逆转录病毒介导的小干扰RNA稳定抑制了LRP16基因表达

RNA干涉是近年被广泛关注的一项技术,通过19～21nt的双链核酸介导使靶基因mRNA特异降解,目前已被广泛应用于细胞水平的基因功能研究。通过沉默LRP16基因表达介绍一项利用逆转录病毒介导发夹环样小干扰RNA的策略。首先选择了LRP16基因mRNA翻译起始位点下游 374nt和 668nt位置分别作为小干扰RNA作用靶位点,通过设计21nt的反义序列,构建了pL374和pL6682个以pLPC为骨架的逆转录病毒载体,针对绿色荧光蛋白序列构建pGFPi载体做阴性对照,茎环样结构小RNA由U6启动子驱动转录生成。3个载体分别与VSVG共转染293GP2细胞,包装假病毒,再分别感染MCF-7细胞,嘌呤霉素筛选获得稳定生成小干扰RNA的细胞。Northern blot实验表明pL374和pL668可分别将LRP16基因抑制90％和60％,为进一步研究LRP16基因功能奠定了基础。另外,首次将mU6启动子序列插入pLPC逆转录病毒载体骨架,将其改造为可介导发夹环样小干扰RNA产生的质粒载体。     

小干扰RNA抑制LRP16基因表达限制了MCF-7乳腺癌细胞增殖

雌激素雌二醇上调人乳腺癌细胞MCF 7中LRP16基因表达 ,该基因过表达促进MCF 7细胞增殖 .为进一步探讨LRP16基因不同表达水平对MCF 7细胞增殖的影响以及对雌激素的反应性增殖能力 ,采用针对LRP16基因特异的小干扰RNA策略 ,通过逆转录病毒介导及抗性筛选构建了LRP16基因被稳定抑制的 2个MCF 7细胞系 ,针对绿色荧光蛋白的干扰序列作为阴性对照 .Northern印迹实验检测了LRP16基因在各个细胞株中mNRA的水平 ,与对照组细胞比较 ,针对LRP16基因不同位置的 2个小干扰RNA可分别将该基因抑制 90 %和 6 0 % .细胞增殖试验结果显示 ,MCF 7细胞中LRP16基因表达抑制率越高 ,细胞增殖速率减慢越显著 (P <0 0 5 ) ;软琼脂集落形成试验结果显示 ,抑制LRP16基因在MCF 7细胞中表达 ,限制了细胞锚定非依赖性生长 ;细胞周期分析结果表明 ,LRP16基因抑表达使MCF 7细胞G1 S周期转换受抑 ;Western印迹结果表明 ,LRP16基因表达抑制的细胞中细胞周期蛋白E及细胞周期蛋白D1蛋白水平显著下调 ,但未检测到P5 3及Rb蛋白表达水平的影响 .雌二醇刺激的增殖实验结果显示 ,抑制LRP16基因表达没有消除MCF 7细胞的反应性增殖特征 .上述结果表明 ,LRP16基因表达量与MCF 7细胞增殖能力密切相关 ,抑制其表达可有效限制MCF 7细胞的增殖能力 ,提     

LRP16短发夹RNA慢病毒载体的构建及LRP16稳定抑制细胞的建立简

目的：构建靶向LRPl6基因的短发夹RNA（shRNA）慢病毒表达载体,鉴定其在HeLa细胞中对LRP16的抑制效果。方法：构建pWPT-U6-LRPl6shRNA-CMV-GFP慢病毒载体,通过病毒感染、细胞筛选、Western印迹等步骤,获得LRP16基因稳定抑制的细胞株。结果：构建了具有LRP16干扰效果的慢病毒载体,感染HeLa细胞后获得了稳定沉默LRP16及对照的细胞株;经克隆筛选,在荧光显微镜下观察到近似100％感染细胞发出绿色荧光;Western印迹证实pWPT-U6-L374-CMV-GFP和pWPT-U6-L668-CMV-GFP均可显著抑制HeLa细胞株中LRP16蛋白的表达,其中pWPT-Gsi-L374-GFP的抑制效果更好。结论：构建了靶向人LRP16基因shRNA慢病毒载体及LRP16稳定抑制的HeLa细胞系。     

