逆转录病毒介导的小干扰RNA稳定抑制子LRP16基因表达

RNA干涉是近年被广泛关注的一项技术,通过19～21 nt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+374 nt和+668 nt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pL668 2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.     

LRP16短发夹RNA慢病毒载体的构建及LRP16稳定抑制细胞的建立

目的:构建靶向LRP16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-LRP16shRNA-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。     

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     

cmv-3′LTR嵌合启动子对逆转录病毒载体MFG滴度及外源基因表达的影响

为减轻逆转录病毒载体介导的外源基因的沉默,进一步提高逆转录病毒载体MFG介导的外源基因的表达水平,同时探讨逆转录病毒3′端长末端重复序列(long terminalrepeat,LTR)内U3区对病毒基因表达的影响,将逆转录病毒载体3′端LTR内的U3区用cmv核心增强子、启动子序列替代,同时去除了3个与逆转录病毒载体启动子甲基化有关的序列NCR、DR,并以egfp为报告基因,构建了MFG egfp和MFG egfp cmv表达载体。结果显示:利用cmv启动子替代MFG载体3′端LTR的U3启动子序列,会显著降低MFG载体的病毒滴度及其介导的外源报告基因的表达。提示利用cmv启动子替代病毒载体的3′端LTR内的U3区,并不是提高MoMLV(moloneymurineleukemivirus)逆转录病毒载体介导外源基因的表达及其病毒滴度的理想策略。结果也同时提示:在MoMLV逆转录病毒3′端LTR的U3区,可能存在与病毒RNA加工、成熟及稳定性有关的信号序列。     

cmv-3’LTR嵌合启动子对逆转录病毒载体MFG滴度及外源基因表达的影响

为减轻逆转录病毒载体介导的外源基因的沉默,进一步提高逆转录病毒载体MFG介导的外源基因的表达水平,同时探讨逆转录病毒3’端长末端重复序列(long-terminal repeat,LTR)内U3区对病毒基因表达的影响,将逆转录病毒载体3’端LTR内的U3区用cmv核心增强子、启动子序列替代,同时去除了3个与逆转录病毒载体启动子甲基化有关的序列NCR、DR,并以egfp为报告基因,构建了MFG-egfp和MFG-egfp-cmv表达载体。结果显示：利用cmv启动子替代MFG载体3’端LTR的U3启动子序列,会显著降低MFG载体的病毒滴度及其介导的外源报告基因的表达。提示利用cmv启动子替代病毒载体的3’端LTR内的U3区,并不是提高MoMLV(moloney murineleukemi virus)逆转录病毒载体介导外源基因的表达及其病毒滴度的理想策略。结果也同时提示：在MoMLV逆转录病毒3’端LTR限的U3区,可能存在与病毒RNA加工、成熟及稳定性有关的信号序列。     

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.     

携带人NFBD1基因shRNA重组逆转录病毒载体的构建及鉴定

建立逆转录病毒介导的NFBD1基因RNA干扰表达体系,并观察其在宫颈癌SiHa细胞中对NFBD1表达的影响.将人NFBD1基因RNA干扰双链DNA片段重组到pSUPER Retro质粒中,构建携带人NFBD1基因RNA干扰的逆转录病毒载体pSUPER-shRNA-NFBD1,经PT67细胞包装后,产生的重组逆转录病毒感染宫颈癌细胞株SiHa细胞,并用嘌呤霉素筛选产生稳定的细胞克隆,用实时荧光定量PCR和Westernblotting检测细胞中NFBD1 mRNA和蛋白表达的变化.重组逆转录病毒质粒经测序鉴定正确;逆转录病毒感染SiHa细胞后用嘌呤霉素筛选出稳定的细胞克隆;实时荧光定量PCR和Westernblotting检测人NFBD1 mRNA和蛋白表达水平明显低于阴性对照组和未干扰组.携带人NFBD1基因RNA干扰双链DNA片段的逆转录病毒感染SiHa细胞后能明显抑制NFBD1 mRNA和蛋白表达,为进一步研究NFBD1在宫颈癌中的作用奠定了基础.     

用pLNCX2携带人MCPH1基因shRNA重组逆转录病毒载体的构建及鉴定

目的建立逆转录病毒介导的MCPH1基因RNA干扰表达体系并观察其在宫颈癌Caski细胞中对MCPH1表达的影响。方法将人MCPH1基因RNA干扰双链DNA片段重组到逆转录病毒质粒pLNCX2中,构建携带人MCPHI基因RNA干扰的逆转录病毒载体pLNCX2-shRNA—MCPH1,经PT67细胞包装后,产生的重组逆转录病毒感染宫颈癌细胞株Caski细胞,并用G418筛选产生稳定的细胞克隆,用RT—PCR和Western印迹检测细胞中MCPH1mRNA和蛋白表达的变化。结果重组逆转录病毒质粒经测序鉴定正确,逆转录病毒感染Caski细胞后用G418筛选出稳定的细胞克隆,RT—PCR和Western印迹检测人MCPH1mRNA和蛋白表达水平明显低于阴性对照组和未干扰组。结论携带人MCPHI基因RNA干扰双链DNA片段的逆转录病毒感染Caski细胞后能明显抑制MCPHImRNA和蛋白表达,为进一步研究MCPH1在宫颈癌中的作用奠定了基础。     

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     

A Unique Protease Cleavage Site Predicted in the Spike Protein of the Novel Pneumonia Coronavirus (2019-nCoV) Potentially Related to Viral Transmissibility

