期刊文献+
共找到304篇文章
< 1 2 16 >
每页显示 20 50 100
MicroRNA-regulated viral vectors for gene therapy 被引量:10
1
作者 Anja Geisler Henry Fechner 《World Journal of Experimental Medicine》 2016年第2期37-54,共18页
Safe and effective gene therapy approaches require targeted tissue-specific transfer of a therapeutic transgene.Besides traditional approaches, such as transcriptional and transductional targeting, micro RNA-dependent... Safe and effective gene therapy approaches require targeted tissue-specific transfer of a therapeutic transgene.Besides traditional approaches, such as transcriptional and transductional targeting, micro RNA-dependent posttranscriptional suppression of transgene expression has been emerging as powerful new technology to increase the specificity of vector-mediated transgene expression. Micro RNAs are small non-coding RNAs and often expressed in a tissue-, lineage-, activation- or differentiation-specific pattern. They typically regulate gene expression by binding to imperfectly complementary sequences in the 3' untranslated region(UTR) of the m RNA. To control exogenous transgene expression, tandem repeats of artificial micro RNA target sites are usually incorporated into the 3' UTR of the transgene expression cassette, leading to subsequent degradation of transgene m RNA in cel s expressing the corresponding micro RNA. This targeting strategy, first shown for lentiviral vectors in antigen presenting cells, has now been used for tissue-specific expression of vector-encoded therapeutic transgenes, to reduce immune response against the transgene, to control virus tropism for oncolytic virotherapy, to increase safety of live attenuated virus vaccines and to identify and select cell subsets for pluripotent stem cell therapies, respectively. This review provides an introduction into the technical mechanism underlying micro RNA-regulation, highlights new developments in this field and gives an overview of applications of micro RNA-regulated viral vectors for cardiac, suicide gene cancer and hematopoietic stem cell therapy, as well as for treatment of neurological and eye diseases. 展开更多
关键词 Micro rna Micro rna regulation Micro rna target sites viral vectors Adeno-associated virus rna interference Gene therapy Vector targeting
下载PDF
HCV-RNA positivity in peripheral blood mononuclear cells of patients with chronic HCV-infection: does it really mean viral replication? 被引量:29
2
作者 Volker Meier Sabine Mihm +1 位作者 Perdita Wietzke-Braun Guliano Ramadori 《World Journal of Gastroenterology》 SCIE CAS CSCD 2001年第2期228-234,共7页
AIM: To analyze the association of HCV-RNA with peripheral blood mononuclear cells (PBMC) and to answer the question whether HCV-RNA positivity in PBMC is due to viral replication. METHODS: HCV-RNA was monitored in se... AIM: To analyze the association of HCV-RNA with peripheral blood mononuclear cells (PBMC) and to answer the question whether HCV-RNA positivity in PBMC is due to viral replication. METHODS: HCV-RNA was monitored in serum and PBMC preparations from 15 patients with chronic HCV infection before, during and after an IFN-alpha therapy using a nested RT/PCR technique. In a second