EB病毒潜伏膜蛋白LMP1编码基因沉默对NF—kB表达的影响

目的：探讨EBV阳性胃上皮细胞中潜伏膜蛋白1（latentmembraneprotein-1,LMP1）基因沉默对NF-kB转录表达的影响。方法：以稳定表达LMP1的EBV阳性胃上皮细胞系作为靶细胞,采用化学合成的siRNA特异性沉默LMP1,用RT-PCR和Westem-blotting分别检测其在不同时间段mRNA和蛋白水平特异性沉默效果;Westernblotting及免疫酶染色法检测LMP1基因沉默对NF—kB转录表达及核转移的影响。结果：siRNA在mRNA和蛋白水平可特异性沉默LMP1的表达,且有时间效应关系;Westem blotting及免疫酶染色法检测结果显示LMP1沉默可干扰NF—KB表达,导致靶细胞核内NF-kB水平下降,细胞浆内水平升高,而NF—kB总蛋白有下降趋势。结论：LMP1基因特异性沉默能够影响NF-kB表达,抑制其核转移。     

针对核因子-kB P65基因的短发夹干扰RNA逆转录病毒载体构建与鉴定

目的:构建针对人核因子kB亚基P65基因mRNA的短发夹干扰RNA(shRNA)逆转录病毒表达载体,并探讨小干扰RNA(siRNA)靶向抑制NF-kB P65基因表达的作用.方法:根据shRNA设计原则,在人NF-kB P65全长序列中选取合19个核苷酸靶序列,设计形成siRNA的DNA模板并克隆到shRNA表达载体pSUPER.retro.neo中,构建针对NF-kB P65基因的shRNA表达载体.经293A细胞包装,并感染NIH3T3细胞进行病毒滴度测定后,感染THP-1细胞.分别采用RT-PCR和Western blot从mRNA和蛋白水平检测干扰效果.结果:限制性酶切和基因测序证实针对人NF-kB P65亚基的shRNA表达逆转录病毒载体成功构建;其感染THP-1细胞后,NF-kB P65的mRNA和蛋白表达明显抑制.结论:成功构建了NF-kB P65 shRNA逆转录病毒表达载体,该载体能高效感染THP-1并明显抑制NF-kB P65的表达.     

利用RNA干扰抑制人肝癌细胞中核因子-kB p65基因的表达

目的:用小干扰RNA(siRNA)抑制核因子-KB(NF-kB)p65基因在人肝细胞癌细胞中的表达.方法:从p65的cDNA序列中挑选3个RNA干扰靶位点,用体外转录法制备siRNA,以萤光素酶基因的siRNA为对照,分别转染Hep3B和SMMC-7721细胞,用逆转录半定量PCR和免疫印迹检测siRNA对p65基因表达的抑制效率.结果:3条siRNA对p65基因的表达都有抑制作用,其中2条siRNA的抑制作用更为显著,最高抑制效率约为70%.结论:制备的p65-siRNA可用于研究NF-KB在肝细胞癌发生发展中的作用.     

Spl基因RNA干扰载体的构建及鉴定

目的:构建干扰载体pSilencer 3.1-spl,并初步研究其对Spl基因的干扰作用.方法:根据Spl cDNA编码序列,设计并合成针对Spl基因的特异性RNA干扰片段,并将其克隆入pSilencer 3.1-Hl neo干扰载体中,构建Spl基因小干扰RNA(siRNA)真核表达载体pSilencer 3.1-Spl;分别将阴性对照载体pSilencer 3.1与重组载体pSilencer 3.1-Spl经脂质体LipofectAMINE2000介导转染HeLa细胞,采用RT-PCR、Western blot方法分别检测Spl基因的转录与表达水平.结果:构建了Spl基因siRNA真核表达载体pSilencer 3.1-Spl,经酶切、测序鉴定证实克隆正确,并在mRNA水平和蛋白水平证实了载体的干扰效果.结论:特异性siRNA能明显抑制Spl基因在HeLa细胞中的表达,为进一步研究Spl的生物学功能和作用机制奠定了实验基础.     

