Construction of the pIRES2-ZsGreen1 eukaryotic expression vector of factor Ⅸ gene and expression in HEK-293 cells

Objective To construct p IRES2-ZsG reen1/FⅨexpression vector,using the pcDNA/FⅨplasmid containing FⅨcDNA as template,and expressing in HEK-293cells.Methods The total ORF of FⅨgene was amlified from pcDNA/FⅨplasmid,then the amplified fragment was clonded into the p IRES2-ZsG reen1 vector using

Mycoplasma contamination-mediated attenuation of plasmid DNA transfection efficiency is augmented via L-arginine deprivation in HEK-293 cells

目的:明确支原体污染对HEK-293细胞质粒DNA转染效率的影响,并从支原体对细胞精氨酸代谢的角度探究其机制。创新点:支原体是细胞培养中的常见污染源。HEK-293是目前常用的生产蛋白、包装病毒的常用细胞系。然而,目前支原体污染对于质粒DNA转染效率的影响未见报道。本研究首次报道支原体污染对HEK-293细胞质粒DNA转染效率的影响,并揭示其机理。方法:采用4’,6-二脒基-2-苯基吲哚(DAPI)和聚合酶链反应(PCR)方法鉴定HEK-293细胞中的支原体污染情况以及支原体抗生素Plasmocin对支原体污染的清除效果。通过聚乙烯亚胺(PEI)方法对支原体污染的HEK-293细胞及支原体清除后的HEK-293细胞转染质粒,比较转染效率差异。通过高效液相色谱法(HPLC)分析支原体污染的和支原体清除后的HEK-293细胞的细胞裂解产物和细胞上清中的L-精氨酸、瓜氨酸含量变化。在支原体污染的HEK-293细胞中补充L-精氨酸,观察质粒转染效率的改变情况。结论:支原体污染能大大降低HEK-293细胞中质粒DNA的转染效率,且其原因与支原体能耗竭细胞中的L-精氨酸有关。

Construction of an Expression Plasmid pEGFP-N1-boTLR2 for Full-length Bovine TLR2 and Its Expression in HEK293 Cells

[Objective] This study aimed to construct a full-length bovine TLR2 expression plasmid pEGFP-N1-boTLR2 and express it in HEK293 cells. [Method] A fulllength coding sequence of bovine TLR2 was cloned by RT-PCR, and ligated into the pMD18-T simple vector and then subcloned into the pEGFP-N1 vector. A recombinant eukaryotic expression plasmid containing the full-length CDS region of bovine TLR2 was constructed and transiently transfected into HEK293 cells. The transfection efficiency and the location of recombinant protein were examined by FCM and confocal microscopy. Then the bovine TLR2 mRNA expression in HEK293/boTLR2 was detected by qRT-PCR. Finally, we analyzed the biological activity through the response that lipoteichoic acid stimulates HEK293/boTLR2 cells. [Result] The full-length TLR2 gene was successfully cloned and ligated into eukaryotic expression vector. The recombinant expression vector expressed bovine TLR2 in HEK293 cells. HEK293/boTLR2 cells produced higher levels of IL-8 secretion than nontransfected HEK293 cells when stimulated with LTA from Staphylococcus aureus. [Conclusion] The established cell model can provide a fast, flexible and convenient means for screening TLR agonists and antagonists, and may also be useful for investigating the interaction between TLR agonists and TLRs.

Inhibitory Effects of Neferine on Na_v1.5 Channels Expressed in HEK293 Cells

Neferine, a bisbenzylisoquinoline alkaloid in Lotus Plumule, was proved to have a wide range of biological activities. In the present study, using whole-cell patch-clamp technique, we investigated the effects of neferine on Nav1.5 channels that are stably expressed in HEK 293 cells. We found that neferine potently and reversibly inhibited Nav1.5 currents in a concentration dependent manner with a half-maximal inhibition（IC50） being 26.15 μmol/L. The inhibitory effects of neferine on Nav1.5 currents were weaker than those of quinidine at the same concentration. The steady-state inactivation curve was significantly shifted towards hyperpolarizing direction in the presence of 30 μmol/L neferine, while the voltage-dependent activation was unaltered. Neferine prolonged the time to peak of activation, increased the inactivation time constants of Nav1.5 currents and markedly slowed the recovery from inactivation. The inhibitory effect of neferine could be potentiated in a frequency-dependent manner. These results suggested that neferine can block Nav1.5 channels under the open state and inactivating state and it is an open channel blocker of Nav1.5 channels.