approach, PBMC from healthy donors were incubated in HCV positive plasma. RESULTS: In the IFN-alpha responding patients,HCV-RNA disappeared first from total RNA preparations of PBMC and then from serum. In contrast, in relapsing patients, HCV-RNA reappeared first in serum and then in PBMC. A quantitative analysis of the HCV-RNA concentration in serum was performed before and after transition from detectable to non detectable HCV-RNA in PBMC-RNA and vice versa. When HCV-RNA was detectable in PBMC preparations, the HCV concentration in serum was significantly higher than the serum HCV-RNA concentration when HCV-RNA in PBMC was not detectable. Furthermore, at no time during the observation period was HCV specific RNA observed in PBMC, if HCV-RNA in serum was under the detection limit. Incubation of PBMC from healthy donors with several dilutions of HCV positive plasma for two hours showed a concentration dependent PCR positivity for HCV-RNA in reisolated PBMC. CONCLUSION: The detectability of HCV-RNA in total RNA from PBMC seems to depend on the HCV concentration in serum. Contamination or passive adsorption by circulating virus could be the reason for detection of HCV-RNA in PBMC preparations of chronically infected patients. 展开更多
关键词 Adult Aged Antiviral Agents Female HEPACIVIRUS Hepatitis C Chronic Humans INTERFERON-ALPHA Leukocytes Mononuclear Male Middle Aged rna viral Research Support Non-U.S. Gov't Reverse Transcriptase Polymerase Chain Reaction viral Load Virus Replication
下载PDF
Intracellular Transport of HIV-1 Matrix Protein Associated with Viral RNA
3
作者 Anatoliy I. Gozhenko Valentina A. Divocha +2 位作者 Galina K. Vorkunova Alissa G. Bukrinskaya Sergey I. Lupandin 《World Journal of AIDS》 2013年第1期33-35,共3页
HIV-1 matrix protein (MA) is a multifunctional structural protein localized on N terminus of Gag precursor p55. MA participates in HIV-1 assembly as membranotropic part of Gag precursor as well as an individual protei... HIV-1 matrix protein (MA) is a multifunctional structural protein localized on N terminus of Gag precursor p55. MA participates in HIV-1 assembly as membranotropic part of Gag precursor as well as an individual protein spliced from Gag early in infection. MA is found in the nuclei of infected cells and in plasma membrane, the site of virus assembly, in association with viral genome RNA. MA mutated variant M4 which contains two changed amino acids in N-terminal regions is also associated with viral RNA, but it is localized in the nuclear and cytoskeleton fractions but not in the plasma membrane suggesting that the mutant is deprived of membranotropic signal and “sticks” in the nuclei an d cytoskeleton, its previous location sites. These data allow suggesting that MA involved into transmission of viral RNA is transported to plasma membrane by cytoskeleton. 展开更多
关键词 HIV-1 Matrix Protein GAG PRECURSOR P55 CYTOSKELETON viral rna Transport of viral Complex Plasma Membranes Cell Fractionatiomn
下载PDF
Reverse genetics: Unlocking the secrets of negative sense RNA viral pathogens 被引量:1
4
作者 Kathryn Edenborough Glenn A Marsh 《World Journal of Clinical Infectious Diseases》 2014年第4期16-26,共11页
