UL27、UL29基因shRNA表达载体的构建及对HSV-2的干扰效应研究

探讨Ⅱ型单纯疱疹病毒(Herpes simplex virus type 2,HSV-2)UL27、UL29基因联合靶向siRNA对HSV-2复制的影响。构建UL27、UL29基因的siRNA的重组表达载体并转染293细胞,通过实时荧光定量PCR技术和蛋白质印迹方法检测UL27、UL29基因的表达,终点滴定法检测细胞上清液中的各组病毒滴度,MTT法检测细胞的存活率。结果显示:(1)成功构建短发夹RNA(shRNA)重组表达载体。(2)转染后48 h,与空白组(空载体)相比,UL27 shRNA75组对UL27基因mRNA的抑制率为75.17%(P0.05),UL29 shRNA1461组对UL29基因mRNA抑制率为66.08%,具有显著性差异(P0.05)。UL27 shRNA75联合UL29 shRNA1461联合干扰组对UL27基因抑制率约为91.28%,UL29基因表达抑制率约为80.40%,与空白组比较具有显著性差异(P0.05)。(3)终点滴定法结果显示单干扰组和联合干扰组可不同程度降低上清液中的病毒感染滴度,与空白组比较差异性显著(P0.01)。(4)Western blot检测目的基因蛋白,单干扰组与联合干扰组可不同程度降低目的基因蛋白的表达,其中UL27shRNA75+UL29 shRNA1461联合干扰组能显著抑制相应的蛋白表达水平,蛋白表达量明显减少,与单干扰组相比具有显著差异(P0.05)。(5)经MTT法检测,UL27 shRNA75、UL29 shRNA1461、UL27 shRNA75+UL29 shRNA1461联合干扰组的细胞存活率明显提高,差异有显著意义(P0.05)。构建的pGPU6/GFP/Neo-UL27、pGPU6/GFP/Neo-UL29重组表达载体,能在体外细胞水平上不同程度的干扰HSV-2 UL27、UL29基因表达,UL27、UL29联合干扰效率更高,抑制HSV-2在HEK293细胞中复制。     

靶向UL27shRNA抑制Ⅱ型单纯疱疹病毒在HEK293细胞中的复制

按照shRNA(small hairpin RNA)设计原则,针对Ⅱ型单纯疱疹病毒(herpes simplex virus type 2, HSV-2)的UL27基因序列保守区域筛选设计、合成4条干扰靶序列并构建表达UL27序列特异性siRNA(short interfering RNA)的质粒载体pGPU6/GFP/Neo．通过脂质体介导重组表达载体转染HEK293细胞 (human embryonic kidney 293 cell)再接种HSV-2．采用实时荧光定量PCR(real-time fluorescent quantitative PCR)技术检测UL27各组的mRNA转录水平,终点滴定法检测细胞上清液中的病毒滴度,四甲基偶氮唑盐(four methyl thiazolyl tetrazolium, MTT)法测定细胞存活率,Western印迹法检测蛋白表达效果．结果显示,UL27shRNA75组对UL27基因mRNA表达抑制效果最佳,同时能显著抑制感染细胞的CPE(cytopathic effect, CPE),降低上清液中的病毒感染滴度,提高细胞的生存率,抑制UL27基因的蛋白表达．提示本研究构建的pGPU6/GFP/Neo-UL27表达载体能在细胞水平上不同程度地干扰HSV-2 UL27基因表达,抑制HSV-2在HEK293细胞中复制．     

敲减单纯疱疹病毒Ⅱ型（HSV-2）UL30蛋白表达可抑制HSV-2复制

按照shRNA（small hairpin RNA）设计要求,选择编码单纯疱疹病毒Ⅱ型DNA多聚酶催化亚单位的U_L30（unique long 30,U_L30）基因序列保守区域,设计、合成并构建表达U_L30序列特异性siRNA（short interfering RNA）的质粒载体pUL30．通过磷酸钙转染法将其转染入HEK（human embryonic kidney）293细胞中,用蛋白印迹法检测对HSV-2 UL30蛋白表达的影响,观察受染细胞病变效应（cytopathic effect,CPE）,终点滴定法测定细胞上清液中病毒感染滴度（50% tissue culture infective dose,TCID₅₀）．结果表明,针对U_L30基因的siRNA能有效抑制UL30蛋白表达,同时显著抑制受染细胞的CPE,降低上清液中病毒感染滴度．提示本研究建立的针对U_L30基因特异性siRNA能有效阻断HSV-2在HEK293细胞内的复制,U_L30基因是一个潜在的抗HSV-2复制的药物靶标．     