LRP16对乳腺癌MCF-7细胞增殖的影响

用Northern印迹方法检测雌二醇 (17β E2 )对LRP16mRNA表达的时间及剂量依赖性调控作用 .构建LRP16基因启动子序列调控的萤光素酶报告子 (pS0 ) ,并与雌激素受体α和 β(ERα和ERβ)表达载体共转染COS 7和MCF 7细胞后测定萤光素酶活性 .将LRP16基因的表达载体转染MCF 7细胞 ,测定过表达LRP16对细胞的生长特性的影响 .17β E2 使MCF 7细胞中LRP16mRNA表达水平增加 ,增加幅度未显示出 17β E2 培养时间和剂量的依赖性 .pS0 与ERα表达载体共转染细胞的相对萤光素酶活性较非共转染组 (对照组 )及pS0 ERβ表载体共转染组升高 5～ 10倍 .LRP16基因过表达促进MCF 7细胞的增殖 .研究表明 ,雌激素可能通过ERα上调乳腺癌MCF 7细胞LRP16基因的表达并促进细胞增殖     

利用载体介导小干扰RNA诱导RSRC1基因沉默

目的：设计并构建人RSRC1基因小干扰RNA（siRNA）的真核表达载体,并观察其沉默效果。方法：以人RSRC1基因的cDNA序列为靶标,设计含有小发卡结构的2条寡核苷酸序列,并将其克隆到siRNA表达载体pSliencer2.1-U6neo上,转化大肠杆菌DH5α菌株,抽提质粒,测序正确后将重组质粒转染人胚肾293T细胞,通过Western blot和荧光分析检测其抑制效果。结果：重组体测序成功后,Western blot分析证明构建的siRNA能有效抑制外源性及内源性RSRC1表达;将siRNA重组质粒和带GFP标签的RSRC1共转染293T细胞,荧光显微镜下GFP的亮度明显减弱。结论：获得了2条人RSRC1siRNA真核表达载体,均能有效地抑制RSRC1基因表达。     

RNA干扰与基因敲除

RNAi是指通过双链RNA介导特异性降解靶mRNA,导致转录后水平基因沉默的现象。其作用途径有RdRP依赖的RNAi的途径与非RdRP依赖的RNAi途径2种。利用RNAi的基因敲除技术在dsRNA序列选择、质粒或病毒为载体的dsRNA体内合成、发夹样siRNA的转录、dsRNA的导入方法等方面取得了很大进展,在研究人类或其他生物基因组中未知基因及蛋白质的功能等领域具有诱人的应用前景。     

shRNA慢病毒载体稳定抑制LRP16 表达的HepG2 细胞的构建及鉴定

目的:构建LRP16基因抑制表达的Hep G2稳定细胞系,鉴定其LRP16基因抑制表达的效果。方法:构建LPP-HSH008357-LVRH1GP-200短发卡RNA(sh RNA)慢病毒表达载体,用该抑制表达慢病毒感染Hep G2细胞系,通过荧光筛选及药筛,获得LRP16基因稳定抑制表达细胞系;最终运用Q-PCR和Western blot鉴定该稳定细胞系中LRP16的表达。结果:构建了LRP16基因抑制表达及抑制表达对照的Hep G2稳定细胞系,并通过Q-PCR和Western blot进行了鉴定。Q-PCR结果显示相对于对照稳转株(LPP-CSHCTR001-LVRH1GP-100),抑制表达稳转株(LPP-HSH008357-7-LVRH1GP-200)LRP16基因的抑制效率是4组抑制表达细胞中效果最理想的一组,其抑制效率高达98%;Western blot结果也显示该抑制表达稳转株(LPP-HSH008357-7-LVRH1GP-200)的LRP16蛋白表达量明显低于野生型Hep G2细胞及对照稳转株(LPP-CSHCTR001-LVRH1GP-100),其结果与Q-PCR一致。结论:构建并鉴定了人LRP16基因抑制表达Hep G2稳定细胞系及其相应的对照稳转株。     

