Packaging and Functional Identification of Recombinant Adeno-associated Virus Encoding cdc2-siRNA

Cyclin dependent kinases （cdks） play an important role in the pathogenesis of multiple neurodegenerative diseases. To explore the possibility of cdks-related gene therapy for neurodegen-erative diseases, we packed recombinant adeno-associated virus （rAAV） encoding cdc2-siRNA. The expressing plasmid pAAV-MCS-EGFP-U6-cdc2-siRNA was constructed by using molecular biological techniques. The rAAV encoding cdc2-siRNA （rAAV-EGFP-U6-cdc2-siRNA） was packed by calcium phosphate mediated co-transfection of the plasmid pAAV-MCS-EGFP-U6-cdc2-siRNA, p-RC and p-Helper into AAV-293 cells. DNA sequencing proved the successful construction of U6-cdc2-siRNA in pAAV-MCS-EGFP. Seventy-two h after packaging, the expression of EGFP could be detected in AAV-293 cells. Western blotting revealed that cdc2 gene expression in AAV-293 cells was down-regulated markedly after transfection with rAAV-EGFP-U6-cdc2-siRNA, which evidenced the satisfactory silencing effect of this virus. It was concluded that the packaging of rAAV encoding cdc2-siRNA was successful. rAAV encoding cdc2-siRNA could silence cdc2 gene effectively, which might offer a novel means for the treatment of neurodegenerative diseases.

Recombinant adeno-associated virus delivered human thioredoxin-PR39 prevents hypoxia-induced apoptosis of ECV304 cells

Human thioredoxin and antibacterial peptide, PR39, have been shown to have potent antioxidant effects that may prolong survival of cells during hypoxia. The pSSCMV/human thioredoxin-PR39 vector was successfully constructed in this study and used to infect ECV304 cells. Transfected ECV304 cells were incubated at 1%, 5% hypoxic, and normal oxygen conditions. We found that the number of apoptotic cells after transfection with recombinant adeno-associated virus-human thioredoxin -PR39 was significantly lower than controls, suggesting a protective effect of the recombinant human thioredoxin-PR39 protein on hypoxic cells.

The Helper Activities of Different Avian Viruses for Propagation of Recombinant Avian Adeno-Associated Virus

To compare the helper activities of different avian viruses for propagation of recombinant avian adeno-associated virus （rAAAV）, AAV-293 cells were cotransfected with the AAAV vector pAITR-GFP containing green fluorescent protein （GFP） gene, the AAAV helper vector pcDNA-ARC expressing the rep and cap genes, and the adenovirus helper vector pHelper expressing Ad5 E2A, E4, and VA-RNA genes. Chicken embryonic fibroblast （CEF） or chicken embryonic liver （CEL） cells were cotransfected with the AAAV vector and the AAAV helper vector, followed by infection with Marek＇s disease virus （MDV）, avian adenovirus, chicken embryo lethal orphan （CELO） virus or infectious bursal disease virus （IBDV）. Infectious rAAAV particles generated by the two strategies were harvested and titrated on CEF and CEL cells. A significantly higher viral titer was obtained with the helper activity provided by the pHelper vector than by MDV or CELO virus. Further experiments showed that rAAAV-mediated green fluorescent protein （gfp） expression was overtly enhanced by MDV or CELO virus super infection or treatment with sodium butyric acid, but not by IBDV super infection. These data demonstrated that MDV and CELO viruses could provide weak helper activity for propagation of rAAAV, and rAAAV- mediated transgene expression could be enhanced by super infection with the helper viruses.

A novel method for purification of recombinant adeno-associated virus vectors on a large scale

A novel method for recombinant adeno-associ-ated virus (rAAV) purification on large scale is described. The method involves three steps, including chloroform treatment, PEG/NaCl precipitation and chloroform extraction. The whole procedure can be performed in four hours. Using this purification method, we can reproducibly obtain, from 4 × 109 of proviral cells cultured in roller bottles, purified rAAV-GFP stocks with titers of around 5×1013 particles/mL and purity greater than 95%. The infectious titers of the vector stocks were up to 2×1012 TU/mL, thus particle-to-infectivity rate was about 25. Under an electronic microscope, most rAAV particles appeared full and a few were in intermediate form. Empty particles were rarely seen. The purified rAAV-GFP stocks have been successfully used in in vitro and in vivo transfection experiments. Therefore, this new method offers a simple, rapid and cost-effective way for large-scale rAAV purification.