Negative-sense RNA viruses comprise several zoonotic pathogens that mutate rapidly and frequently emerge in people including Influenza, Ebola, Rabies, Hendra and Nipah viruses. Acute respiratory distress syndrome, enc... Negative-sense RNA viruses comprise several zoonotic pathogens that mutate rapidly and frequently emerge in people including Influenza, Ebola, Rabies, Hendra and Nipah viruses. Acute respiratory distress syndrome, encephalitis and vasculitis are common disease outcomes in people as a result of pathogenic viral infection, and are also associated with high case fatality rates. Viral spread from exposure sites to systemic tissues and organs is mediated by virulence factors, including viral attachment glycoproteins and accessory proteins, and their contribution to infection and disease have been delineated by reverse genetics; a molecular approach that enables researchers to experimentally produce recombinant and reassortant viruses from cloned cD NA. Through reverse genetics we have developed a deeper understanding of virulence factors key to disease causation thereby enabling development of targeted antiviral therapies and well-defined live attenuated vaccines. Despite the value of reverse genetics for virulence factor discovery, classical reverse genetic approaches may not provide sufficient resolution for characterization of heterogeneous viral populations, because current techniques recover clonal virus, representing a consensus sequence. In this review the contribution of reverse genetics to virulence factor characterization is outlined, while the limitation of the technique is discussed withreference to new technologies that may be utilized to improve reverse genetic approaches. 展开更多
关键词 Reverse genetics viral pathogen NEGATIVE SENSE rna viruses Influenza A VIRUS EBOLA VIRUS RABIES VIRUS Hendra VIRUS Nipah VIRUS
下载PDF
Investigation on Viral Pathogens in <i>Vitis vinifera</i>from Four Production Bases in Hangzhou Vicinity of China by sRNAseq and Molecular Validation
5
作者 Hongmei Li Lingzhu Wei +1 位作者 Jiang Wu Nongnong Shi 《American Journal of Plant Sciences》 2021年第12期1791-1799,共9页
This is the first systematic investigation of viral pathogens in <i>Vitis</i> <i>vinifera</i> from Hangzhou vicinity of China. About 7 viruses and 5 viroids were annotated from four production ... This is the first systematic investigation of viral pathogens in <i>Vitis</i> <i>vinifera</i> from Hangzhou vicinity of China. About 7 viruses and 5 viroids were annotated from four production bases “Dushicun”, “Wangjiayuan”, “Xiajiangcun”, and “Yangducun” covering 15 cultivars through sRNAseq technique. At least 3 viruses<a name="OLE_LINK4"></a>—grapevine leaf roll-associated virus 3 (GLRaV-3), grapevine fleck <span>virus (GFkV) and grapevine geminivirus A (GGVA), and 4 viroids—hop stunt</span> viroid (HSVd), citrus viroid II (CVd-II), grapevine yellow speckle viroid 1 (GYSVd-1) and grapevine yellow speckle viroid 2 (GYSVd-2) infected all four bases. “Yangducun” base showed 11, the most infected pathogens. GYSVd-1 showed the highest accumulation in host of Wangjiayuan base. The main in<span>fected pathogens were verified by reverse-transcription polymerase chain reaction</span> (RT-PCR) technique, the detected rate reached to 85% - 100%. The results provide an important basis for effective and precise detection of viral diseases in the area and for the virus-free cultivation in future. 展开更多
