Reference Gene Selection for Normalization of PCR Analysis in Chicken Embryo Fibroblast Infected with H5N1 AIV

Chicken embryo fibroblasts (CEFs) are among the most commonly used cells for the study of interactions between chicken hosts and H5N1 avian influenza virus (AIV).In this study,the expression of eleven housekeeping genes typically used for the normalization of quantitative real-time PCR (QPCR) analysis in mammals were compared in CEFs infected with H5N1 AIV to determine the most reliable reference genes in this system.CEFs cultured from 10-day-old SPF chicken embryos were infected with 100 TCID50 of H5N1 AIV and harvested at 3,12,24 and 30 hours post-infection.The expression levels of the eleven reference genes in infected and uninfected CEFs were determined by real-time PCR.Based on expression stability and expression levels,our data suggest that the ribosomal protein L4 (RPL4) and tyrosine 3-monooxygenase tryptophan 5-monooxygenase activation protein zeta polypeptide (YWHAZ) are the best reference genes to use in the study of host cell response to H5N1 AIV infection.However,for the study of replication levels of H5N1 AIV in CEFs,the β-actin gene (ACTB) and the ribosomal protein L4 (RPL4) gene are the best references.

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.

Adaptability of Fowlpox Virus in Chicken Embryo Passage Cells

[Objective] To observe whether fowlpox virus （FPV） can proliferate in chicken embryo passage fibroblasts or not and then try to use chicken embryo passage fibroblasts to replace primary chicken embryo cells for FPV culture. [Method] Primary chicken embryo fibroblasts were prepared and subcultured. After FPV were inoculated on the 20th passage fibroblasts, cytopathy was observed. Then, the FPV culture was identified and determined quantificationally. [Result] Specific cytopathy appeared in the FPV-inoculated chicken embryo passage fibroblasts. The titer of the yielded FPV culture reached the standard for production of fowl pox vaccine. Further analysis reveals that the chorioallantoic membrane lesions were caused by FPV. [ Conclusion] FPV can reproduce in chicken embryo passage fibroblasts, and the Uter of FPV cell culture can meet the pro- duction requirements of fowl pox vaccine.

Effects of Proliferation of CEF with Ginsenoside and Its Derivatives

Objective The research aimed to provide theoretical basis for studying anti-MDV mechanism of ginsenoside and its derivatives in vitro. Method Effects of ginsenoside and its derivatives on proliferation activity of chick embryo fibroblast （CEF） in vitro were determined by using neutral red dye absorption method. Result The results showed the proliferation effects of different drugs are not completely same, and are more obvious with low toxic drugs. Detected at different action times, the differences of OD values was biggest at 72 h when compared with normal control group, while there was no significant difference at 24 h. Conclusion Ginsenoside and its derivatives could promote the proliferation of CEF cells in medium as low concentrations, which have time-dependent characteristic.

中性红染色法检测人参皂苷及其衍生物对CEF增殖的影响

[目的]为体外研制人参皂苷及其衍生物的抗MDV作用机制提供理论依据。[方法]采用中性红染料吸收法,检测了人参皂苷及其衍生物对鸡胚成纤维细胞(CEF)体外培养中增殖活性的影响。[结果]各药物的促增殖作用不完全相同,低毒性的药物促增殖作用更明显。从药物对CEF细胞的不同作用时间点来看,以72 h的OD值和正常对照的差异最大,在24 h和正常对照组差异不显著。[结论]人参皂苷及其衍生物在中、低浓度能够促进CEF细胞的增殖,且药物作用具有时间依赖性。

芝芪菌质多糖对CEF的增殖和抵抗NDV感染的研究

[目的]明确芝芪菌质多糖是否是芝芪菌质提高动物免疫力的有效成分。[方法]用不同浓度的乙醇对芝芪菌质水提物进行分级沉淀,得到3种芝芪菌质多糖(GAP30、GAP60和GAP90),采用中性红染料吸收法,研究其对鸡胚成纤维细胞(CEF)增殖的影响及抵抗NDV感染的效果。[结果]GAP30、GAP60、GAP90的得率分别为0.37%、0.70%、1.04%,表明乙醇分级沉淀已将芝芪菌质中的多糖成分提取完全。GAP30、GAP60在浓度为1×10-1、1×10-2mg/ml时能显著促进CEF增殖,GAP90在浓度为1×10-3mg/ml时即能显著促进CEF增殖。GAP30、GAP60在浓度为1×10-2mg/ml时能显著抵抗NDV感染,GAP90在浓度为1×10-1、1×10-2mg/ml时能显著抵抗NDV感染。[结论]芝芪菌质多糖能不同程度地促进CEF增殖、抵抗NDV感染,以GAP90的效果最好。