A novel and highly efficient production system for recombinant adeno-associated virus vector

Recombinant adeno-associated virus(rAAV) has proven to be a promising gene delivery vector for human gene therapy. However, its application has been limited by difficulty in obtaining enough quantities of high-titer vector stocks. In this paper, a novel and highly efficient production system for rAAV is described. A recombinant herpes simplex virus type 1(rHSV-1) designated HSV1-rc/△UL2, which expressed adeno-associated virus type2(AAV-2) Rep and Cap proteins, was constructed previously. The data confirmed that its functions were to support rAAV replication and packaging, and the generated rAAV was infectious. Meanwhile, an rAAV proviral cell line designated BHK/SG2, which carried the green fluorescent protein(GFP) gene expression cassette, was established by transfecting BHK-21 cells with rAAV vector plasmid pSNAV-2-GFP. Infecting BHK/SG2 with HSV1-rc/△UL2 at an MOI of 0.1 resulted in the optimal yields of rAAV, reaching 250 transducing unit(TU) or 4.28×104 particles per cell. Therefore, compared with the conventional transfection method, the yield of rAAV using this "one proviral cell line, one helper virus" strategy was increased by two orders of magnitude. Large-scale production of rAAV can be easily achieved using this strategy and might meet the demands for clinical trials of rAAV-mediated gene therapy.

腺相关病毒感染GDF11对2型糖尿病大鼠血管损伤的保护作用

目的探讨腺相关病毒感染上调体内生长和分化因子11(GDF11)表达水平对2型糖尿病大鼠(T2DM)主动脉损伤的影响。方法随机选取9周龄雄性SD大鼠,采用高糖高脂饲料加小剂量链脲佐菌素(STZ)联合诱导,建立T2DM模型。正常大鼠和糖尿病模型大鼠随机分为5组:空白对照组(Control组)、阴性病毒对照组(NC组)、GDF11腺相关病毒组(GDF11组)、糖尿病组(DM组)、糖尿病+GDF11腺相关病毒组(DM+GDF11组)。喂养8周后,检测大鼠血清中胰岛素(INS)、晚期糖基化终末产物(AGES)、重组生长转化因子11(GDF11)、总胆固醇(T-CHO)、三酰甘油(TG)、低密度脂蛋白(LDL-C)、高密度脂蛋白(HDL-C)、不对称二甲基精氨酸(ADMA)、丙二醛(MDA)浓度;采用过碘酸雪夫氏染色(PAS染色)观察糖原沉积部位,苏木精-伊红染色(HE)观察血管损伤情况,扫描电镜观察血管内皮细胞和血管弹性纤维损伤情况,蛋白印迹和免疫组化检测血管损伤相关蛋白的表达水平。结果在动物实验中与Control组相比,生化指标提示:DM组大鼠血清中AGES、T-CHO、TG、LDL-C和MDA浓度升高(P<0.05),INS、GDF11、HDL-C、ADMA显著低于Control组(P<0.05),DM+GDF11组AGES和HDL-C与DM组无明显差异,T-CHO、TG、LDL-C和MDA相比较DM组降低(P<0.05),INS、GDF11和ADMA相比较DM组升高(P<0.05)。病理染色提示:DM组PAS染色提示糖原颗粒在主动脉内皮及内皮下沉积,HE染色观察到主动脉中膜增厚,内皮细胞及弹性纤维断裂走形不规则,电镜观察到DM组血管内皮损伤,弹性纤维断裂,DM+GDF11组这些变化有所减轻。蛋白印迹和免疫组化表示内皮细胞相关蛋白在DM组中表达下降(P<0.05),间充质标志物在DM组中表达升高(P<0.05),DM+GDF11组中这些蛋白有所回调,且差异有统计学意义(P<0.05)。结论提高体内GDF11表达水平可以改善糖尿病导致的主动脉血管损伤,推断可能与其抑制内皮间充质转化保护血管内皮细胞的功能从而改善血管损伤有关。