小干扰RNA对庚型肝炎病毒基因在人Huh-7细胞中表达的抑制作用

RNA干扰(RNAi)是由小干扰RNA(siRNA)引发的生物细胞内同源基因的转录后基因沉默现象, 是近年来兴起的一项研究生物基因调控与功能的崭新技术. 庚型肝炎病毒(HGV)是一单正链RNA病毒, 复制时不与宿主细胞基因组整合, 尤其适合用于RNAi的研究. 构建了含HGV完整结构基因并携带筛选标志潮霉素基因的真核表达载体pVAX.EH, 转染Huh-7细胞后, 筛选获得稳定表达HGV 结构蛋白的Huh-7细胞株(Huh-7-EH). RT-PCR和Western blot检测证实, HGV结构基因能在Huh-7-EH细胞中转录、表达, 并能进行剪切和翻译后修饰. 以体外转录法制备了2对靶向HGV E2基因的siRNA(1-E2 siRNA和2-E2 siRNA), 将其导入Huh-7-EH细胞中, 采用Western blot和克隆形成实验证实, HGV 1-E2 siRNA和2-E2 siRNA均能特异性抑制HGV结 构蛋白的表达, 抑制作用可维持1周以上. 其中2-E2 siRNA的抑制作用更强, 转染后对Huh-7-EH细胞潮霉素抗性克隆形成的抑制率达到了99%. Huh-7-EH细胞转染siRNA后对潮霉素敏感, 说 明HGV E2 siRNA不仅使HGV E2区的mRNA降解, 还可使融合在HGV E2区下游的潮霉素mRNA降解. 综上所述, 本实验建立的稳定表达HGV结构蛋白的Huh-7-EH细胞株, 能作为用于研究HGV复制和RNAi的细胞模型; HGV结构基因区的siRNA可同时抑制HGV结构蛋白及其下游的潮霉素基因的表达, 证明RNAi在真核细胞Huh-7-EH内可能存在放大作用.     

针对多效蛋白基因的小干扰RNA的设计及其稳定表达载体的构建

目的:设计多效蛋白基因特异性的小干扰RNA(siRNA),并构建一系列能在哺乳动物细胞内稳定表达这些siRNA的表达质粒,以便为在体外研究多效蛋白基因的功能打下基础。方法:设计并合成具有多效蛋白基因特异性的一组寡核苷酸片段,并克隆到pSilencer3.1-H1hygro载体;用脂质体LipofectAMINE2000转染和潮霉素筛选等方法建立能稳定表达相应siRNA的一组Pten-/-细胞克隆;利用Northern印迹检测这些细胞内多效蛋白基因的表达情况。结果:设计并构建了3个针对多效蛋白基因的siRNA表达质粒,并证明其中的1种质粒能在Pten-/-细胞内稳定表达相应的siRNA,并显著地抑制了该细胞多效蛋白基因的表达。结论:设计并构建出的针对多效蛋白基因的siRNA表达载体所表达的siRNA具有较强的RNA干涉功能,为多效蛋白基因的功能研究奠定了实验基础。     

小环载体介导的siRNA 稳定抑制乙肝病毒的复制和表达

【目的】尝试构建表达小干扰RNA(small interfering RNA,siRNA)的小环载体,并初步鉴定其对乙肝病毒(hepatitis B virus,HBV)复制及其基因表达的抑制作用。【方法】设计并合成靶向HBV S区的siRNA,将其克隆到小环载体pMC.BESPX-MCS2上,测序正确后将重组体pMC-H1-siHBS-U6转化入感受态E.coliZYCY10P3S2T,然后在培养基中加入L-阿拉伯糖,诱导其降解细菌骨架,获取只含有目的基因表达盒的小环RNA干扰载体pmc-H1-siHBS-U6。将小环RNA干扰载体与HBV真核表达质粒pHBV1.3共转染Huh-7细胞,分别在转染后1-7天,ELISA法检测Huh-7细胞上清中的HBsAg、HBeAg,并且通过Real-time RT-PCR法分析干扰RNA对HBV DNA及mRNA的抑制效果。【结果】成功构建了靶向HBV S基因的siRNA小环表达载体pmc-H1-siHBS-U6。该载体能显著抑制Huh-7细胞HBsAg和HBeAg分泌,并且其抑制效果能够维持2-3周时间。Real-time PCR证实HBV的DNA与mRNA水平分别降低了71%和80%,而对照siRNA及空载体则无此作用。【结论】成功构建了靶向HBV的小环RNA干扰载体,并且其能稳定、高效、特异地抑制HBV基因的表达与复制,该研究不仅对探索HBV的基因治疗提供了重要线索,而且为RNA干扰的应用提供了新的运载体系。     