抑制Dicer基因对shRNA功能发挥的影响

本文将Dicer基因的RNA酶Ⅲ结构域作为靶区,设计并构建了两个抗Dicer基因的小发夹样RNA(shRNA)表达载体,将其转染2215、结肠癌TC细胞和基因组中整合有绿色荧光蛋白基因(GFP)的HepG2 A9细胞,通过RT-PCR评价RNA干扰抑制Dicer基因表达的效率;当HepG2 A9细胞Dicer基因表达被上述RNA干扰抑制时,再转染抗GFP的shRNA表达载体,通过RT-PCR和荧光显微镜观察GFP表达水平.结果显示,在不同细胞系中,这两个抗Dicer基因shRNA表达载体,均能明显抑制Dicer基因的表达;当Dicer基因受抑时,后续转染抗GFP的shRNA表达载体不能有效抑制GFP的表达.结果表明,抗Dicer基因shRNA表达载体,能够明显抑制Dicer基因的表达;shRNA表达载体的功能发挥需要Dicer酶的直接参与.     

siRNA干扰HSV-1 UL30 DNA聚合酶基因的研究

目的：筛选高效沉默HSV-1UL30基因的siRNA,研究siRNA沉默UL30基因后对HSV-1繁殖的影响。方法：设计并化学合成12对靶向UL30基因的siRNA,与pEGFP-N1-Fi融合表达质粒共转染VERO细胞,流式细胞术筛选高效抑制Fi-EGFP融合蛋白的siRNA,实时荧光定量PCR检测siRNA对感染细胞内UL30mRNA表达的抑制效果,CPE法和空斑减数实验评价siRNA对HSV-1繁殖的抑制效果。结果：共转染实验筛选出高效抑制Fi-EGFP融合蛋白的siRNA4、siRNA10及siRNA8,这3对siRNA均能显著降低感染细胞内UL30mRNA的表达水平及病变细胞释放到培养上清的子代病毒滴度,siRNA4和siRNA10在感染后36h对HSV-1的繁殖有明显的抑制效果,其病斑分别比对照组减少61.17%、51.46%（P〈0.05）,siRNA4、siRNA10及siRNA8组最终形成的空斑直径分别比对照组减小29.94%、23.49%、21.69%（P〈0.01）。结论：筛选到高效抑制UL30的3对siRNAs,siRNA4及siRNA10在病斑形成早期对HSV-1的繁殖有明显的抑制效果,说明siRNA4、siRNA10及siRNA8均能延缓病斑的扩大和病斑数目的增长,对病毒的繁殖有一定的抑制效果。     

抑制Dicer基因对shRNA功能发挥的影响

本文将Dicer基因的RNA酶III结构域作为靶区,设计并构建了两个抗Dicer基因的小发夹样RNA(shRNA)表达载体,将其转染2215、结肠癌TC细胞和基因组中整合有绿色荧光蛋白基因(GFP)的HepG2A9细胞,通过RT-PCR评价RNA干扰抑制Dicer基因表达的效率;当HepG2A9细胞Dicer基因表达被上述RNA干扰抑制时,再转染抗GFP的shRNA表达载体,通过RT-PCR和荧光显微镜观察GFP表达水平。结果显示,在不同细胞系中,这两个抗Dicer基因shRNA表达载体,均能明显抑制Dicer基因的表达;当Dicer基因受抑时,后续转染抗GFP的shRNA表达载体不能有效抑制GFP的表达。结果表明,抗Dicer基因shRNA表达载体,能够明显抑制Dicer基因的表达;shRNA表达载体的功能发挥需要Dicer酶的直接参与。     

特异性干扰ICP27基因的siRNA对HSV-1病毒复制的影响

针对单纯疱疹病毒1型(herpes simplex virus 1,HSV-1)的ICP27基因和其他疱疹病毒相关基因的高度保守区设计小干扰RNA(small interfering RNA,siRNA),研究其抑制病毒复制的效果。首先构建相应的小发夹RNA(small hairpin RNA,shRNA),然后通过病毒滴度测定、real-time PCR和细胞致病变效应(cytopathic effect,CPE)检测所设计的siRNA抑制病毒复制的能力。结果显示,所设计的shRNA-2(靶序列起始位置815)和shRNA-3(靶序列起始位置1 367)具有明显地抑制病毒复制的效果。尤其是shRNA-3,抑制病毒复制的效果更明显,在病毒滴度实验中,与阴性对照相比,其抑制倍数为81,同时可以下调ICP27基因的mR NA表达水平。实验结果表明shRNA-3能够显著抑制HSV-1病毒复制的能力,可以作为HSV-1感染性疾病的补充治疗手段,其对应的靶序列可以作为抗HSV-1新的靶标。     

