Metaphor Literal Meaning Representation and Generation

在隐喻理解中,隐喻字面语义表示是隐喻深层语义表示的前提;确切地说,隐喻字面语义表示语言作为隐喻计算的输入语言直接影响到隐喻的最终释义,因此隐喻字面语义表示对隐喻的机器理解有着重要的影响作用。但在国内学术界,还鲜有这方面的研究。鉴于此,该文结合汉语隐喻特点,从隐喻字面语义表示的角度出发,将汉语隐喻分为无嵌套隐喻和嵌套隐喻两种。并在分析隐喻字面语义(浅层语义信息和隐喻信息)的基础上,提出了隐喻角色依存表示语言作为隐喻字面表示语言,最后给出隐喻角色依存表示语言生成算法。实验表明,该方法引入到汉语隐喻解释机制中是富有成效的。The representation of the metaphor literal meaning is the premise of deeper semantic representation and the further processing of metaphor.In fact,as the input language of the metaphor computation system,the metaphor literal meaning representation language would influence the final semantic calcualtion results.In this paper,we first classify the Chinese Metaphor into two categories,the Un-Nested Metaphor and the Nested Metaphor,based on the analysis of Chinese metaphor characteristics.We further design the metaphor role dependency representation language to describe the metaphor literal meaning in terms of its shallow semantic and metaphor information.Finally,the experiments show that the proposed method is quite effective in interperating Chinese metaphor.国家自然科学基金资助项目(60373080);福建省青年科技人才创新资助项目(2008F3105

油酰乙醇胺对脂多糖诱导的THP-1细胞炎症因子表达的影响

目的探讨油酰乙醇胺(OEA)对细菌脂多糖(LPS)诱导的人急性白血病单核细胞(THP-1)中前炎症因子TNF-α、IL-1β、IL-6表达的影响,并初步探讨OEA作为过氧化物酶体增殖物激活受体-α(PPAR-α)激动剂参与对炎症调节的作用机制。方法体外培养的THP-1细胞,分别加入不同浓度的OEA(10,20,40μmol/L)或非诺贝特(100μmol/L)共同孵育1 h后,用1μg/mL LPS分别诱导6或24 h。采用RT-PCR、实时定量PCR和酶联免疫吸附检测测定细胞中TNF-α、IL-1β、IL-6 mRNA和蛋白的表达的变化,并使用实时定量PCR及Western blot方法检测PPAR-α及Toll样受体4(TLR4)的mRNA和蛋白的表达。结果相对于正常THP-1细胞,LPS诱导后细胞中炎症因子(TNF-α、IL-1β、IL-6)表达明显增加。OEA对TNF-α、IL-1β、IL-6 mRNA和蛋白的表达有抑制作用,并呈现出一定的剂量依赖性。且OEA在激活PPAR-α表达的同时能够抑制TLR4的表达。结论 OEA对LPS诱导的炎症反应有抑制作用,其机制可能与激活PPAR-α,下调TLR4的表达有关

油酰乙醇胺对血管紧张素Ⅱ诱导的血管平滑肌细胞增殖的影响

目的研究油酰乙醇胺(OEA)对血管紧张素Ⅱ(AngⅡ)刺激大鼠主动脉血管平滑肌细胞(VSMCs)增殖的抑制作用以及对p38信号通路的影响。方法分离大鼠胸主动脉,组织贴块法培养VSMCs,AngⅡ刺激VSMCs建立细胞增殖模型,不同浓度OEA(5,10,20μmol/L)作用后,用溴脱氧核苷尿嘧啶(BrdU)掺入的方法检测细胞增殖活性;流式细胞术检测细胞周期变化;Western-bolt法检测对P-p38和p38蛋白表达的影响。结果与AngⅡ组比较,随着OEA浓度升高,VSMCs的增殖受到抑制、G0/G1比例显著升高,G2/M比例显著降低,且P-p38和p38蛋白的表达量降低并呈浓度依赖关系。结论 OEA对VSMCs的增殖有抑制作用,其机制可能是抑制了p38MAPK信号通路