关键词 Vitis vinifera viral Disease Small rna Deep Sequencing RT-PCR
下载PDF
植物RNA作为载体RNA在病毒核酸提取过程中的保护效果研究
6
作者 江嘉琦 李江峰 +3 位作者 彭运平 胡霏 何小维 王羽 《检验医学与临床》 CAS 2024年第13期1875-1879,1884,共6页
目的探究植物RNA作为载体RNA在病毒核酸提取过程中对目标核酸的保护效果。方法分别提取绿萝、水稻、竹子3种常见植物中的RNA作为载体RNA,同时以商业试剂Takara载体RNA为对照,提取甲型流感病毒(Flu A)、乙型流感病毒(Flu B)、呼吸道合胞... 目的探究植物RNA作为载体RNA在病毒核酸提取过程中对目标核酸的保护效果。方法分别提取绿萝、水稻、竹子3种常见植物中的RNA作为载体RNA,同时以商业试剂Takara载体RNA为对照,提取甲型流感病毒(Flu A)、乙型流感病毒(Flu B)、呼吸道合胞病毒A型(RSV A)核酸,并利用实时荧光定量反转录聚合酶链反应(RT-qPCR)定量分析提取得到的病毒核酸浓度,以评估植物RNA在核酸提取中对病毒核酸的保护效果。结果经琼脂糖凝胶电泳检测,所提取植物RNA的28S rRNA、18S rRNA条带清晰明亮,无弥散现象,所得RNA具有良好的完整性。且经验证,植物RNA对病毒核酸扩增无干扰。裂解液中分别加入0、1000、3000、5000、7000、9000 ng绿萝RNA进行Flu A RNA提取时,提取物经RT-qPCR扩增后的Ct值分别为35.06±0.14、33.01±0.42、32.45±0.33、31.95±0.34、31.74±0.28、31.92±0.24,使用Takara载体RNA提取核酸的Ct值为31.96±0.34。Ct值随着绿萝RNA添加量增加而降低,当添加量≥5000 ng时,Ct值接近使用Takara载体RNA的提取组,继续提高绿萝RNA用量,Ct值趋于稳定,且与使用TaKaRa载体RNA的Ct值比较,差异无统计学意义(P>0.05)。添加5000 ng绿萝RNA与添加0 ng绿萝RNA相比,Ct值相差3.11,根据浓度差等于2ΔCt计算可知添加5000 ng绿萝RNA提取得到的Flu A核酸浓度比不添加载体RNA高了8.63倍。进一步研究发现,添加绿萝RNA、水稻RNA、竹子RNA及Takara载体RNA,提取得到的Flu A、Flu B和RSV A核酸经RT-qPCR扩增后得到的Ct值与不添加载体RNA比较,差异均有统计学意义(P<0.05)。绿萝RNA作为载体RNA在提取Flu A、Flu B、RSV A混合病毒核酸时,对比无载体RNA的对照组,分别降低了2.61、2.90、1.45个Ct值,即添加了绿萝RNA后提取Flu A、FluB、RSV A所得的核酸浓度分别提高了6.11、7.46、2.73倍。且添加了水稻RNA和竹子RNA提取混合病毒核酸所得的核酸浓度也分别至少提高了2.63倍和2.60倍。结论在病毒核酸提取过程中植物RNA具有保护病毒核酸的作用,可以提高提取得到的目的病毒RNA浓度,可用作病毒核酸提取时的载体RNA,为核酸提取中的载体RNA选择提供更多来源。 展开更多
关键词 植物rna 载体rna 病毒检测 病毒rna提取 核酸保护
下载PDF
Predictions in Clinical Efficiency of SARS-CoV-2 RNA-Dependent RNA Polymerase (RdRp) Inhibitors by Molecular Docking
7
作者 Pui-Jen Tsai 《Journal of Biosciences and Medicines》 2024年第10期178-196,共19页
This study utilizes the enzyme-substrate complex theory to predict the clinical efficacy of COVID-19 treatments at the biological systems level, using molecular docking stability indicators. Experimental data from the... This study utilizes the enzyme-substrate complex theory to predict the clinical efficacy of COVID-19 treatments at the biological systems level, using molecular docking stability indicators. Experimental data from the Protein Data Bank and molecular structures generated by AlphaFold 3 were used to create macromolecular complex templates. Six templates were developed, including the holo nsp7-nsp8-nsp12 (RNA-dependent RNA polymerase) complex with dsRNA primers (holo-RdRp-RNA). The study evaluated several ligands—Favipiravir-RTP, Remdesivir, Abacavir, Ribavirin, and Oseltamivir—as potential viral RNA polymerase inhibitors. Notably, the first four of these ligands have been clinically employed in the treatment of COVID-19, allowing for comparative analysis. Molecular docking simulations were performed using AutoDock 4, and statistical differences were assessed through t-tests and Mann-Whitney U tests. A review of the literature on COVID-19 treatment outcomes and inhibitors targeting RNA polymerase enzymes was