细胞MEK1/2蛋白及其相关通路在单纯疱疹病毒Ⅱ型（HSV-2）复制中的作用

基于细胞Raf/MEK/ERK信号通路与病毒复制的关系,应用Western印迹检测 p-ERK1/2蛋白的表达、用终点滴定法测定病毒增殖量（TCID_５０）,以及观察感染细胞的细胞病变效应（CPE）等,揭示单纯疱疹病毒Ⅱ型(HSV-2)复制与 ERK通路的关系. 结果表明,HSV-2的复制可引起细胞ERK通路的活化;用U0126预先抑制ERK通路的活化,或用特异性siRNA敲减MEK1/2基因的表达可显著地抑制病毒复制.提示ERK信号通路以及MEK1/2蛋白对HSV-2的复制具有重要的作用.该研究对进一步阐明细胞ERK通路各激酶蛋白在病毒复制中的作用机制、寻找抗病毒作用靶标等奠定了良好的基础.     

shRNA表达载体构建方法的优化

目的探讨shRNA表达载体的构建方法 ,以加速RNA干扰研究的进程。方法对shRNA表达载体的构建过程进行分析和监测 ,并加以优化。结果发现shRNA表达载体构建的退火过程容易产生障碍 ,经优化退火缓冲液的NaCl含量后 ,能明显提高退火效率及shRNA表达载体构建的成功率。结论shRNA表达载体构建的退火过程需加以关注 ,退火缓冲液中NaCl含量应提高至 2 0 0mmol/L以上为宜     

neuronatin shRNA真核表达载体的构建及其生物学功能

目的:获得能持续干扰neuronatin（nnat）基因表达的细胞,观察nnat基因沉默对神经细胞发育与分化的影响,为研究基因功能奠定基础。方法:构建含nnat基因短发夹RNA(shRNA)表达质粒,将质粒转染大鼠肾上腺嗜铬细胞瘤细胞PC12,RT-PCR方法筛选出最有效干扰质粒,稳定转染PC12细胞后观察细胞表型变化,免疫荧光检测nnat蛋白表达,NGF诱导观察nnat表达下调对细胞分化的影响。结果:成功构建并筛选出有效的靶向nnat基因的shRNA真核表达载体;载体稳定转染PC12细胞之后能特异性沉默nnat基因的表达,PC12细胞长出突起,向神经元方向分化,加入诱导因子NGF后能促进突起生长。结论:nnat可能是作为神经分化抑制因子在神经发育与成熟过程中发挥作用。     

Determination of HSV-1 UL5 and UL29 gene copy numbers in an HSV complementing Vero cell line

The genetic stability of transgenes is a critical characteristic used to assess constructed cell lines used for vaccine production. The evaluation of gene copy numbers by a qPCR method, is one of the most common approaches used to assess the consistency of transgenes in a constructed cell line. The cell line AV529-19 is a Vero-based cell line specifically engineered to express the HSV-1 UL5 and UL29 open reading frames. AV529-19 is used to support the replication of a defective HSV-2 viral candidate vaccine called HSV529. To assess the genetic stability of the UL5 and UL29 transgenes in AV529-19 cells, a digital PCR-based approach was developed. During characterization of the test method, the specificity, accuracy, and intermediate precision of the assay was investigated based on regulatory guidelines. The developed assay was used to monitor the stability of the transgenes in the manufactured AV529-19 cell lines by comparison of transgene copy numbers in the master cell bank (MCB) with their copy numbers in the extended cell bank (ECB). Results showed that the UL29 and UL5 transgenes are stable in that there are one and three copies of the UL29 and UL5 genes, respectively, per cell in both the AV529-19 MCB and ECB.     

Allosteric signaling and a nuclear exit strategy: binding of UL25/UL17 heterodimers to DNA-Filled HSV-1 capsids

UL25 and UL17 are two essential minor capsid proteins of HSV-1, implicated in DNA packaging and capsid maturation. We used cryo-electron microscopy to examine their binding to capsids, whose architecture observes T = 16 icosahedral geometry. C-capsids (mature DNA-filled capsids) have an elongated two-domain molecule present at a unique, vertex-adjacent site that is not seen at other quasiequivalent sites or on unfilled capsids. Using SDS-PAGE and mass spectrometry to analyze wild-type capsids, UL25 null capsids, and denaturant-extracted capsids, we conclude that (1) the C-capsid-specific component is a heterodimer of UL25 and UL17, and (2) capsids have additional populations of UL25 and UL17 that are invisible in reconstructions because of sparsity and/or disorder. We infer that binding of the ordered population reflects structural changes induced on the outer surface as pressure builds up inside the capsid during DNA packaging. Its binding may signal that the C-capsid is ready to exit the nucleus.     