NDV基因Ⅶ型与基因Ⅱ型感染CEF后microRNA表达谱分析

本研究旨在探究新城疫病毒(Newcastle disease virus,NDV)流行株HB株(基因Ⅶ型)与疫苗株La Sota株(基因Ⅱ型)在感染鸡胚成纤维细胞(Chicken embryo fibroblasts,CEF)36 h后宿主细胞microRNA(miRNA)表达谱变化情况。通过高通量测序技术分别对La Sota株与HB株感染CEF后36 h后的样本与参考鸡源基因组进行系统比对,筛选差异表达miRNA并对其靶基因进行GO功能注释以及KEGG通路富集。最后随机筛选5条miRNA通过实时荧光定量PCR(Real-time quantification PCR,RT-qPCR)进行验证。结果表明,La Sota与HB感染组中已知miRNA分别为56.9%和47.8%;La Sota与HB感染组通过差异性比较后共筛选出10条差异表达miRNA;通过对差异表达基因的靶基因进行GO与KEGG富集发现,其主要在细胞代谢、生物合成以及应激信号传导等通路上出现显著富集;RT-qPCR结果与RNA-seq结果趋势一致,证明了测序结果的可靠性。为进一步揭示不同NDV毒株感染CEF以及在感染过程中miRNA发挥的调控作用提供了研究基础。

基于CRISPR-Cas9技术构建TET2基因敲除的鸡胚成纤维细胞系

为研究甲基胞嘧啶双加氧酶2(tet methylcytosine dioxygenase 2,TET2)及其介导的羟甲基化修饰在调控天然免疫反应中的作用,利用CRISPR-Cas9基因编辑技术构建TET2基因敲除的鸡胚成纤维细胞系。针对鸡TET2 mRNA的2种剪接变体的共有CDS序列设计4组sgRNA,构建sgRNA表达质粒,连同Cas9-T2A-GFP质粒共转染DF-1细胞,筛选高切割效率的sgRNA;将转染该sgRNA的DF-1细胞,进行流式细胞分选,获取表达绿色荧光蛋白(green fluorescent protein,GFP)的细胞,再通过有限稀释法筛选单克隆细胞,并用DNA测序进行鉴定。单克隆敲除细胞扩大培养后,Western blot和Dot blot检测TET2蛋白的表达水平和羟甲基化(5hmC)水平。DNA测序结果表明,TET2-gRNA-2靶位点附近分别发生2和28 bp的缺失突变,引起TET2蛋白移码突变,将该细胞株命名为DT-6。DT-6细胞传代15次以上,细胞形态稳定。Western blot结果显示,与DF-1细胞相比,DT-6细胞几乎不表达TET2蛋白。Dot blot结果显示,与DF-1细胞相比,DT-6细胞全基因组羟甲基化水平显著降低。利用CRISPR-Cas9技术成功构建了敲除TET2基因的鸡胚成纤维细胞系,为研究鸡TET2及其介导羟甲基化修饰参与调控天然免疫反应的途径和分子机制奠定基础。

不同胰蛋白酶在制备腮腺炎减毒活疫苗中的效果比较

目的比较基因重组胰蛋白酶和猪源胰蛋白酶在腮腺炎减毒活疫苗中的使用效果。方法使用浓度为10%、15%、20%基因重组胰蛋白酶制备鸡胚成纤维细胞,通过细胞密度、细胞活性、24 h以及48 h细胞贴壁状态等指标确定基因重组胰蛋白酶使用浓度;与猪源胰蛋白酶进行比较,通过细胞密度、细胞活性、48 h细胞贴壁状态以及病毒滴度等指标比较两种胰蛋白酶的使用效果;使用基因重组胰蛋白酶制备3批腮腺炎减毒活疫苗,检定疫苗的稳定性;规模化放大验证该工艺的稳定性。结果通过研究发现基因重组胰蛋白酶的使用浓度为15%;与猪源胰蛋白酶进行比较,两种胰酶制备的细胞密度水平一致,无显著性差异(P>0.05),48 h后细胞均生长至单层,细胞状态良好,按照同一MOI进行接毒,病毒滴度无显著性差异(P>0.05);使用CF-10进行试验,病毒滴度也无差异(P>0.05);连续3批使用基因重组胰蛋白酶制备的疫苗热稳定性良好,且该工艺可以规模化放大。结论在制备腮腺炎减毒活疫苗中可以使用浓度15%的基因重组胰蛋白酶替代猪源胰蛋白酶,作为鸡胚成纤维细胞消化液使用。