基于hACE2转导建立SARS-CoV-2 spike假病毒感染病证结合的小鼠病毒肺炎模型

目的建立与评价一种安全、经济、有效的病证结合小鼠新冠病毒感染肺炎模型。方法30只KM种小鼠随机分为空白组、对照组及实验1组、实验2组、实验3组,每组各6只。每天把KM小鼠置于模拟寒湿环境中4 h,将表达hACE2的重组腺相关病毒(pAAV-hACE2)采用改良悬挂法气管内给药转导至肺组织,继以新型冠状病毒(SARS-CoV-2)spike假病毒采用相同的气管内给药方式造模。观察各组小鼠一般情况,检测体重变化、肺指数、血清炎性因子及肺部病理变化。结果免疫组化法显示h ACE2在小鼠肺组织中有效表达;在寒湿环境中给予SARS-CoV-2 spike假病毒后,实验组小鼠表现出类似疫毒犯肺证候的体征;且同样喂养条件和时间下,与空白组和对照组小鼠比较,实验组小鼠出现体重下降;实验1、2、3组小鼠出现肺指数显著增大(P<0.05或P<0.01),血清炎性因子白细胞介素-1β(IL-1β)、白细胞介素-6(IL-6)、白细胞介素-8(IL-8)、肿瘤坏死因子-α(TNF-α)显著升高(P<0.01),肺组织病理改变明显。结论本研究成功建立了一种安全、经济、有效的病证结合小鼠新冠病毒感染肺炎模型。

Prevalence of neutralizing antibodies against liver-tropic adeno-associated virus serotype vectors in 100 healthy Chinese and its potential relation to body constitutions

Recombinant adeno-associated virus （rAAV） serotype 2, 3 and 8 vectors are the most promising liver- tropic AAV serotype vectors. Liver diseases are significant problems in China. However, to date, few studies on AAV neutralizing antibodies （Nabs） were working with the Chinese population or with the rAAV3 vectors. The present study aimed to determine the prevalence of Nabs in Chinese population against wild-type AAV2, AAV3 and AAV8 capsids as well as additional two AAV3 variants. In addition, we performed a preliminary analysis to investigate the potential influence of traditional Chinese medicine body constitutions on AAV Nabs. Our work demonstrated that the majority of healthy Chinese subjects were positive for AAV Nabs, with the order of AAV2 〉 AAV3 = AAVLK03 〉 AAV8. There was no difference between： 1）AAV3 and its variants; 2） male and female subjects; and 3） different age cohorts （〈 35, 36- 50, and 〉 51 years old）. People in the Qi-deficiency constitution had significantly increased AAV8 Nabs than people in the Gentleness constitution. Our studies may have impact on the future clinical design of AAV-based gene therapy in the Chinese population.

rAAV在遗传性耳聋治疗中的研究进展

据世界卫生组织2021年报道,50%以上先天性听力损失是由遗传性因素变异引起的。临床上用于提高耳聋患者听力的几种主要方式(如佩戴助听器、植入人工耳蜗)都有一定局限性。近年来,重组腺相关病毒(recombination adeno-associated virus,r AAV)作为相对安全的基因治疗载体在遗传性疾病的临床及基础研究中被广泛应用。单r AAV由于包装载体大小受限,在大基因片段缺陷造成的疾病研究与治疗中的应用受限。目前已有团队开发了双重r AAV用于治疗大基因片段缺陷造成的疾病。文章着重介绍了双重r AAV在大基因片段缺陷造成的耳聋中的研究进展,为将来开发更多耳聋基因治疗r AAV提供帮助。

Construction and Detection of a Novel Type of Recombinant Human rAAV2/2-ND4

Purpose:To construct a novel AAV-mediated gene delivery of the human ND4 complex I subunit and to detect its expression level in mitochondria for potential application in gene therapy for Leber's hereditary optic neuropathy (LHON). Methods:A novel type of normal human ND4 gene was synthesized artificially to contain a mitochondrial targeting sequence that induces the translocation of this gene into mitochondria.This recombinant adeno-associated virus type 2/serotype 2 (rAAV2/2)-mediated NADH dehydrogenase subunit 4 (ND4) gene was constructed, purified, condensed, and amplified by PCR.The physical titer of rAAV2/2-ND4 was determined by slot-blot hybridization using a digoxigeninlabeled H1 probe.Expression of ND4 in mitochondria was evaluated by immunofluorescence. Results: The constructed rAAV2/2-ND4 specifically amplified the target gene band of ND4 and the physical titer of ND4 gene was 1.0×1011 vg/mL,confirming that the recombinant adenovirus vector contained the ND4 target gene. Expression of the ND4 gene was detected in mitochondria by immunofluorescence. Conclusion:A new type of rAAV2/2-ND4 was successfully constructed and may have potential in gene therapy for LHON.