Construction of recombinant plasmid pEGFP-C2-L539fs/47 and its expression in HEK293 cells

Objective:To reconstruct pEGFP-C2-L539fs/47,a HERG nonsense mutant in eukaryotic expression plasmid,and observe the fusion protein expressed in HEK293 cells(human embryo kidney cells).Methods:After double digestion of pcDNA3-L539fs/47 and pEGFP-C2-HERG with sbf I and Eco91 I,the small product fragment,from pcDNA3-L539fs/47,was subcloned into the big fragment of pEGFP-C2-HERG under T4 ligase.pEGFP-C2-L539fs/47 was identified by agarose gel electrophoresis and sequencing.pcDNA3-L539fs/47 and pEGFP-C2-L539fs/47 were transiently transfected into HEK293 cells by Lipofect,respectively.The expression of fusion protein in HEK293 cells was detected through immunofluorescence,laser confocal imaging scanning in vivo,Western blot and PCR.Results:Mutation region cDNA fragment(about 1 kb) and target vector fragment(about 7.2 kb) were ligated after purification and gel recovery.Agarose gel electrophoresis and sequencing successfully demonstrated eukaryotic expression plasmid pEGFP-C2-L539fs/47,constructed approximately 8.2 kb,sequencing consistent with template gene.The transfection efficiency of recombinant plasmid by fluorescence microscopy was more than60%.Western blot analysis detected pcDNA3-L539fs/47 expression of the protein size 60 KD,the expression of pEGFP-C2 fusion protein size of approximately 90 KD.The L539fs/47 gene expression in HEK293 cells was significant by PCR analysis.Confocal laser imaging showed that pEGFP-C2-L539fs/47 protein was successfully expressed in cytoplasm and cytomembrane of HEK293 cells.Conclusion:pEGFP-C2-L539fs/47 containing the HERG gene mutant was successfully constructed by double digestion method and expressed fusion protein in HEK293 cells,which laid a foundation for the further study on L539fs/47.

Cellular Oxidative Damage of HEK293T Cells Induced by Combination of CdCl_2 and Nano-TiO_2

This study investigated the conjoined cellular oxidative damage of human embryo kidney 293T（HEK293T） cells induced by cadmium chloride（CdCl2） and nanometer titanium dioxide（nano-TiO2）.RT-PCR technique was used to detect the expressions of Heme oxygenase-1（HO-1） and 8-oxoguanine DNA glycosylase（OGG1）.The activities of superoxide dismutase（SOD） and catalase enzyme（CAT） and concentrations of reactive oxygen species（ROS） and maldondialdehyde（MDA） were measured by different approaches.The results showed that CdCl2 and nano-TiO2 at a low concen-tration of 0.75 total toxic unit（TU） exerted an additive effects on HO-1 gene expression,CAT activities and MDA concentrations.When the total TU was increased to 1 or 1.25 TU,the interaction was syner-getic.Moreover,the mixture with high proportion of CdCl2 produced an additive effect on the OGG1 gene expression,and the interaction was changed to be synergetic when the concentration of CdCl2 was lower than or equal to that of nano-TiO2.Synergetic effects of CdCl2 and nano-TiO2 on cellular oxida-tive damage of HEK293T cells were found as indicated by the changes in the SOD activities and ROS concentrations.It was concluded that CdCl2 and nano-TiO2 exerts synergistic effects on the cellular oxidative damage of HEK293T cells,and the sensitivity of these indicators of oxidative damage varies with the proportion of CdCl2 and nano-TiO2 in the mixture.