conducted, and the inhibitors were ranked according to their clinical efficacy: Remdesivir > Favipiravir-RTP > Oseltamivir. Docking results obtained from the second and third templates aligned with clinical observations. Furthermore, Abacavir demonstrated a predicted efficacy comparable to Favipiravir-RTP, while Ribavirin exhibited a predicted efficacy similar to that of Remdesivir. This research, focused on inhibitors of SARS-CoV-2 RNA-dependent RNA polymerase, establishes a framework for screening AI-generated drug templates based on clinical outcomes. Additionally, it develops a drug screening platform based on molecular docking binding energy, enabling the evaluation of novel or repurposed drugs and potentially accelerating the drug development process. 展开更多
关键词 AlphaFold 3 rna-Dependent rna Polymerase Anti-viral Drugs Molecular Docking
下载PDF
病毒编码的RNA沉默抑制子的特征及其生物技术应用 被引量:3
8
作者 孙燕霞 刘红梅 《山东科学》 CAS 2008年第2期21-26,38,共7页
RNA沉默是一种依赖核酸序列特异性的RNA降解过程,是动物、植物抵抗病毒等外源核酸的一种保守防御机制。而针对寄主的这种防御机制,许多病毒演化出RNA沉默抑制子以克服这种防御反应。本文综述了几种动物、植物病毒抑制子的结构和作用方式... RNA沉默是一种依赖核酸序列特异性的RNA降解过程,是动物、植物抵抗病毒等外源核酸的一种保守防御机制。而针对寄主的这种防御机制,许多病毒演化出RNA沉默抑制子以克服这种防御反应。本文综述了几种动物、植物病毒抑制子的结构和作用方式,讨论了病毒抑制子之间的交叉抑制功能,病毒运动和沉默抑制子之间的关系,病毒RNA和亚病毒寄生物通过沉默抑制子而进行的自我保护原理,抑制子对于miRNA(microRNA)途径的影响以及病毒抑制子在生物技术方面的应用。 展开更多
关键词 rna沉默 病毒沉默抑制子 小分子干扰rna rna
下载PDF
ceRNA调控网络在冠心病中的研究进展 被引量:1
9
作者 马露 杨雷 +4 位作者 李菀榆 文江 谭维(综述) 邓常清 张伟(审校) 《临床与病理杂志》 CAS 2022年第12期3107-3116,共10页
冠状动脉粥样硬化性心脏病(coronary atherosclerotic heart disease,CHD)是威胁人类健康的严重疾病之一,深入研究其病理机制对于其诊疗具有重要意义。非编码RNA(non-coding RNA,ncRNA)在CHD的发生、发展中发挥重要作用,而竞争性内源RNA... 冠状动脉粥样硬化性心脏病(coronary atherosclerotic heart disease,CHD)是威胁人类健康的严重疾病之一,深入研究其病理机制对于其诊疗具有重要意义。非编码RNA(non-coding RNA,ncRNA)在CHD的发生、发展中发挥重要作用,而竞争性内源RNA(competing endogenous RNA,ceRNA)揭露了ncRNA在CHD中的关键作用。各种ncRNA、假基因、病毒转录物作为ceRNAs参与CHD的血管内皮损伤与修复、血管新生、脂质代谢、细胞外基质降解、炎症反应、细胞衰老、氧化应激损伤等病理过程。此外,部分ncRNAs还具有诊断和治疗的作用。深入研究ceRNA调控机制在CHD中的关键作用,对于CHD的病理机制研究、早期诊断、靶向药物研制具有重要的参考和借鉴价值。 展开更多
关键词 冠心病 竞争性内源rna 长链非编码rna 微小rna 环状rna 病毒转录物 串扰
下载PDF
RNA沉默在植物生物逆境反应中的作用 被引量:4
10
作者 谢兆辉 《遗传》 CAS CSCD 北大核心 2010年第6期561-570,共10页
RNA沉默是真核生物共有的基因表达调节机制和防御机制。在植物RNA沉默中,一些小RNAs,如微小RNAs和小干扰RNAs,在植物防御病毒、细菌或食草动物的反应中具有重要作用。为了抑制宿主的RNA沉默系统,植物病毒或细菌进化出了在RNA沉默不同阶... RNA沉默是真核生物共有的基因表达调节机制和防御机制。在植物RNA沉默中,一些小RNAs,如微小RNAs和小干扰RNAs,在植物防御病毒、细菌或食草动物的反应中具有重要作用。为了抑制宿主的RNA沉默系统,植物病毒或细菌进化出了在RNA沉默不同阶段起作用的病毒沉默抑制子或细菌沉默抑制子,来克服寄主的RNA沉默反应。文章就植物RNA沉默、病毒沉默抑制子、细菌沉默抑制子及其相关防御反应的一些新进展做一概述。 展开更多
关键词 rna沉默 微小rna 小干扰rna 病毒沉默抑制子 细菌沉默抑制子
下载PDF
非编码RNA与肝脏疾病
11
作者 石娟娟 党双锁 《世界华人消化杂志》 CAS 2016年第13期1952-1959,共8页
非编码RNA(non-coding RNA,ncRNA)是一类不具有编码蛋白质功能的RNA,在复制、转录和转录后等多种水平调控基因表达,参与细胞分化、个体发育和疾病发生发展等多种生物学进程.ncRNA表达或功能异常均与肝脏疾病的发生发展密切相关,目前研... 非编码RNA(non-coding RNA,ncRNA)是一类不具有编码蛋白质功能的RNA,在复制、转录和转录后等多种水平调控基因表达,参与细胞分化、个体发育和疾病发生发展等多种生物学进程.ncRNA表达或功能异常均与肝脏疾病的发生发展密切相关,目前研究显示肝细胞癌、病毒性肝炎和酒精肝损伤等肝脏疾病中有多种ncRNAs表达水平发生了显著变化,并在疾病的发生发展和预后中起着核心调控作用.因此,ncRNA的研究是生物学研究领域的热点和难点,有望成为肝脏疾病潜在的诊断标准、预后标志和临床治疗靶点. 展开更多
关键词 非编码rna 微小rna 长链非编码rna 肝细胞癌 病毒性肝炎
下载PDF
两种核酸提取方法对小鼠诺如病毒RNA提取效能的比较 被引量:7
12
作者 田胜男 苏静芬 +1 位作者 向志光 刘云波 《中国比较医学杂志》 CAS 2013年第9期57-60,共4页
