种作用途径感染MDCK细胞后的特异性荧光明显减弱;鸡胚培养法的结果显示,NAC明显抑制了流感病毒H1N1在鸡胚内的增殖,实验组血凝效价低于1：2,对照组血凝效价为1：1024;神经氨酸酶活性抑制试验和透射电镜的结果显示,NAC能够明显抑制流感病毒川N1的神经氨酸酶活性,对流感病毒H1N1的病毒体结构也有明显的破坏作用。结论NAC在体外对流感病毒川N1有明显的抑制作用,其抑制机制可能与NAC对流感病毒血凝素和神经氨酸酶活性抑制及病毒体的直接破坏有关。     

Direct sequencing of the HA gene of influenza (H3N2) virus in original clinical samples reveals sequence identity with mammalian cell-grown virus.

When influenza (H3N2) viruses from infected individuals are grown in embryonated chicken eggs, viruses are isolated which differ antigenically and structurally from viruses grown in mammalian Madin-Darby canine kidney (MDCK) cell culture [G.C. Schild, J.S. Oxford, J.C. de Jong, and R.G. Webster, Nature (London) 303:706-709, 1983]. To determine which of these viruses is most representative of virus replicating in the infected individual, a region of the HA gene of virus present in original clinical samples was amplified by using the polymerase chain reaction and sequenced directly. Comparison of 170 amino acid residues of HA1 flanking and containing the receptor-binding site and antigenic sites indicated that over this region, the HA of virus replicating in the infected individual was identical to that of virus after growth in MDCK cells and was distinct from the HA of viruses grown in eggs. Therefore, cultivation of human influenza H3N2 virus in mammalian MDCK cells results in a virus similar to the predominant population of virus found in the infected individual.