手动膜片钳检测盐酸罗哌卡因及其右旋异构体对HEK293细胞hERG电流的影响

目的研究比较盐酸罗哌卡因和盐酸罗哌卡因右旋异构体对高表达hERG钾通道的HEK293细胞hERG电流的影响。方法用手动膜片钳检测转染后hERG钾通道稳定表达的HEK293细胞电流,多菲莱德做阳性药,将盐酸罗哌卡因和盐酸罗哌卡因右旋异构体依次稀释成30.00、10.00、3.33、1.11、0.37μmol·L^(-1),依次作用于细胞,记录电流变化,计算抑制率。结果盐酸罗哌卡因0.37、1.11、3.33、10、30μmol·L^(-1)对电流Iherg-tail的抑制率分别为(6.12±0.30)%、(13.04±1.20)%、(19.21±0.33)%、(35.56±0.66)%、(65.37±4.17)%,IC_(50)为19.482μmol·L^(-1)(n=15)。盐酸罗哌卡因右旋异构体0.37、1.11、3.33、10.00、30.00μmol·L^(-1)对电流Iherg-tail的抑制率分别为(4.13±3.43)%、(7.34±5.60)%、(9.49±2.75)%、(16.60±0.87)%、(31.36±1.45)%,IC_(50)>30μmol·L^(-1)(n=15)。阳性对照药品多菲莱德0.00185、0.00556、0.01667、0.05000、0.15000μmol·L^(-1)对电流Iherg-tail的抑制率分别为(7.81±2.77)%、(19.67±1.88)%、(57.16±4.39)%、(89.71±3.55)%、(99.66±0.89)%、IC_(50)为0.015μmol·L^(-1)(n=15)。结论和阳性对照药品多菲莱德比较,盐酸罗哌卡因对hERG通道为弱抑制作用,盐酸罗哌卡因右旋异构体对hERG通道为无明显抑制作用。

Protective Effect of Reduced Glutathione C_(60) Derivative against Hydrogen Peroxide-induced Apoptosis in HEK 293T Cells

Hydrogen peroxide（H_2O_2） and free radicals cause oxidative stress, which induces cellular injuries, metabolic dysfunction, and even cell death in various clinical abnormalities. Fullerene（C_（60）） is critical for scavenging oxygen free radicals originated from cell metabolism, and reduced glutathione（GSH） is another important endogenous antioxidant. In this study, a novel water-soluble reduced glutathione fullerene derivative（C_（60）-GSH） was successfully synthesized, and its beneficial roles in protecting against H_2O_2-induced oxidative stress and apoptosis in cultured HEK 293 T cells were investigated. Fourier Transform infrared spectroscopy and 1H nuclear magnetic resonance were used to confirm the chemical structure of C_（60）-GSH. Our results demonstrated that C_（60）-GSH prevented the reactive oxygen species（ROS）-mediated cell damage. Additionally, C_（60）-GSH pretreatment significantly attenuated H_2O_2-induced superoxide dismutase（SOD） consumption and malondialdehyde（MDA） elevation. Furthermore, C_（60）-GSH inhibited intracellular calcium mobilization, and subsequent cell apoptosis via bcl-2/bax-caspase-3 signaling pathway induced by H_2O_2 stimulation in HEK 293 T cells. Importantly, these protective effects of C_（60）-GSH were superior to those of GSH. In conclusion, these results suggested that C_（60）-GSH has potential to protect against H_2O_2-induced cell apoptosis by scavenging free radicals and maintaining intracellular calcium homeostasis without evident toxicity.