目的比较两种核酸提取方法对小鼠诺如病毒RNA的提取效能。方法用Trizol提取法和QIAamp Viral RNA Mini Kit提取法分别提取感染小鼠诺如病毒(Murine Norovirus,MNV)的小鼠小肠组织样品RNA和细胞培养物RNA,测定RNA浓度;用MNV特异的引物对... 目的比较两种核酸提取方法对小鼠诺如病毒RNA的提取效能。方法用Trizol提取法和QIAamp Viral RNA Mini Kit提取法分别提取感染小鼠诺如病毒(Murine Norovirus,MNV)的小鼠小肠组织样品RNA和细胞培养物RNA,测定RNA浓度;用MNV特异的引物对分离的核酸样品进行一步法RT-PCR扩增。结果Trizol提取法提取小肠组织的RNA浓度高于QIAamp Viral RNA Mini Kit提取法;QIAamp Viral RNA Mini Kit提取得到的细胞培养物RNA浓度高于Trizol提取法。经QIAamp Viral RNA Mini Kit提取的两种核酸样品均能扩增出特异条带,而Trizol提取的核酸样品未见特异条带。结论在MNV的检测中,QIAamp Viral RNA Kit更适合组织样品中MNV病毒核酸的提取。 展开更多
关键词 TRIZOL QIAamp viral rna MINI KIT 小鼠诺如病毒
下载PDF
组织保护剂对病毒核酸与豚鼠皮肤组织样本RNA的保存效果探究
13
作者 李华 徐兰举 +3 位作者 黄学亮 王亚如 刁立琴 于月欣 《生物技术进展》 2024年第1期60-65,共6页
病毒核酸和生物组织样本RNA容易受到外部环境的影响,极易发生降解,造成实验结果产生严重偏差。以病毒核酸与豚鼠皮肤组织样本RNA为研究对象,探究组织保护剂保存它们在不同温度放置不同时间后,对病毒载量以及豚鼠皮肤组织样本中RNA的保... 病毒核酸和生物组织样本RNA容易受到外部环境的影响,极易发生降解,造成实验结果产生严重偏差。以病毒核酸与豚鼠皮肤组织样本RNA为研究对象,探究组织保护剂保存它们在不同温度放置不同时间后,对病毒载量以及豚鼠皮肤组织样本中RNA的保护效果。结果发现,在4℃保存30 d,25℃保存7 d或37℃保存24 h后,与初始病毒核酸量相比较,组织保护剂中保存的病毒载量未发生明显变化(P>0.05)。在4℃保存30 d,25℃保存7 d或37℃保存24 h后,与液氮储存组相比较,组织保护剂组与市售RNA later组均可以保持豚鼠皮肤组织中样本RNA的提取量和纯度,差异无统计学意义(P>0.05)。结果表明,组织保护剂可作为科研或临床组织样本的储存保存液,在4℃、25℃以及37℃条件下放置一定时间,不影响病毒核酸的病毒载量以及豚鼠皮肤组织样本RNA的提取量和纯度,使样本保存更简便高效。 展开更多
关键词 组织保护剂 病毒载量 组织样本rna 保护效果
下载PDF
Serum concentration of sFas and sFasL in healthy HBsAg carriers,chronic viral hepatitis B and C patients 被引量:7
14
作者 Tadeusz Wojciech Lapinski Oksana Kowalczuk +1 位作者 Danuta Prokopowicz Lech Chyczewski 《World Journal of Gastroenterology》 SCIE CAS CSCD 2004年第24期3650-3653,共4页
AIM:To estimate the amount of apoptosis among healthy HBsAg carriers,patients with chronic HBV infection treated wibh lamivudine and patients with chronic HCV infection treated with interferon alpha and ribavirin.Acti... AIM:To estimate the amount of apoptosis among healthy HBsAg carriers,patients with chronic HBV infection treated wibh lamivudine and patients with chronic HCV infection treated with interferon alpha and ribavirin.Activity of apoptosis was evaluated by serum sFas/sFasL concentration measurement. Moreover dependence between apoptosis and HBV-DNA or HCV-RNA levels was studied. METHODS:Eighty-six persons were included into study:34 healthy HBsAg carders,33 patients with chronic HBV infecl^on and 19 patients with chronic HCV infection.Serum levels of sFas/sFasL were measured by ELISA assay.HBV-DNA and HCV-RNA were measured by RT-PCR assay.Levels of sFas/sFasL were determined before and 2 and 12 wk after therapy in patients with chronic hepatitis B and C infection. HBV-DNA or HCV-RNA was detected before treatment and 6 mo after treatment. RESULTS:Twenty-four (71%) healthy HBsAg carders showed HBV-DNA over 10~5/mL,which was comparable to the patients with chronic hepatitis B.independently from HBV-DNA levels, the concentration of sFas among healthy HBsAg carders was comparable to healthy persons.Among patients with chronic hepatitis B and C,the concentration of sFas was significantly higher in comparison to healthy HBsAg carriers and healthy persons.In chronic hepatitis B patients the concentration of sFas was decreased during lamivudine treatment.Among chronic hepatitis C patients the concentration of sFas was increased during IFN alpha and ribavirin treatment,sFasL was not detected in control group.Furbhermore sFasL occurred more frequently in chronic hepatitis C patients in comparison to chronic hepatitis B patients. CONCLUSION:There are no correlations between apoptosis and HBV-DNA levels.However ther is an association between apoptosis and activity of inflammation in patients with chronic HBV infection.Apoptosis can be increased in patients with chronic hepatitis C by effective treatment which may be a result of apoptosis stimulation by IFN-α. 展开更多