正Dear Editor,In December 2019, a novel human coronavirus caused an epidemic of severe pneumonia(Coronavirus Disease 2019,COVID-19) in Wuhan, Hubei, China(Wu et al. 2020; Zhu et al. 2020). So far, this virus has spread to all areas of China and even to other countries. The epidemic has caused 67,102 confirmed infections with 1526 fatal cases     

Curcuminoids as inhibitors of thioredoxin reductase: A receptor based pharmacophore study with distance mapping of the active site

Curcumin is the yellow pigment of turmeric that interacts irreversibly forming an adduct with thioredoxin reductase (TrxR), an enzyme responsible for redox control of cell and defence against oxidative stress. Docking at both the active sites of TrxR was performed to compare the potency of three naturally occurring curcuminoids, namely curcumin, demethoxy curcumin and bis-demethoxy curcumin. Results show that active sites of TrxR occur at the junction of E and F chains. Volume and area of both cavities is predicted. It has been concluded by distance mapping of the most active conformations that Se atom of catalytic residue SeCYS498, is at a distance of 3.56 from C13 of demethoxy curcumin at the E chain active site, whereas C13 carbon atom forms adduct with Se atom of SeCys 498. We report that at least one methoxy group in curcuminoids is necessary for interation with catalytic residues of thioredoxin. Pharmacophore of both active sites of the TrxR receptor for curcumin and demethoxy curcumin molecules has been drawn and proposed for design and synthesis of most probable potent antiproliferative synthetic drugs.     

Comparative morphology of the carpel in the Liliaceae: Hewardieae, Petrosavieae, and Tricyrteae

The young pistils in the melanthioid tribes, Hewardieae, Petrosavieae and Tricyrteae, are uniformly tricarpellate and syncarpous. They lack raphide idioblasts. All are multiovulate, with bitegmic ovules. The Petrosavieae are marked by the presence of septal glands and incomplete syncarpy. Tepals and stamens adhere to the ovary in the Hewardieae and the Petrosavieae but not in the Tricyrteae. Two vascular bundles occur in the stamens of the Hewartlieae and Tricyrtis latifolia. Ventral bundles in the upper part of the ovary of the Hewardieae are continuous with compound septal bundles and placental bundles in the lower part. Putative ventral bundles occur in the alternate position in the Tricyrteae and putative placental bundles in the opposite. position in the Petrosavieae. The dichtomously branched stigma in each carpel of the Tricyrteae is supplied by a bifurcated dorsal bundle.     

Enterovirus 71 3C proteolytically processes the histone H3 N-terminal tail during infection

Highlights
1. The N-terminal tail of histone H3 is specifically cleaved during EV71 infection.
2. Viral protease 3C is identified as a protease responsible for proteolytically processing the N-terminal H3 tail.
3. Our finding reveals a new epigenetic regulatory mechanism for Enterovirus 71 in virus-host interactions.     

Detection of EBV and HHV6 in the Brain Tissue of Patients with Rasmussen’s Encephalitis

Rasmussen’s encephalitis (RE) is a rare pediatric neurological disorder, and the exact etiology is not clear. Viral infection may be involved in the pathogenesis of RE, but conflicting results have reported. In this study, we evaluated the expression of both Epstein-Barr virus (EBV) and human herpes virus (HHV) 6 antigens in brain sections from 30 patients with RE and 16 control individuals by immunohistochemistry. In the RE group, EBV and HHV6 antigens were detected in 56.7% (17/30) and 50% (15/30) of individuals, respectively. In contrast, no detectable EBV and HHV6 antigen expression was found in brain tissues of the control group. The co-expression of EBV and HHV6 was detected in 20.0% (6/30) of individuals. In particular, a 4-year-old boy had a typical clinical course, including a medical history of viral encephalitis, intractable epilepsy, and hemispheric atrophy. The co-expression of EBV and HHV6 was detected in neurons and astrocytes in the brain tissue, accompanied by a high frequency of CD8⁺ T cells. Our results suggest that EBV and HHV6 infection and the activation of CD8⁺ T cells are involved in the pathogenesis of RE.     

Perinatal Vertical Transmission of Chikungunya Virus in Ruili,a Town on the Border between China and Myanmar

正Dear Editor,Chikungunya virus (CHIKV), an arbovirus in the family of Togaviridae, genus Alphavirus, is transmitted by the A.aegyptii or A. albopictus mosquito, and causes disease in humans characterized by fever, rash, and arthralgia (Silva and Dermody 2017; Suhrbier 2019). It was first reported in 1953 in Tanzania, and caused only a few outbreaks and sporadic cases in Africa and Asia in last century. However, in the epidemic in 2004, CHIKV acquired mutations that conferred enhanced transmission by the A. albopictus mosquito(Schuffenecker et al. 2006). Since then, it has successively caused outbreaks in Africa, the Indian Ocean, South East Asia, the South America, and Europe (Zeller et al. 2016).     

Development of a Novel Reverse Transcription Loop-Mediated Isothermal Amplification Method for Rapid Detection of SARS-CoV-2

In conclusion, the novel visual RT-LAMP assay is a simple, rapid, and sensitive approach for detection of SARS-CoV-2, and it is ready for application in primary care and community hospitals or health care centers, and even patients' own houses in response to the current SARS-CoV-2 epidemic because the assay does not require sophisticated equipment and skilled personnel. Furthermore, it is also ready to be used in fields for screening samples from wild animals and environments to facilitate the identification of potential intermediate hosts that mediate the cross-species transmission of SARS-CoV-2 from bats to humans.