Salvia fruticosa reduces intrinsic cellular and H_2O_2-induced DNA oxidation in HEK 293 cells;assessment using flow cytometry

Objective:To investigate the role of water-soluble extract of Salvia fruticosa(Creek sage)(S.fruticosa) leaves in reducing both intrinsic cellular and H_2O_2-induced DNA oxidation in cultured human embryonic kidney 293 cells.S.fruiicosa.native to the Eastern-Mediterranean basin,is widely used as a medicinal herb for treatment of various diseases.Methods:Dried leaves of 5.fruticosa were extracted in phosphate buffer saline and purified using both vacuum and high pressure filtrations.Each mL of the preparation contained(7.1±1.0)mg of extract.HEK-293 cells were incubated in one set with S.fruticosa extract in the presence of 0.1 mmol/L H_2O_2,and in the other set with the addition of the extract alone.The DNA oxidation was measured using fluorescence upon fluorescein isothiocyanate derivarization of 8-oxoguanine moieties.The fluorescence was measured using flow cytometry technique.Results:Cells incubated 3 h with 150μL extract and exposed to 0.1 mmol/L H_2O_2 showed lower intensity of fluorescence,and thus lower DNA oxidation.Moreover,cells incubated 3 h with 100μl.of the extract showed lower intensity of fluorescence,and thus lower intrinsic cellular DNA oxidation compared to control(without S.fruticosa).Conchisions:The results from this study suggest that the water-soluble extract of S.fruticosa leaves protects against both H_2O_2-induced and intrinsic cellular DNA oxidation in human embryonic kidney 293 cells.

氟康唑对豚鼠心室肌细胞I_K和在HEK-293细胞中表达的HERG钾通道的抑制作用

目的研究氟康唑对豚鼠心室肌细胞延迟整流钾电流(IK)和在HEK-293细胞中表达的HERG钾通道的抑制作用。方法应用酶解法消化豚鼠单个心室肌细胞,观察氟康唑对IK的影响;采用磷酸钙沉淀瞬时转染的方法将HERG基因表达于HEK-293细胞上,观察氟康唑对野生型HERG钾通道电流、激活和失活曲线的影响,以及氟康唑对Y652A和F656C突变型HERG钾通道的作用;IK和HERG电流的记录均采用全细胞膜片钳技术。结果氟康唑(0.01、0.1、1、3、10、30、100、300和1 000μmol.L-1)浓度依赖性地抑制IK和HERG钾电流,其IC50值分别为(68.1±21.6)μmol.L-1和(48.2±9.4)μmol.L-1,对HERG钾通道的电压依赖性激活和失活曲线无影响;与野生型(WT)比较,Y652A和F656C突变型可减弱氟康唑对HERG通道的阻断作用。结论氟康唑能阻断IK和HERG通道,Y652和F656是氟康唑与HERG通道结合的关键位点。

凋亡相关蛋白在汉坦病毒诱导HEK-293细胞凋亡过程中的表达及意义

目的探讨Bcl-2、Bax及Caspase-3在汉坦病毒诱导人胚肾细胞(HEK-293)凋亡过程中的变化,为研究汉坦病毒诱导人胚肾细胞损伤的机制提供参考。方法体外培养HEK-293细胞,分为正常对照组和汉坦病毒处理的感染组,采用间接免疫荧光法检测HEK-293内汉坦病毒抗原;用Westen blot方法检测Bcl-2、Bax及Caspase-3蛋白表达水平。结果汉坦病毒感染HEK-293细胞1 d后即开始出现荧光阳性细胞,随着时间延长,荧光强度逐渐增强,细胞胞浆内出现大量片状或颗粒性的黄绿色荧光;Western blot结果显示,与对照组比较,汉坦病毒感染1 d后Bcl-2、Bax蛋白及Caspase-3酶原活化片段表达量未见明显变化(P>0.05),感染3 d和5 d后Bcl-2蛋白表达降低,Bax蛋白表达上调,Caspase-3酶原活化片段表达升高(P<0.05)。结论汉坦病毒可感染HEK-293细胞并在其体内增殖,其损伤机制可能与Bcl-2表达减少和Bax蛋白表达上调,通过线粒体途径诱导HEK-293细胞发生凋亡有关。