关键词 Adolescent Adult Aged Antigens CD95 Apoptosis Biological Markers Carrier State DNA viral Female Hepatitis B Surface Antigens Hepatitis B Chronic Hepatitis C Chronic Humans LAMIVUDINE Male Membrane Glycoproteins Middle Aged rna viral Reverse Transcriptase Inhibitors Solubility
下载PDF
病毒感染相关microRNA的研究进展 被引量:1
15
作者 刘妍 徐东平 《胃肠病学和肝病学杂志》 CAS 2007年第1期90-94,共5页
关键词 MICROrna 非编码rna 病毒感染 基因调控
下载PDF
RNA编辑功能的研究进展 被引量:2
16
作者 郑玉姝 赵朴 刘兴友 《生命科学》 CSCD 2008年第3期454-457,共4页
RNA编辑产生RNA和蛋白质多样性。最近研究表明,RNA编辑在抗体多样性、病毒应答、剪接调节和miRNA调节方面发挥重要作用,并且越来越多的证据表明,RNA编辑与脑发育和神经性疾病的发生有关。因此,深入理解RNA编辑的功能有望促进我们理解这... RNA编辑产生RNA和蛋白质多样性。最近研究表明,RNA编辑在抗体多样性、病毒应答、剪接调节和miRNA调节方面发挥重要作用,并且越来越多的证据表明,RNA编辑与脑发育和神经性疾病的发生有关。因此,深入理解RNA编辑的功能有望促进我们理解这一与疾病诊断和治疗有关的有趣机制。 展开更多
关键词 rna编辑 抗体多样性 病毒应答 剪接调节 mirna调节
下载PDF
LncRNAs are potentially involved in the immune interaction between small brown planthopper and rice stripe virus 被引量:4
17
作者 CHEN Meng-yao YE Wan-yi +6 位作者 XIAO Hua-mei LI Mei-zhen CAO Zheng-hong YE Xin-hai ZHAO Xian-xin HE Kang LI Fei 《Journal of Integrative Agriculture》 SCIE CAS CSCD 2019年第12期2814-2822,共9页
Small brown planthopper(SBPH, Laodelphax striatellus Fallén) is an important vector of major crop pathogen rice stripe virus(RSV). Controlling SBPH population is an efficient approach to control RSV. Long non-cod... Small brown planthopper(SBPH, Laodelphax striatellus Fallén) is an important vector of major crop pathogen rice stripe virus(RSV). Controlling SBPH population is an efficient approach to control RSV. Long non-coding RNAs(lnc RNA) have been reported to block virus replication in hosts. However, the function of lnc RNAs in RSV infection and replication is still unknown. Here, we aimed to study regulatory mechanisms of lnc RNA in an immune system during RSV infection. First, lnc RNA genes were predicted from SBPH transcriptomes using a bioinformatics pipeline based on characteristics of lnc RNA. We identified 4 786 lnc RNA genes corresponding to 5 790 transcripts in SBPH from an RNA-Seq dataset of 15 transcriptomes. Differential expression analysis indicated that 3, 11, and 25 lnc RNA genes were highly expressed in gut, salivary gland, and ovary, respectively, of viruliferous SBPH(Student’s t-test, P<0.05). We randomly selected eight lnc RNAs for expression validation using quantitative real-time PCR, confirming the differential expression of these lnc RNAs between viruliferous and non-viruliferous SBPH. In summary, we present evidence that the expression of lnc RNA genes was induced by RSV infection, suggesting that RSV might be involved in the antivirus immune system in SBPH and participate in regulating the RSV replication mechanism. These data provide helpful information for future investigations of the interaction between lncRNA and RSV. 展开更多