IL-18、IL-12及相关因子在大鼠实验性自身免疫心肌炎心肌中的表达时程和特征

目的:探讨IL-18、IL-12及相关细胞因子在大鼠实验性自身免疫心肌炎(EAM)心肌中的表达时程和特征。方法:以猪心脏肌球蛋白加等体积弗氏完全佐剂,辅结核杆菌H37Ra株之乳液为抗原,于Lewis大鼠双后肢皮下注射造模(EAM);用胶原酶灌流和网筛过滤法分离纯化心肌细胞;经免疫组化技术评估心肌损伤程度;按实时荧光定量法测急性期和慢性期,IL-18、IL-12及相关因子(IL-18R,IL-18RAcPL,IL-18BP以及IL-12p40,IL-12p35,IL-12Rβ1,IL-12Rβ2)mRNA表达情况。结果:IL-18、IL-12及相关因子表达主要在急性期,免疫后2周表达增多并达峰值(P<0.01,与正常对照组比较),4周后减少,并与EAM病程正相关;IL-18、IL-12及相关因子主要在巨噬细胞表达,其受体复合物在αβT细胞表达;慢性期仅IL-18BP在心肌细胞有表达。结论:IL-18、IL-12及相关因子参与EAM病理过程,各因子主要集中于急性期巨噬细胞和αβT细胞表达

Preparation of Morphology-Tuned γ-MnO_2 and Catalytic Performance for the Liquid-Phase Oxidation of Toluene

通过在回流法制备流程中引入CTAb(十六烷基三甲基溴化铵)、PEg6000(聚乙二醇6000)及P123(聚环氧乙烷-聚环氧丙烷-聚环氧乙烷三嵌段共聚物)等表面活性剂对γ-MnO2催化剂进行形貌控制,同时采用X射线衍射(Xrd)、扫描电镜(SEM)、n2吸附(bET)、热重分析(TgA)、O2程序升温脱附(O2-TPd)以及H2程序升温还原(H2-TPr)等技术对不同形貌γ-MnO2的结构、氧脱附及还原性能进行表征,并考察了其在常压和无溶剂条件下甲苯选择性氧化反应体系的催化特性.同时,对于陈化时间对形貌的影响作用进行了考察.结果表明:不同形貌的γ-MnO2的氧化还原特征及催化活性存在显著差异,其中在经PEg6000进行修饰的γ-MnO2中含有较多的阴离子空位及混合价态,因此有助于分子氧在表面的活化,具有较高的表面比活性;而经P123进行表面修饰的γ-MnO2成晶结构规整、比表面积大,对甲苯液相直接氧化反应则表现出最佳的质量比活性,甲苯转化率达18.1%,含氧化合物总选择性为87.4%,其中苯甲酸的选择性达到73.2%.Introducing surfactants including hexadecyltrimethylammonium bromide (CTAB),macrogol 6000 (PEG6000),and poly(ethylene glycol)-block-poly(propylene glycol)-block-poly(ethylene glycol) triblock copolymer (P123) into the refluxing aqueous crystal nucleus slurry yielded morphology-tuned microcrystalline γ-MnO2.γ-MnO2 and the influence of surfactant modification were investigated by X-ray diffraction (XRD),scanning electron microscopy (SEM),N2 adsorption (BET),thermogravimetry analysis (TGA),O 2 temperature programmed desorption (O2-TPD),and temperature programmed H2 reduction (H 2-TPR).Surfactants led to differences in γ-MnO2 morphology,surface area,oxygen desorption behavior and reducibility.The effect of reflux time on catalyst morphology is discussed.The catalytic performance of γ-MnO2 during the solvent-free atmospheric oxidation of toluene was evaluated.PEG6000 modified γ-MnO2 exhibited the highest catalytic activity judging by surface area because of a greater mixed valency and more anion vacancies.The greatest mass specific activity was obtained for P123 modified γ-MnO2 with the largest surface area.Optimized reaction conditions yielded an 18.1% toluene conversion,and 87.4 and 73.2% total selectivity and selectivity for benzoic acid,respectively.国家重点基础研究发展规划项目(973)(2010CB226903)资助~