Suppression of gene expression by RNA interference in cultured plant cells

Suppression by double-stranded RNA (dsRNA) of the expression of a target gene is known as RNA interference (RNAi). No quantitative analysis of the effects of RNAi on the expression of specific genes in cultured plant cells has been reported. However, as it is possible to produce populations of cultured plant cells that are uniform and divide synchronously for functional analysis of genes of interest, we performed a quantitative study of the effects of RNAi in such cells. We constructed dsRNA expression plasmids for a luciferase gene under the control of the cauliflower mosaic virus (CaMV) 35S promoter by simply connecting sense and antisense sequences in a head-to-head manner. An RNAi effect was observed 24 hours after the introduction of dsRNA expression plasmids into tobacco BY-2 cells by electroporation. The simple system for suppression of specific genes in plant cells should be useful in attempts to elucidate the roles of individual genes in plant cells.     

The roles of aerobic exercise training and suppression IL-6 gene expression by RNA interference in the development of insulin resistance

ObjectiveTo demonstrate the hypothesis that aerobic exercise training inhibits the development of insulin resistance through IL-6 and probe into the possible molecular mechanism about it.MethodsRats were raised with high-fat diets for 8 weeks to develop insulin resistance, and glucose infusion rates (GIRs) were determined by hyperinsulinemic–euglycemic clamping to confirm the development of insulin resistance. Aerobic exercise training (the speed and duration time in the first week were respectively 16 m/min and 50 min, and speed increased 1 m/min and duration time increased 5 min every week following it) and/or IL-6shRNA plasmid injection (rats received IL-6shRNA injection via the tail vein every two weeks) were adopted during the development of insulin resistance. The serum IL-6, leptin, adiponectin, fasting blood glucose, fasting serum insulin, GIR, IL-6 gene expression levels, p-p38 in various tissues and p-STAT3/t-STAT3 ratio in the liver were measured.ResultsRats fed with high-fat diets for 8 weeks were developed insulin resistance and the IL-6mRNA levels of IL-6shRNA injection groups in various tissues were significantly lower than those of control group (P < 0.05), respectively. The development of insulin resistance in exercise rats significantly decreased, however, compared with that, the GIR of exercise rats injected by IL-6shRNA was lower (P < 0.05). The IL-6mRNA levels were highest in the fat tissue and lowest in the skeletal muscles in all the rats. The serum adiponectin levels decreased (P < 0.05) following the development of insulin resistance, and it increased (P < 0.05) when the rats were intervened by aerobic exercise training for 8 weeks at the same time. However, there were not significant differences when serum leptin concentrations were compared (P > 0.05). The p-p38 significantly increased in the rats fed with high-fat diets, however, p-p38 of the exercise high-fat diets rats in the liver and fat tissues significantly decreased than that (P < 0.05). The changes of p-p38 in exercise rats injected by IL-6shRNA were irregular. The activation of STAT3 in the liver significantly increased (P < 0.05) following the development of insulin resistance, and it decreased (P < 0.05) when the rats were intervened by aerobic exercise training for 8 weeks at the same time, and the gene silencing of IL-6 did not have effects on the activation of STAT3 in the liver (P > 0.05).ConclusionsIn conclusion, aerobic exercise training prevented the development of insulin resistance through IL-6 to a certain degree. The gene expression and secretion of IL-6 could inhibit the development of insulin resistance. The mechanism of the effects were possibly related with elevating the levels of serum adiponectin, and/or inhibiting the activation of STAT3 in the liver and p38MAPK in the skeletal muscles, liver and fat tissues.     

Biochemical mechanisms of suppression of RNA interference by plant viruses

RNA interference (RNAi) plays an important biological role in regulation of gene expression of eukaryotes. In addition, RNAi was shown to be an adaptive protective molecular immune mechanism against viral diseases. Antiviral RNAi initiates from generation of short interfering RNAs used in the subsequent recognition and degradation of the viral RNA molecules. As a response to protective reaction of plants, most of the viruses encode specific proteins able to counteract RNAi. This process is known as RNAi suppression. Viral suppressors act on various stages of RNAi and have biochemical properties that enable viruses to effectively counteract the protective system of plants. Modern molecular and biochemical investigations of a number of viral suppressors have significantly expanded our understanding of the complexity of the nature of RNAi suppression as well as mechanisms of interaction between viruses and plants.