先导编辑在鸡胚成纤维细胞系中的效率研究

为探究先导编辑在鸡细胞系中的基因编辑效率,研究通过点突变和重组连接的方式构建先导编辑的表达质粒,使用在线软件设计并化学合成靶向OVM、MSTN和NHE1基因的先导编辑引导RNA(pegRNA)质粒,脂质体转染上述质粒至鸡胚成纤维细胞系(DF-1)中并进行药物筛选,PCR产物TA克隆测序检测并统计各位点的编辑效率。结果显示:测序和PCR鉴定结果表明先导编辑表达质粒构建成功;DF-1中OVM基因经先导编辑后成功产生错义突变,其中精确编辑效率为41.10%、错误插入与缺失(indel)效率为6.67%,均显著优于对照组的常规基因编辑(P<0.05);MSTN基因的先导编辑精确编辑效率为10.24%、indel效率为13.57%,NHE1基因的先导编辑精确编辑效率为24.88%、indel效率为7.18%。结果验证了先导编辑在鸡细胞系中的有效性和普适性,为其进一步应用于基因编辑鸡的制备奠定基础。

shRNA-triggered RNAi inhibits expression of NDV NP gene in chicken embryo fibroblast

RNA interference(RNAi)technology is a powerful tool for identifying gene functions.Chicken embryo fibroblast(CEF)is an ideal model for studying the interaction between avian viruses and their hosts.To establish a methodological platform for RNAi studies in CEF,three plasmid vectors expressing short hairpin RNAs(shRNAs)targeted against the Newcastle disease virus(NDV)NP gene were constructed.One of them,ndv1,was proven effective on blocking viral replication in CEF and chicken embryos.Four hours prior to infection with NDV,the CEF was transfected with the plasmids by Silent-fect.An unrelated shRNA sequence(HK)was used in mock transfection.The expression of a potent shRNA resulted in up to 2.3,21.1 and 9.8 fold decreases in NP gene expression at 3,6 and 9 h post infection in CEF,respectively.The ndv1 was able to completely inhibit the replication of the virus in CEF within 48 post infection.Furthermore,the pathological changes in CEF caused by NDV were delayed,and the degree of pathological changes was lighter compared with the mock transfection in the presence of ndv1.When the complex of shRNASilent-fect and NDV was co-injected into the allantoic cavity of 10-day-old embryonated eggs with 10^(5) or 10^(6) ELD50 NDV,NDV replication was decreased by 94.14% and 62.15% after 17 h,respectively.These findings suggest that the newly synthesized NP protein is critical for NDV transcription and replication and provide a basis for identifying the functions of viral genes and screening for effective siRNAs against viruses in CEF and chicken embryo by RNAi.

鸡胚成纤维细胞cDNA表达文库的构建

鸡胚成纤维细胞(CEF)是研究鸡传染性法氏囊病病毒(IBDV)的主要细胞材料,而构建CEF的cDNA表达文库是筛选IBDV在CEF中的细胞受体,研究细胞嗜性的基础平台。采用Gateway技术构建CEF的表达文库,避免使用限制性内切酶切割cDNA,能够解决常规方法构建cDNA文库的技术缺陷。该技术将CEF的mRNA分离纯化后,以5′端生物素标记的Oligo(dT)primer为引物反转录后连接Adapter,层析柱纯化,通过BP重组反应构建cDNA入门文库,其平均滴度为1.1×106cfu/mL,文库总容量为1.2×107cfu,平均插入片段为2243bp,重组率为100%。通过LR重组反应将入门文库转换为表达文库,经测定平均滴度为5×105cfu/mL,文库总容量为5.5×106cfu,平均插入片段为2411bp,重组率为100%。结果表明,所构建的文库具有较高的重组率和较大的库容量,可作为较高质量的文库来研究IBDV的相关基因,为研究病毒受体和病毒入侵途径,进一步了解IBDV的致病机理奠定了基础。

鸡胚成纤维细胞cDNA酵母表达文库的构建与鉴定

试验提取CEF细胞总RNA,运用SMART和LD-PCR技术合成cDNA,通过同源重组克隆入真核表达质粒pGADT7,转化酵母菌Y187,构建cDNA表达文库。文库滴度高达6.94×107cfu/mL,重组率达100%。随机挑选10个克隆进行测序,全部为原鸡序列。本研究为进一步研究重要禽源病毒与宿主细胞的相互作用奠定了基础。

传染性法氏囊病病毒在鸡胚细胞上的优化繁殖

研究了传染性法氏囊病病毒（ＩＢＤＶ）在鸡胚细胞上繁殖的优化条件，结果表明，鸡胚细胞体外增殖培养后对ＩＢＤＶ的敏感性并不减弱，而且有提高。维持培养基中血清浓度的变化（体积分数在０．０１～０．１０范围内）对病毒的繁殖影响不大。该病毒更适宜于稍偏酸性和较高温度下繁殖。