大鼠内侧隔核谷氨酸能神经元的纤维投射

目的:通过立体定位注射重组腺相关病毒(rAAV)方法观察大鼠内侧隔核(MS)中谷氨酸能神经元的纤维投射。方法:将rAAV2/9-CaMKⅡa-EGFP、rAAV/retro-hSyn-mCherry病毒混合后注射到大鼠MS,待病毒在大鼠体内表达3周后灌注取脑、切片观察,检测MS的纤维投射情况。结果:rAAV2/9-CaMKⅡa-EGFP病毒主要标记到齿状回、黑质、红核、丘脑、乳头体上核,海马的CA2、CA3区;rAAV/retro-hSyn-mCherry病毒主要标记到背侧海马和内梨形背侧核、伏核神经元,少部分标记到第一躯体感觉皮层、第二视皮质和海马的CA1区神经元。结论:大鼠MS谷氨酸能神经元投射的脑区主要在边缘系统、基底节区以及海马,海马和部分皮层有纤维投射到MS。

重组腺相关病毒基因药物临床前评价方法的回顾与展望

重组腺相关病毒(rAAV)基因药物在临床应用过程中长期疗效不确定,甚至存在安全性风险,是制约其广泛应用的主要障碍.对现有rAAV基因药物临床前评价方法进行分析和梳理.结果表明:仅进行药效学评价不能揭示rAAV转导的细胞和分子机制,而基于转导过程分析的物理转导与功能转导评价存在结果不一致,不能反映rAAV转导的细胞异质性和靶细胞的空间分布特征等问题,难以准确预测rAAV基因药物的临床疗效和安全性,需要从单分子、单细胞水平开展rAAV载体胞内命运评价的新方法,以切实保障新型rAAV基因药物的临床有效性和安全性.

西多福韦促进2型重组腺相关病毒体外转导分析

为研究小分子药物西多福韦(CDV)对2型重组腺相关病毒(rAAV2)体外转导效率的影响,采用不同剂量CDV干预rAAV2-GFP和rAAV2-LacZ载体转导Hela细胞,从转基因表达量、阳性细胞数量、胞内病毒基因组数等方面研究CDV对rAAV2转导的影响.结果表明,CDV能促进rAAV2体外转导Hela细胞,转基因表达量、阳性细胞数、胞内病毒基因组数与对照组相比,差异具有统计学意义,且其促进作用呈现一定的剂量和时间依赖性.

导入酵母NDI1基因减少鱼藤酮诱导的分化型帕金森病细胞模型的损伤

目的探讨导入酵母NDI1基因能否替代人功能缺陷的线粒体复合体Ⅰ,为复合体Ⅰ功能障碍所致散发型帕金森病(PD)的基因治疗提供研究基础。方法将表达酵母NDI1的重组腺相关病毒(rAAV-NDI1)感染鱼藤酮诱导的分化型帕金森病细胞模型。设DMSO+空载、鱼藤酮+空载、鱼藤酮+NDI1共3组。用Western blot、免疫荧光染色、氧耗测定、ATP含量测定、ROS测定等方法检测细胞病理学、线粒体功能方面指标。结果鱼藤酮+NDI1组较鱼藤酮+空载组,细胞形态明显改善,细胞存活率显著上升(P<0.05),pS129α-突触核蛋白、全细胞自噬显著下降(P<0.05,P<0.001);复合体Ⅰ依赖性氧耗显著升高(P<0.01),细胞总ATP合成、线粒体氧化磷酸化偶联的ATP合成显著上升(P<0.01),线粒体ROS、线粒体自噬显著降低(P<0.01,P<0.001)。结论导入酵母NDI1基因可以在鱼藤酮诱导的分化型帕金森病细胞模型中,替代性弥补复合体Ⅰ的功能缺陷,对细胞病理学、线粒体功能的损伤具有改善作用。