Au(Ⅲ)离子在黑曲霉菌上的吸附热力学和动力学特性

以黑曲霉菌作为生物吸附剂,研究其对Au(Ⅲ)离子的吸附特性,考察了pH值、吸附时间、温度和初始Au(Ⅲ)离子浓度等因素对吸附过程的影响。结果表明,Au(Ⅲ)离子在黑曲霉菌上的吸附过程对溶液pH值具有一定的依赖性,最佳pH值为2.0～3.0。升温能明显加快吸附进程,20℃下吸附过程分为2个阶段进行,分别对应于Au(Ⅲ)离子还原前和还原后的吸附,24h后吸附趋于平衡,而30℃、40℃、60℃下吸附过程均无明显分段现象,并分别于12h、6h和1h后趋于吸附平衡。Au(Ⅲ)离子初始浓度367.94mg·L–1时,升温明显促进了吸附的进行。Au(Ⅲ)离子在黑曲霉菌上的吸附等温线可用Langmuir方程很好地模拟,20℃、30℃、40℃和50℃时其饱和吸附量分别为185.19mg·g–1、202.02mg·g–1、235.85mg·g–1和277.78mg·g–1。热力学参数吉布斯自由能变(0ΔG)、吸附焓变(0ΔH)和吸附熵变(0ΔS)的计算结果表明,Au(Ⅲ)离子在黑曲霉菌上的吸附过程是一个自发的吸热和熵增过程。其吸附动力学可用准二级速率方程描述,吸附活化能为55.71kJ·mol–1。傅立叶变换红外光谱分析的结果进一步揭示了菌体表面的酰氨基、羧基和羟基是参与吸附的主要功能基团

Preparation and application of monoclonal antibodies against Herpes simplex virus-1

目的:制备并筛选HSV-1单抗,建立定量检测HSV-1病毒颗粒抗原的双抗体夹心ElISA方法,用于HSV-1病毒颗粒的质控。方法:以HSV-1免疫bAlb/C小鼠制备单克隆抗体,以筛选的中和单克隆抗体1f6为捕捉抗体,HrP标记的2b1为检测抗体,构建定量检测HSV-1病毒颗粒抗原的双抗体夹心ElISA方法,并对本方法的特异性、灵敏度、精密度、准确性和线性等性能进行验证。用本方法定量检测的病毒量与病毒滴度作回归分析。结果:构建的双抗体夹心定量检测HSV-1病毒颗粒抗原的ElISA方法,线性范围为0.125~2μg/Ml,相关系数为r2=0.995 5,定量限度为0.125μg/Ml,试剂的变异系数CV<10%,抗原回收率介于85.6%~107.1%之间。与HSV-1以外的其他样本无交叉反应。本方法检测与病毒感染滴度具有很好的相关性。结论:成功构建了定量检测HSV-1含量的ElISA方法,为HSV-1病毒颗粒抗原定量检测提供快速手段。Objective: To prepare and screen monoclonal antibodies against Herpes simplex virus-1( HSV-1),and develop a double antibody sandwich quantitative enzyme-linked immunosorbent assay( Q-ELISA) for detection of HSV-1 particle.This method was used to control the quality of viral particle in the developing and manufacturing process of HSV-1.Methods: BALB / c mice was immunized with HSV-1 to prepare monoclonal antibodies.A double antibody sandwich Q-ELISA was developed to determine concentration of HSV-1 particle,which was based on the neutralizing monoclonal antibody 1F6 as capture antibody,and 2B1 as HRP-conjugated antibody.The performance of the reagent was evaluated,including specificity,sensitivity,precision,accuracy and linear.And the relation between the amount of virus detected by this method and the virus titer was analyzed by regression analysis method.Results: The QELISA for HSV-1 particle was developed.The quantitation scope was 0.125- 2 μg / ml,the coefficient correlation was 0.995 5,the limit of detection was 0.125 μg / ml,the recovery was between 85.6% and 107.1%,the variation coefficient was lower than 10%,and the reagent does not react with other samples except HSV-1 antigen.This method has a good correlation with virus titer.Conclusion: The QELISA for HSV-1 particle was successfully developed,which provide a new approach for rapid and quantitative detection of HSV-1 antigen

黑曲霉负载银纳米颗粒的制备及其抗菌性能

采用非酶还原法,以黑曲霉菌原位还原银氨离子制备一种新型银纳米颗粒(AgNPs)/菌体复合抗菌材料,着重考察了反应温度与pH值对还原过程和所得复合材料的抗菌性能及稳定性的影响。结果表明,在温度为30℃、60℃和pH 9.5、11.5条件下,能够合成出粒径为6.9～8.2nm的近球形AgNPs。该AgNPs均匀地分布在菌体表面上,对E.coli显示出高的抗菌性能:最小抑菌浓度(MIC)为217～434mg·L-1(以菌粉总质量表示)或8～20mg Ag·L-1(以银含量表示)。提高反应温度有利于提高菌体银负载量,但AgNPs粒径增大,抗菌性能有所下降;提高反应pH值有利于提高还原速率,而对抗菌性能影响不显著。复合材料中AgNPs与菌体结合牢固,单位质量复合材料释出的Ag+含量为1.7～6.8mg.g-1,提高反应温度和pH值后Ag+的释出均减少