siRNA靶向沉默p22phox表达对内皮细胞衰老抑制作用的研究

设计特异性siRNA(Short interference RNA)诱导人脐静脉内皮细胞株ECV-304细胞NAD(P)H氧化酶活性亚单位p22phox基因沉默, 探讨p22phox基因沉默在血管紧张素Ⅱ(AngⅡ)诱导的ECV-304衰老中的作用及机理。应用体外转录合成3种siRNA转染体外培养的ECV-304, RT-PCR鉴定对p22phox基因沉默的效率和特异性, 确立适宜的转染浓度和基因沉默的持续时间; ECV-304分为空白对照组、AngⅡ组、siRNA转染组、AngⅡ+siRNA转染组, 观察细胞衰老改变及活性氧水平, 分析各组细胞p22phox的mRNA及蛋白表达。结果表明: 3种siRNA中, 一种对p22phox mRNA表达抑制率达到83％, 在一定转染浓度范围内, siRNA诱导的基因沉默效率呈剂量依赖性, 抑制效率高峰期在24~36 h; 给予AngⅡ后, b-gal染色阳性细胞数显著增加, 出现衰老的特征性改变, 衰老细胞p22phox的 mRNA及蛋白表达增加, 伴有一氧化氮(NO)生成减少, 活性氧生成增加, siRNA诱导p22phox基因沉默后降低了活性氧水平, 增加NO生成, 改善了AngⅡ诱导的ECV-304细胞的衰老改变。siRNA干扰技术可成功诱导NAD(P)H氧化酶p22phox基因沉默, 从而减缓AngⅡ诱导体外培养的ECV-304衰老进程, p22phox是防治衰老有希望的分子靶点。     

用鼻咽相对特异性调控区建立N-LMP1转基因小鼠

为了研究EBV LMP1在鼻咽癌发生发展中的作用 ,构建了EDL 2、PLUNC p双启动子调控鼻咽癌来源的LMP1(latentmembraneprotein 1,潜伏膜蛋白 1)的表达载体 ,采用受精卵前核显微注射法构建转基因小鼠。结果表明 ,在所获得的 5 8只转基因首建鼠中 ,4只整合阳性 ,其中的一只转基因小鼠在鼻咽、前胃、舌根等部位检测到了外源基因的表达。     

转录因子Sp1上调前列腺癌细胞中CD59的表达

目的:构建针对Sp1基因siRNA真核表达载体,转染前列腺癌细胞PC-3,研究反式作用因子Sp1时CD59表达的影响.方法:应用siRNA表达载体介导的RNAi技术,构建含特异性sp1基因的重组载体pSUPER-siSp1,脂质体法转染前列腺癌细胞,G418筛选建立稳定表达转染基因的细胞株,Western blotting检测转染细胞中sp1和CD59基因的表达,MTT和染料释放试验判断CD59基因抑制后对补体溶破的抵抗作用.结果:成功构建了Sp1基因siRNA真核表达载体,转染PC-3细胞可表达荧光蛋白,稳定转染的Pc-3细胞Sp1及CD59基因蛋白水平降低,MTT和染料释放实验表明CD59基因受抑制后对补体溶破的抵抗作用降低.结论:siRNA-Sp1重组载体有效地抑制了CD59的表达,降低CD59的抗补体活性,结果证明反式作用因子Sp1是CD59表达调控中重要的转录因子,为探讨CD59在肿瘤细胞中高表达的研究奠定了基础.     