三种逆行示踪工具标记小鼠前扣带回皮质传入核团的比较

目的:通过对小鼠前扣带回皮层(ACC)立体定位注射重组腺相关病毒(rAAV2⁃retro)、荧光乳胶微球(retrobeads)及狂犬病毒(RV)的方法,比较三种逆行示踪工具对ACC上游传入核团的标记效果。方法:将rAAV2⁃retro⁃hSyn⁃EGFP⁃P2A⁃Cre⁃WPRE⁃hGH⁃PA、retrobeads(Red)等量混合后注射到小鼠ACC脑区,待病毒表达3周后灌注取脑、切片观察。另外将rAAV2/9⁃EF1α⁃DIO⁃oRVG(19G)、rAAV2/9⁃EF1α⁃DIO⁃NLS⁃mCherry⁃P2A⁃TVA⁃T2A⁃RVG、rAAV2/9⁃CaMKIIα⁃Cre混合后注射到小鼠ACC脑区,待病毒表达2周后将RV⁃EnvA⁃ΔG⁃EGFP注射到相同部位,1周后灌注取脑、切片观察,比较三种策略标记到ACC上游传入核团的神经元数量及形态。结果:retrobeads标记到的核团最多,但无法标记神经元形态及树突结构;RV标记到的核团数量次之,胞体及树突结构标记完整,而且可以观察到清晰的树突棘;rAAV2⁃retro标记到的核团最少,能标记到树突,但无法标记树突棘。三者在内侧眶皮层、腹侧眶皮层、视皮层等区域均能够高效标记。其中,RV在丘脑腹前核和腹外侧核标记效率高于其他两种工具。结论:ACC接受脑内的广泛投射,而三种逆行示踪剂在标记效率和标记神经元结构完整性上各有优劣。

CD151对人舌鳞癌细胞Tca8113迁移作用的影响

背景与目的:CD151在肿瘤组织中的高表达与肿瘤的转移和预后密切相关,但其具体机制尚不清楚。本研究旨在探讨携带全长正义和反义CD151基因的重组腺相关病毒(rAAV-CD151,rAAV-antiCD151)对人舌鳞癌细胞Tca8113细胞迁移的影响。方法:利用含酶切位点的PCR引物克隆CD151基因,分别呈正向和反向插入包装质粒pAAV,并包装成rAAV-CD151,rAAV-antiCD151,斑点杂交测定病毒滴度;rAAV-CD151与rAAV-antiCD151分别转染Tca8113细胞2周后,Westernblot检测CD151表达,通过Boyden趋化小室研究其对Tca8113细胞迁移的影响。结果:斑点杂交结果显示rAAV-CD151和rAAV-antiCD151病毒滴度分别为2.0×1011pfu/ml,1.0×1011pfu/ml;转染rAAV-CD151后,Tca8113细胞CD151的表达较未转染组增加了108%,细胞迁移数(93.6±11.6)显著高于未转染组和转染rAAV-GFP对照组(53.0±6.6和46.0±7.0,P<0.05);转染rAAV-antiCD151后,Tca8113细胞CD151的表达较未转染组减少了79%,细胞迁移数(24.0±4.4)显著低于未转染组和转染rAAV-GFP对照组(P<0.05)。结论:CD151在肿瘤细胞的迁移中起重要的作用,是肿瘤转移的重要分子基础。携带反义CD151基因的重组腺相关病毒作为一种新的治疗工具,可以特异性阻断肿瘤细胞CD151表达,抑制肿瘤细胞的迁移。

HIV-1B亚型gp120基因密码子优化前后免疫原性的比较

对HIV 1B亚型gp120基因按照哺乳动物优势密码子的使用原则进行优化,以Westernblot方法比较其体外表达量。将优化前的野生型gp120基因和改造后的modgp120基因插入重组腺伴随病毒载体,构建了重组病毒rAAV wtgp120和rAAV modgp120,比较两者免疫Balb/C小鼠后的抗体和CTL应答。Westernblot检测结果显示:优化后基因的体外表达量明显高于野生型基因,rAAV modgp120与rAAV wtgp120相比可更好地诱导Balb/C小鼠的CTL应答,但检测不到明显的抗体反应。由此得出结论,优化后gp120基因的体外表达量明显高于野生型基因,并且可以诱导更强的特异性CTL应答,但检测不到gp120抗体。