Development of a quantitative ELISA detection method for Coxsackievirus A group 16 strain(CA16) antigen

目的:建立柯萨奇病毒A组16型(CA16)抗原的双抗体夹心ElISA定量检测方法,用于CA16灭活疫苗的研发和生产过程的抗原定量检测。方法:以CA16中和单抗T26H12为包被抗体、nA14b9为标酶抗体,构建定量检测CA16抗原的双抗体夹心ElISA方法,并对方法的特异性、灵敏度、精密度、准确性、线性和稳定性进行分析。结果:建立了双抗体夹心定量检测CA16抗原的ElISA方法。方法的线性相关系数r2=0.998,线性范围为8~128 ng/Ml,定量限度为8 ng/Ml;变异系数CV80%;与CA16以外的其他样本没有交叉反应。结论:构建的CA16抗原ElISA定量检测方法的各项性能符合定量检测需要,可用于CA16疫苗的研发和生产过程的抗原活性的定量检测。Objective:To develop an a quantitative enzyme linked immunosorbent assay(Q-ELISA) to determine the concentration of Coxsackievirus A Group 16 Strain(CA16) antigen.This method was used to determine CA16 antigen content at each stage of CA16 vaccine developing and manufacturing process.Methods:A double antibody sandwich Q-ELISA was developed to determine concentration of CA16 antigen,which was based on the high-affinity neutralizing monoclonal antibodies T26H12 as capture antibodies,and NA14B9 as HRP-labeled antibody.The performance of reagent were evaluated.Results:The Q-ELISA for CA16 antigen content was successfully developed.The reagent had good performance.The quantitation scope was 8-128 ng/ml,the coefficient correlation was 0.998,the limit of detection was 8 ng/ml,the recovery was between 87% and 113.8%.The stability was up to 80% after reagent was heated for 6 days at 37℃.The variation coefficient was lower than 15%,and thereagent was no reaction with other sample except CA16 antigen.Conclusion:The Q-ELISA for CA16 antigen was developed with good specificity,accuracy,precision and stability.The method can be used to determine CA16 antigen content during development and production of CA16 vaccine

Development of aquantitative ELISA detection method for Varicella Zoster Virus(VZV) antigen

目的:建立水痘-带状疱疹病毒(VzV)抗原的双抗体夹心ElISA定量检测方法,用于质控VzV灭活疫苗研发和生产中抗原含量。方法:以VzV中和单抗5f6C8为包被抗体、8H5d1为酶标抗体,构建定量检测VzV抗原的双抗体夹心ElISA方法,并对本方法的特异性、灵敏度、准确性、线性和稳定性等性能进行分析。结果:建立的双抗体夹心定量检测VzV抗原的ElISA方法,线性范围为0.4μg~13μg/Ml,相关系数为r2=0.994,定量限度为0.4μg/Ml;变异系数CV80%。与VzV以外的相关病毒样本没有交叉反应。结论:构建的VzV抗原ElISA定量检测方法的各项性能符合定量检测需要,可用于VzV灭活疫苗的研发和生产过程的抗原含量检测。Objective:To develop a quantitative enzyme linked immunosorbent assay(Q-ELISA) to determine the concentration of Varicella Zoster Virus(VZV) antigen.This method was used to determine VZV antigen content at each stage of VZV inactived vaccine developing and manufacturing process.Methods: A double antibody sandwich Q-ELISA was developed to determine concentration of VZV antigen,which was based on the the high-affinity neutralizing monoclonal antibodies 5F6C8 as capture antibodies,and 8H5D1 as HRP-labeled antibody.The performance of reagent were evaluated.Results: The Q-ELISA for VZV antigen content was successfully developed.The reagent had good performance.The quantitation scope was 0.4 μg~13 μg/ml,The coefficient correlation was 0.994,the limit of detection was 0.4 μg /ml,the recovery was between 87.5% and 111.6%.The stability was up to 80% after reagent was heated for 6 days at 37℃.The variation coefficient was lower than 15%,and the reagent was no reaction with other sample except VZV antigen.Conclusion: The Q-ELISA for VZV antigen was developed with good specificity,accuracy and stability.The method can be used to determine VZV antigen content during development and production of VZV inactived vaccine