RNA干扰沉默低氧诱导因子-1α对低氧下大鼠肺动脉平滑肌细胞增殖的影响

本研究应用基因克隆技术,将合成的发卡样特异性低氧诱导因子-1α（hypoxia inducible factor-1alpha,HIF-1α）干扰寡核苷酸（siRNA）序列插入真核表达载体中,构建出特异性HIF-1α基因RNA干扰（RNAi）真核表达载体。采用组织块种植法,原代培养大鼠肺动脉平滑肌细胞（pulmonary artery smooth muscle cells,PASMCs）,将构建出的特异性HIF-1αRNAi真核表达载体转染到PASMCs;分别在常氧和低氧下进行细胞培养,采用RT-PCR检测PASMCsHIF-1αmRNA表达水平,用MTT和流式细胞仪检测细胞增殖水平,探讨低氧条件下HIF-1αRNAi真核表达载体对PASMCs增殖的影响。结果表明,低氧培养48h后,正常PASMCs和转染了HIF-1αsiRNA阴性表达载体的细胞增殖显著,HIF-1αmRNA表达水平也显著升高;而转染了HIF-1αsiRNA阳性表达质粒的细胞增殖不显著,HIF-1αmRNA表达水平较低。结果提示：HIF-1αRNAi真核表达载体能显著干扰培养的PASMCsHIF-1αmRNA表达,同时抑制低氧环境下PASMCs的增殖。     

Sp1基因RNA干扰载体的构建及鉴定

目的：构建干扰载体pSilencer3.1-Sp1,并初步研究其对Sp1基因的干扰作用。方法：根据Sp1cDNA编码序列,设计并合成针对Sp1基因的特异性RNA干扰片段,并将其克隆入pSilencer3.1-H1neo干扰载体中,构建Sp1基因小干扰RNA（siRNA）真核表达载体pSilencer3.1-Sp1;分别将阴性对照载体pSilencer3.1与重组载体pSilencer3.1-Sp1经脂质体LipofectAMINE2000介导转染HeLa细胞,采用RT-PCR、Western blot方法分别检测Sp1基因的转录与表达水平。结果：构建了Sp1基因siRNA真核表达载体pSilencer3.1-Sp1,经酶切、测序鉴定证实克隆正确,并在mRNA水平和蛋白水平证实了载体的干扰效果。结论：特异性siRNA能明显抑制Sp1基因在HeLa细胞中的表达,为进一步研究Sp1的生物学功能和作用机制奠定了实验基础。     

Investigation of the mechanism of temperature sensitivity of the electroreceptors of ampullae of lorenzini

In experiments on Black Sea skates (Raja clavata), the potential of the receptor epithelium of the ampullae of Lorenzini and spike activity of single nerve fibers connected to them were investigated during electrical and temperature stimulation. Usually the potential within the canal was between 0 and –2 mV, and the input resistance of the ampulla 250–400 k. Heating of the region of the receptor epithelium was accompanied by a negative wave of potential, an increase in input resistance, and inhibition of spike activity. With worsening of the animal's condition the transepithelial potential became positive (up to +10 mV) but the input resistance of the ampulla during stimulation with a positive current was nonlinear in some cases: a regenerative spike of positive polarity appeared in the channel. During heating, the spike response was sometimes reversed in sign. It is suggested that fluctuations of the transepithelial potential and spike responses to temperature stimulation reflect changes in the potential difference on the basal membrane of the receptor cells, which is described by a relationship of the Nernst's or Goldman's equation type.I. P. Pavlov Institute of Physiology, Academy of Sciences of the USSR, Leningrad. I. M. Sechenov, Institute of Evolutionary Physiology and Biochemistry, Academy of Sciences of the USSR, Leningrad. Pacific Institute of Oceanology, Far Eastern Scientific Center, Academy of Sciences of the USSR, Vladivostok. Translated from Neirofiziologiya, Vol. 12, No. 1, pp. 67–74, January–February, 1980.     

Principles of organization and evolution of systems of regulation of functions

Evolution of living organisms is closely connected with evolution of structure of the system of regulations and its mechanisms. The functional ground of regulations is chemical signalization. As early as in unicellular organisms there is a set of signal mechanisms providing their life activity and orientation in space and time. Subsequent evolution of ways of chemical signalization followed the way of development of delivery pathways of chemical signal and development of mechanisms of its regulation. The mechanism of chemical regulation of the signal interaction is discussed by the example of the specialized system of transduction of signal from neuron to neuron, of effect of hormone on the epithelial cell and modulation of this effect. These mechanisms are considered as the most important ways of the fine and precise adaptation of chemical signalization underlying functioning of physiological systems and organs of the living organism