Construction, phenotypic analysis, and immunogenicity of a UL5/UL29 double deletion mutant of herpes simplex virus 2

A number of studies have shown that replication-defective mutant strains of herpes simplex virus (HSV) can induce protective immunity in animal systems against wild-type HSV challenge. However, all of those studies used viruses with single mutations. Because multiple, stable mutations provide optimal levels of safety for live vaccines, we felt that additional mutations needed to be engineered into a candidate vaccine strain for HSV-2 and genital herpes. We therefore isolated an HSV-2 strain with deletion mutations in two viral DNA replication protein genes, UL5 and UL29. The resulting double deletion mutant virus strain, dl5-29, fails to form plaques or to give any detectable single cycle yields in normal monkey or human cells. Nevertheless, dl5-29 expresses nearly the same pattern of gene products as the wild-type virus or the single mutant viruses and induces antibody titers in mice that are equivalent to those induced by single deletion mutant viruses. Therefore, it is feasible to isolate a mutant HSV strain with two mutations in essential genes and with an increased level of safety but which is still highly immunogenic.     

Comparison of the host immune response to herpes simplex virus 1 (HSV-1) and HSV-2 at two different mucosal sites

A study was undertaken to compare the host immune responses to herpes simplex virus 1 (HSV-1) and HSV-2 infection by the ocular or genital route in mice. Titers of HSV-2 from tissue samples were elevated regardless of the route of infection. The elevation in titers of HSV-2, including cell infiltration and cytokine/chemokine levels in the central nervous system relative to those found following HSV-1 infection, was correlative with inflammation. These results underscore a dichotomy between the host immune responses to closely related alphaherpesviruses.     

Molecular determinants responsible for the subcellular localization of HSV-1 UL4 protein

The function of the herpes simplex virus type 1 (HSV-1) UL4 protein is still elusive. Our objective is to investigate the subcellular transport mechanism of the UL4 protein. In this study, fluorescence microscopy was employed to investigate the subcellular localization of UL4 and characterize the transport mechanism in living cells. By constructing a series of deletion mutants fused with enhanced yellow fluorescent protein (EYFP), the nuclear export signals (NES) of UL4 were for the first time mapped to amino acid residues 178 to 186. In addition, the N-terminal 19 amino acids are identified to be required for the granule-like cytoplasmic pattern of UL4. Furthermore, the UL4 protein was demonstrated to be exported to the cytoplasm through the NES in a chromosomal region maintenance 1 (CRM1)-dependent manner involving RanGTP hydrolysis.     

Interactions of the HSV-1 UL25 Capsid Protein with Cellular Microtubule-associated Protein

An interaction between the HSV-1 UL25 capsid protein and cellular microtubule-associated protein was found using a yeast two-hybrid screen and β-D-galactosidase activity assays. Immunofluorescence microscopy of the UL25 protein demonstrated its co-localization with cellular microtubule-associated protein in the plasma membrane. Further investigations with deletion mutants suggest that UL25 is likely to have a function in the nucleus.     

Molecular Determinants Responsible for the Subcellular Localization of HSV-1 UL4 Protein

The function of the herpes simplex virus type 1(HSV-1)UL4 protein is still elusive. Our objective is to investigate the subcellular transport mechanism of the UL4 protein. In this study,fluorescence microscopy was employed to investigate the subcellular localization of UL4 and characterize the transport mechanism in living cells. By constructing a series of deletion mutants fused with enhanced yellow fluorescent protein(EYFP),the nuclear export signals(NES)of UL4 were for the first time mapped to amino acid residues 178 to 186. In addition,the N-terminal 19 amino acids are identified to be required for the granule-like cytoplasmic pattern of UL4.Furthermore,the UL4 protein was demonstrated to be exported to the cytoplasm through the NES in a chromosomal region maintenance 1(CRM l)-dependent manner involving RanGTP hydrolysis.     

Interactions of the HSV-1 UL25 capsid protein with cellular microtubule-associated protein

An interaction between the HSV-1 UL25 capsid protein and cellular microtubule-associated protein was found using a yeast two-hybrid screen and β-D-galactosidase activity assays. Immunofluorescence microscopy of the UL25 protein demonstrated its co-localization with cellular microtubule-associated protein in the plasma membrane. Further investigations with deletion mutants suggest that UL25 is likely to have a function in the nucleus.