黄芪多糖和淫羊藿多糖对培养细胞增殖和衰老的影响

将安全浓度范围内的黄芪多糖(astragaluspolysaccharide,APS)和淫羊藿多糖(epimediumpolysaccharide,EPS)分别加入到培养12h和24h的鸡胚成纤维细胞(CEF)中,测定加药后CEF增殖率和成层率的动态变化。结果表明,2种多糖均能促进细胞增殖和延缓细胞衰老,EPS的作用强于APS,具有一定的量效、时效关系。

10种中药成分对鸡胚成纤维细胞生长的影响

将鸡胚成纤维细胞 ( CEF)分别与当归多糖 ( CAPS)、黄芪多糖 ( APS)、板蓝根多糖 ( IRPS)、淫羊藿多糖 ( EPS)、蜂胶多糖 ( PPS)、淫羊藿黄酮 ( EF)、蜂胶黄酮 ( PF)、黄芪黄酮 ( AF)、黄芪皂甙 ( AS)和人参皂甙 ( GS)等 10种中药成分一起加入到 96孔细胞培养板中培养 ,分别在培养 2 4、36、4 8、6 0、72 h时用 MTT法测定中药成分对 CEF增殖的影响。结果表明 ,所有中药成分均能显著促进 CEF增殖 。

鸡胚成纤维细胞原代培养及应用

原代培养是指在体外模拟体内生理环境,使从体内取出的组织细胞生存、生长和传代,并维持原有组织细胞的结构和功能特性。鸡胚成纤维细胞具有相对容易获得、增殖能力强、适应性强、良好的耐受性、性状比较稳定等特点,使得其被广泛地应用于分子和细胞生物学研究的许多方面。论文综述了近年来有关鸡胚成纤维细胞的培养技术,如鸡胚的取材、细胞的分离、纯化和培养,同时介绍了应用进展和未来研究方向。

短发夹结构RNA干扰新城疫病毒的增殖

以新城疫病毒(NDV)NP基因为标靶,构建3个细胞内表达发夹样结构小干扰RNA(shRNA)的质粒载体,在鸡胚成纤维细胞(CEF)和鸡胚上进行了RNAi试验,筛选出一个有效抑制病毒复制的小分子ndv1.用阳离子脂质体转染试剂Silent-fect将ndv1转染CEF,以不相关shRNA质粒载体HK为阴性对照,4h后接种NDV,与对照相比,干涉组在病毒感染后3hNP基因的表达量降低2.3倍,6h降低21.1倍,9h降低9.8倍;ndv1能在48h内完全阻断NDV在CEF中的增殖,延缓病变出现时间,减轻病变程度.将Silent-fect-ndv1混合物与NDV同时注入10日龄SPF鸡胚绒毛尿囊腔,能使105ELD50NDV感染后17h鸡胚尿囊液中病毒增殖量减少94.4%,使106ELD50 NDV感染后17h鸡胚尿囊液中病毒增殖量减少62.5%.实验结果证实,在CEF中存在RNAi机制,抑制ND VNP基因的表达能有效阻断该病毒增殖,说明NP基因在NDV复制过程中起重要作用.实验结果为进一步利用RNAi技术在CEF和鸡胚中研究病毒基因组功能及筛选抗病毒小分子奠定了基础.

中药成分对传染性法氏囊病毒感染细胞的影响

将黄芪多糖、当归多糖、蜂胶多糖、淫羊藿多糖、板蓝根多糖、黄芪黄酮、蜂胶黄酮、淫羊藿黄酮、黄芪皂甙、人参皂甙等 1 0种中药成分与鸡传染性法氏囊病毒 (IBDV)以 3种顺序加入到培养 2 4h的鸡胚成纤维细胞 (CEF)中。即先加中药后接种病毒、先接种病毒后加中药、中药和病毒同时加入 ,观察细胞病变的程度 ,以评价它们对IBDV感染细胞的影响。结果表明 ,先加中药后接种病毒和中药与病毒同时加入时 ,多数中药成分处理组在病毒接种后 72h的细胞病变程度明显减轻 ,表明多数中药能抑制病毒感染细胞 ,且有一定的量效和时效关系。

用ELISA检测传染性囊病病毒诱导的细胞凋亡

用5株传染性囊病病毒（IBDV）分别感染鸡胚成纤维细胞（CEF），于感染后不同时间收集接毒组与对照组的细胞进行检测．试验结果显示，接毒组与对照组细胞的DNA在琼脂糖凝胶电泳谱上均呈现梯状条带．用酶联免疫吸附试验（EUSA）检测各组细胞中降解DNA量，发现感染IBDV7h后，接毒组细胞降解DNA量比对照组明显增加，且各接毒组间降解DNA量有一定的差异．试验结果表明：各株IBDV均诱导CEF发生细胞凋亡，但不同IBDV毒株诱导细胞凋亡的能力有差异；ELISA是定量检测细胞凋亡的较好方法．