关键词 lncrna SMALL BROWN PLANTHOPPER rice STRIPE virus rna-Seq viral infection
下载PDF
shRNA病毒递送载体
18
作者 杨洋 张均平 +1 位作者 王明席 许瑞安 《中国医药科学》 2013年第6期29-31,共3页
RNA干扰(RNA interference,RNAi)是一种有力的基因沉默工具,在功能基因组学、微生物学、基因表达调控机制研究等领域广泛应用。RNAi可以用于鉴定药物靶标及治疗疾病,尤其是传统治疗手段无效的重大疾病。如何将双链小干扰RNA(siRNA)高效... RNA干扰(RNA interference,RNAi)是一种有力的基因沉默工具,在功能基因组学、微生物学、基因表达调控机制研究等领域广泛应用。RNAi可以用于鉴定药物靶标及治疗疾病,尤其是传统治疗手段无效的重大疾病。如何将双链小干扰RNA(siRNA)高效传递至体内靶细胞是RNAi成功用于疾病治疗的关键,也是目前研究的热点。由于病毒载体能高效转导多种细胞成为基因工程和基因治疗的主要载体。目前,越来越多的研究将病毒载体应用于介导RNAi,然而病毒载体存在靶向性差、生物安全性等问题。本文针对这些病毒载体的优劣进行归纳并指出今后改进的方向。 展开更多
关键词 rna干扰 小干扰rna 病毒载体 短发夹rna
下载PDF
稳定表达靶向BVDV shRNA细胞系的建立及其对BVDV复制的影响
19
作者 范璐 王丽 +3 位作者 史西保 樊剑鸣 王爱萍 张改平 《河南农业科学》 CSCD 北大核心 2014年第12期134-139,共6页
为研究靶向牛病毒性腹泻病毒(BVDV)的shRNA对BVDV复制的影响,利用脂质体介导法将BVDV shRNA真核表达质粒pSGH1-sh1083和pSGH1-sh8235及对照质粒pSGH1转染MDBK细胞,通过G418抗性以及有限稀释法筛选获得BVDV shRNA单克隆细胞系subclonepSG... 为研究靶向牛病毒性腹泻病毒(BVDV)的shRNA对BVDV复制的影响,利用脂质体介导法将BVDV shRNA真核表达质粒pSGH1-sh1083和pSGH1-sh8235及对照质粒pSGH1转染MDBK细胞,通过G418抗性以及有限稀释法筛选获得BVDV shRNA单克隆细胞系subclonepSGH1-1083和subclonepSGH1-8235及对照细胞系subclonepshmock。通过观察其细胞病变效应(CPE)、测定TCID50及RT-PCR、流式细胞术检测BVDV shRNA细胞系对BVDV复制的影响。结果表明,与阴性对照组相比,单克隆细胞系subclonepSGH1-1083和subclonepSGH1-8235的细胞在感染BVDV 72h后CPE不明显,其TCID50低于阴性对照组;RT-PCR结果显示,单克隆细胞系subclonepSGH1-1083和subclonepSGH1-8235的细胞在感染BVDV后病毒E2基因的表达减弱;流式细胞术检测不同细胞系接毒24h后的结合率,单克隆细胞系subclonepSGH1-1083和subclonepSGH1-8235与病毒结合率分别为11.37%和11.51%,与对照组(20.25%)相比有所降低。综上,稳定转染BVDV shRNA的单克隆细胞系subclonepSGH1-1083和subclonepSGH1-8235对BVDV的复制具有抑制作用。 展开更多
关键词 rna干扰 牛病毒性腹泻病毒 短发夹rna 单克隆细胞系 复制
下载PDF
Circulating microRNAs as non-invasive biomarkers for hepatitis B virus liver fibrosis 被引量:4
20
作者 Diana Gabriela Iacob Adelina Rosca Simona Maria Ruta 《World Journal of Gastroenterology》 SCIE CAS 2020年第11期1113-1127,共15页
Viruses can alter the expression of host microRNAs(miRNA s) and modulate the immune response during a persistent infection. The dysregulation of host miRNA s by hepatitis B virus(HBV) contributes to the proinflammator... Viruses can alter the expression of host microRNAs(miRNA s) and modulate the immune response during a persistent infection. The dysregulation of host miRNA s by hepatitis B virus(HBV) contributes to the proinflammatory and profibrotic changes within the liver. Multiple studies have documented the differential regulation of intracellular and circulating miRNA s during different stages of HBV infection. Circulating miRNA s found in plasma and/or extracellular vesicles can integrate data on viral-host interactions and on the associated liver injury. Hence, the detection of circulating miRNA s in chronic HBV hepatitis could offer a promising alternative to liver biopsy, as their expression is associated with HBV replication, the progression of liver fibrosis,and the outcome of antiviral treatment. The current review explores the available data on miRNA involvement in HBV pathogenesis with an emphasis on their potential use as biomarkers for liver fibrosis. 展开更多
关键词 HEPATITIS B virus Microrna Noncoding rna Liver fibrosis viral HEPATITIS NON-INVASIVE biomarkers EXTRACELLULAR vesicles HEPATITIS management
下载PDF
上一页 1 2 16 下一页 到第
使用帮助 返回顶部