优化阳离子脂质体介导的组织因子小干扰RNA转染HEK-293的转染条件

目的:优化lipofectamine^(TM)2000介导的组织因子(TF)小干扰RNA(siRNA)的转染条件。方法:化学合成法合成特异的TFsiRNA,利用绿色荧光蛋白(GFP)进行标记,分别将1.0μL和1.5μL的lipofectamineTM2000与含有20、30、40、50、60pmol的TFsiRNA混合液制备成相应的转染混合物,转染人胚胎肾细胞株(HKE-293)24h后,在荧光显微镜下计数阳性细胞率。同时,四甲基偶氮唑盐(MTT)法检测每组细胞活性。结果:转染效率和细胞活性与lipofectamineTM2000以及siRNA有明显的交互作用,在1.0μL的lipofectamineTM2000和50pmolsiRNA转染HEK-293细胞时,细胞转染效率最高,转染效率达(86.5±2.4)%,在1.5μL的lipofectamineTM2000转染40pmolsiRNA时,细胞活性为(86.0±7.8)%。结论:经优化转染条件后的li-pofectamineTM2000可高效的将化学合成的siRNA转染入HKE-293细胞株,且细胞活性达85%以上,为建立稳定的沉默转染体系提供实验基础。

HEK-293细胞α_(1B)-肾上腺素受体引起的Ca^(2+)依赖性K^+电流和Ca^(2+)内流(英文)

目的:研究HEK293细胞上α1B肾上腺素受体亚型引起向外K+电流和Ca2+内流的特性。方法:细胞贴附式单通道记录K+通道和Fura2荧光测定胞浆游离Ca2+浓度。结果:肾上腺素或苯肾上腺素可引发一电导为160pS的外向K+电流。该电流可被50μmol·L-1氯乙醛可乐定(CEC),5mmol·L-1依他酸(EGTA)或2mmol·L-1四乙铵(TEA)抑制。硝苯吡啶(nifedipine)不改变该电流及α1B亚型引起的Ca2+内流;后者可被1mmol·L-1LaCl3抑制。结论:激活转染在HEK293细胞上的α1B受体亚型可引起通过硝苯吡啶不敏感Ca2+通道的Ca2+内流。

HEK-293细胞复苏培养及冻存

目的通过对人胚肾293细胞的复苏培养及其冻存的研究,为进一步行干细胞标记实验奠定基础。方法复苏培养人胚肾293细胞,倒置显微镜观察人胚肾293细胞的生长状况,计算细胞贴壁率,绘制细胞生长曲线,冻存保留细胞。结果人胚肾293细胞在普通培养条件下生长良好,6h后大部分细胞已经贴壁,8h细胞已完全贴壁。结论人胚肾293细胞采用改进方法复苏培养及冻存是简便可行的,为进一步行干细胞标记实验奠定了坚实的前期基础。

DNA聚合酶iota在HEK-293细胞中高表达体系的建立

目的:将带有DNA聚合酶iota(DNA Polymerase iota,Polt)目的基因的真核表达质粒PCDNA3.1转入HEK-293细胞,建立DNA聚合酶iota在HEK-293细胞中的高表达体系,为进一步研究DNA聚合酶在DNA损伤修复中的生物学功能奠定了基础。方法:用脂质体2000(Lipofectamine2000)将带有目的基因的真核表达质粒PCDNA3.1转入HEK-293细胞,通过G418筛选抗性克隆,用一步法提取细胞总RNA,采用逆转录聚合酶链式反应(RT-PCR)技术检测出高表达克隆。结果:通过G418筛选筛选出了具有G418抗性的克隆,通过RT-PCR技术检测出高表达DNA聚合酶iota的HEK-293细胞系。结论:建立了高表达DNA聚合酶iota的HEK-293细胞系,为进一步研究DNA聚合酶在DNA损伤修复中的生物学功能奠定了基础。