表达绿色荧光蛋白报告基因重组禽腺联病毒载体系统的构建与鉴定

为了开展重组禽腺联病毒(Recombinant avian adeno-associated virus,rAAAV)介导的基因转移研究,用限制性内切酶消化含AAAV全基因组的重组质粒pCR-AAAV,去除AAAV Rep和Cap蛋白编码序列,将PCR扩增的绿色荧光蛋白(Green fluorescent protein,GFP)报告基因插入AAAV末端反向重复序列(Inverted terminal re-peats,ITR)之间,获得表达GFP基因的AAAV转移载体pAITR-GFP;以含AAAV全基因组的质粒为模板,用PCR分别扩增AAAV Rep、Cap和Rep-Cap蛋白基因,将Rep和Cap基因分别插入真核细胞双表达载体pVITRO2-mcs的两个多克隆位点,将Rep-Cap蛋白基因插入真核细胞表达载体pcDNA3,获得AAAV辅助质粒pVITRO2-ARC和pcDNA-ARC;将pAITR-GFP、pVITRO2-ARC或pcDNA-ARC与腺病毒辅助质粒pHelper组成三质粒转染系统,用磷酸钙沉淀法共转染AAV-293细胞,获得了表达GFP的rAAAV。经SDS-聚丙烯酰胺凝胶电泳分离后,纯化病毒出现分子量正确的VP1、VP2、VP3结构蛋白;经PCR检测证明,重组病毒中含有GFP报告基因;用重组病毒分别感染鸡胚成纤维细胞(CEF)和鸡胚肝CEL细胞,可以观察到GFP报告基因的表达,表达时间持续两周以上。这些试验结果表明,成功建立了辅助病毒非依赖性rAAAV体外包装体系,为禽源细胞的基因转移研究和禽重组活载体疫苗的研制打下了基础。

系列腺病毒伴随病毒载体的构建及表达β-半乳糖苷酶的研究

为了便于开展用重组腺病毒伴随病毒 (recombinantadeno associatedvirus,rAAV)载体进行基因治疗的研究 ,构建了三种通用型AAV载体 pWAV 1、pWAV 2和 pSNAV ,每种载体均含有AAV 2两端的倒转末端重复序列 (in vertedterminalrepeats,ITR) ,中间依次为巨细胞病毒 (CMV)立早增强子和启动子、多克隆位点和 polyA信号。研究者只需将目的基因正向插入多克隆位点 ,即可获得具有完整表达盒的AAV载体质粒。pWAV 1的多克隆位点包括NheⅠ、XhoⅠ、PstⅠ和BamHⅠ ,可插入外源基因的最大容量为 3 3kb ;pWAV 2的多克隆位点为 Kpn Ⅰ、EcoRⅠ、SalⅠ ;pSNAV的多克隆位点为Kpn Ⅰ、EcoRⅠ、SalⅠ和 BglⅡ ,二者所能装载的外源基因容量均为3 6kb。同时 ,还构建了携带 β 半乳糖苷酶基因的AAV载体 pAV lacZ、pSNAV lacZ ,并对制备rAAV的常规方法———共转染法进行了改进。用先前报道的具有rAAV包装功能的一种重组单纯疱疹病毒 (recombinantherpessim plexvirus,rHSV)分别感染经pAV lacZ、pSNAV lacZ转染的BHK 2 1细胞 ,可获得携带 β 半乳糖苷酶基因的rAAV ,滴度达到 5× 10 4 转导单位 (TU) /ml,为实现“一种病毒感染一个载体细胞株”

重组腺相关病毒:很有潜力的基因治疗载体

腺相关病毒(AAV)是细小病毒家族的一员,为无包膜的线性单链DNA病毒.由于AAV具有长期潜伏于人体而不具有任何明显致病性等优点,人们对AAV作为一种理想的基因治疗载体给予了很大期望.但是,近来发现,这类载体在应用上有许多明显的缺陷,包括某些细胞膜上病毒受体数量极少,重组AAV载体位点特异性整合不足,AAV衣壳成分和转基因产物引起宿主的免疫反应等等.这些缺陷促使人们加大对AAV生物学特性和转染过程的研究,从而更好地对AAV载体进行改进,使新一代重组AAV载体具备基因治疗所必需的安全性、高效性和靶向性,以期更广泛地应用于临床.