依托咪酯对HEK-293细胞中异源表达的hERG钾通道电流的抑制作用

目的:观察依托咪酯对HEK-293细胞中异源表达的hERG钾通道电流的抑制作用及其机制。方法:采用脂质体瞬时转染的方法将野生型hERG(WT-hERG)、突变型Y652A-hERG和F656C-hERG分别转染人胚胎肾细胞HEK-293,应用全细胞膜片钳技术记录依托咪酯对转染后HEK-293细胞表达的hERG钾通道电流的抑制作用以及对激活曲线和失活曲线的影响。结果:依托咪酯可浓度依赖性地抑制WT-hERG转染的HEK-293细胞钾通道电流,其半数最大抑制浓度为(6.41±2.43)μmol/L,对激活曲线和失活曲线无明显影响。与WT-hERG转染的HEK-293细胞相比,依托咪酯对突变体Y652A-hERG及F656C-hERG转染的HEK-293细胞内钾通道电流的抑制作用减弱。结论:F656C可能是依托咪酯抑制hERG钾通道的重要靶点。

人TRBP基因在HEK-293细胞中的表达

目的:构建携带人TRBP(TAR RNA结合蛋白)基因的真核表达载体,并将其在HEK-293细胞中表达.方法:用RT-PCR的方法扩增获得TRBP全长cDNA,然后克隆入pFLAG-CMV4真核表达载体.脂质体法瞬时转染HEK-293细胞,间接免疫荧光和Western Blot检测目的蛋白表达.结果:成功获得了全长的TRBP cDNA,构建了含人的TRBP cDNA的真核表达载体.转染HEK-293细胞后提取蛋白,经电泳观察到在Mr46000存在与目的蛋白分子质量相符的条带,该条带可被抗TRBP多克隆抗体及抗FLAGmAb特异性识别.结论:TRBP哺乳动物表达系统的建立,为进一步研究TRBP的生物学效应奠定了基础.

菌多糖对Balb/c 3T_3、Hela、HEK-293细胞增殖的影响

用苯酚法提取JM109大肠杆菌、O157大肠杆菌、霍乱弧菌、伤寒杆菌及多头绒泡菌的菌多糖,用MTT法检测菌多糖在体外对Balb/c 3T_3(鼠成纤维细胞)、Hela(人上皮细胞)和HEK-293(人胚肾细胞)增殖的影响.结果表明,菌多糖在低质量浓度(低于40mg/L)时抑制Hela细胞和HEK-293细胞的增殖,但促进Balb/c 3T_3细胞的增殖;菌多糖超过一定质量浓度(80mg/L)时,对Balb/c 3T_3细胞的增殖作用和对Hela、HEK-293细胞增殖的抑制作用趋于饱和.

人HNA-3a基因的克隆及其在HEK-293细胞的表达

目的:构建人HNA-3a基因全长的真核表达载体,探索一种检测抗人HNA-3a抗体的实验方法,观察HNA-3a蛋白表达情况。方法:参照GeneBank中人HNA-3a基因序列,设计并合成引物,采用RT-PCR方法反转录HNA-3a基因外显子片段全长,定向克隆到pEGFP-N3载体中,然后采用Lipofectamine^(TM) 2000试剂将含目的基因的pEGFP-N3表达载体转染至HEK-293细胞中进行稳定表达,并以免疫荧光和蛋白质免疫印迹法(WB)鉴定目的基因的表达情况。结果:免疫荧光和免疫印迹结果显示,目的基因在HEK-293细胞中获高效表达。结论:成功构建了高效表达HNA-3a蛋白的真核表达载体,为检测人血浆中抗HNA-3a抗体奠定了基础。

GATA5抑制EpCAM表达对肾癌HEK-293细胞系的影响

目的研究GATA5对肾癌HEK-293细胞系增殖调控及对细胞重编程因子EpCAM表达的影响。方法构建pTT5-GATA5表达载体并进行基因序列测序验证;四甲基偶氮唑盐(MTT)法检测细胞增殖率;细胞划痕实验检测细胞划痕修复情况;实时定量反转录-聚合酶链反应(RT-PCR)检测基因mRNA表达;蛋白免疫印迹(Western Blot)检测蛋白表达。结果GATA5抑制HEK-293细胞增殖;GATA5抑制HEK-293细胞划痕修复;GATA5抑制EpCAM的mRNA和蛋白表达。结论GATA5可以抑制肾癌细胞HEK-293细胞的增殖率并抑制EpCAM表达。