人耐药白血病细胞多药耐药基因-1小干扰RNA的构建及功能研究

目的:构建人耐药白血病细胞多药耐药基因-1小干扰RNA并研究其功能.方法:人工合成编码mdrl小发夹状双链RNA的DNA片段,与pSilencer4.1-CMV质粒连接构建RNAi真核表达栽体,采用脂质体介导法转染人耐药白血病细胞K562/A,经潮霉素B筛选转基因阳性克隆细胞,RT-PCR和Western Blotting检测转基因细胞中mdrl基因的表达量,MTT法检测转基因细胞对阿霉素的敏感性.结果:RT-PCR结果显示,与未转基因组和阴性对照组比较,RNA干扰组mdrl基因在mRNA水平上表达量降低43.55%;Western Blotting检测显示,RNA干扰组mdrl基因在蛋白水平上表达量降低69.46%;MTT法检测显示mdrl干扰细胞对化疗药物柔红霉素的敏感性提高23倍.结论:mdrl小发夹状RNA可显著抑制K562/A细胞中的mdrl基因的表达,提高白血病细胞对化疗药物的敏感性,对白血病多药耐药性的逆转和白血病的治疗具有重要理论和实际意义.     

Optimization of Electrofusion Parameters and Interspecific Somatic Hybrid Regeneration in Citrus

This study was primarily attempted to optimize the electrofusion parameters using protoplasts isolated from cell suspension cultures of "Page" tangelo ( Citrus reticulata Blanco x C. paradisi Macf) and mesophyll protoplasts of rough lemon ( Citrus jambhiri Lush) as fusion partners. It was shown that the binuclear heterokaryons frequency reached 15% with the following parameters: alternate current (AC) 125 V/cm, AC time 60 s, direct current (DC) 1 250 V/cm, DC pulse width 50 μs, DC pulse interval O. 5 s, No. of DC pulse 3. Considering the fact that different types of protoplasts have different specific weights, higher frequency of the binuclear heterokaryons was obtained by controlling the centrifugation time after fusion. The fusion products regenerated into plantlets after 3 to 4 months of culture. Chromosome counting of the root tips and morphological observation of the regenerants verified that 78% were tetraploids and the rest were diploids with the leaf morphology of mesophyll parent. Peroxidase (POX) isozyme and RAPD analysis indicated that interspecific somatic hybrids were obtained and an autotetraploid plant of mesophyll parent type was also verified.     

皱叶留兰香迁地栽培后的营养成分及抗性指标测定

皱叶留兰香 (ＭｅｎｔｈａｃｒｉｓｐａｔｅＳｃｈｒａｄ .ｅｘＷｉｌｌｄ .)为唇形科薄荷属 (ＭｅｎｔｈａＬ .)多年生宿根草本植物 ,原分布于地中海沿岸 ,我国云南及贵州等地也有分布。皱叶留兰香及薄荷属某些种类 ,在民间被广泛药用和食用。具有疏风散热、辟秽解毒之功效 ,常用于外感风热、头痛、目赤、食滞气胀、口疮、牙痛等症[1 ] ,现代研究表明薄荷属植物还具有抗病毒、杀菌、抗刺激、利胆[2 ] 及放疗区域皮肤保护[3] 等作用。食用则具有清凉芳香的口味特点 ,在我国西南地区已经成为普通蔬菜 ,广泛用于调料、生食和火锅等。作者对皱…     

日本血吸虫虫卵、童虫和雌雄成虫膜蛋白的双向电泳

血吸虫寄生生活复杂,中间宿主和终末宿主转换,有性繁殖和无性繁殖交替,由其感染引起的血吸虫病仍严重危害人畜健康(陈贤义等,2002).研究表明,血吸虫不仅能利用宿主的免疫信号分子伪装自己获得宿主的免疫兼容(Salzet et al.,2000),而且还在血吸虫中克隆到宿主信号分子的受体(Ahmed et al.,2001).     

血S100B蛋白和尿乳酸/肌酐比值对门静脉高压症术后肝性脑病发生的早期预测价值

目的评价血S100B蛋白和尿乳酸/肌酐对乙肝肝硬化门脉高压症术后肝性脑病发生的早期预测价值。方法回顾性分析65例乙肝肝硬化门脉高压症患者的临床资料,动态检测术后24、48和72h的血S100B蛋白和尿乳酸/肌酐比值水平,根据是否发生术后肝性脑病将受试者分为肝性脑病组与非肝性脑病组,并对肝性脑病组患者进行临床分度。结果乙肝肝硬化门脉高压症患者术后发生肝性脑病组72h内血S100B蛋白含量和24 h内尿乳酸/肌酐比值水平明显高于非肝性脑病组(P<0.001);72h内血S100B蛋白含量和24 h内尿乳酸/肌酐比值之间及与肝性脑病的临床分度呈正相关(P<0.001);当血S100B水平在28ng/L,尿乳酸/肌酐比值在0.47时,单独检测72h血S100B蛋白的敏感度、特异度分别为91.2%、93.6%;尿乳酸/肌酐比值预测肝性脑病的敏感度和特异性度以术后24h最高,分别为89.3%和91.7%;如检测72h血S100B蛋白的同时监测术后24h尿乳酸/肌酐比值可显著提高肝性脑病诊断的准确性,联合应用两项指标进行检测,诊断的敏感度和特异度分别为95.7%和98.6%,较两种方法单独应用敏感度和特异度均提高。结论对门静脉高压症患者术后以临床表现为基础,同时监测72h内血S100B蛋白和24h尿乳酸/肌酐比值,对提高术后肝性脑病的早期诊断和临床分度具有一定应用价值。     

铵减弱拟南芥主根向地性及其相关作用途径

向地性是决定植物根系空间构型的主要因素之一,对植物锚定和水分养分吸收至关重要。除了重力,根系向地性还受土壤环境因子影响。本文采用琼脂培养方法,研究了铵对拟南芥主根向地性反应的影响及相关作用途径。结果表明：短期内,不同浓度（NH4）2SO4均显著抑制主根向地性弯曲,但随着时间的延长,根尖向地性角度逐渐变小。而等（NH4）2SO4浓度的NaCl对主根向地性抑制效应较小,不同浓度的甘露醇不阻碍主根向地性弯曲。纽织化学染色结果显示铵处理12h以内,Col-0根尖没有淀粉体的快速降解过程,并且铵对淀粉体缺失突变体pgm—1主根向地性的影响同Col-0相似。铵处理部分恢复生长素转运载体突变体auxl-22和eir1-1主根向地性缺失。这些结果表明,铵对拟南芥主根向地性的影响独立于根尖淀粉体参与的重力感应途径。     

IDENTIFICATION OF NEW TARGET SEQUENCES FOR PCR DETECTION OF VIBRIO PARAHAEMOLYTICUS BY GENOME COMPARISON

A genome comparison method was used to identify specific target sequences for the polymerase chain reaction (PCR) detection of Vibrio parahaemolyticus, and the CDS value of this bacterium was compared with that of 139 other bacterial genomes. It was found that 20 CDS of V. parahaemolyticus were relatively specific according to their E value in BLAST (a new tool for comparing protein and nucleotide sequences), and four of them were selected for the design of PCR primers. There were positive amplification products of these four pairs of primers from nine V. parahaemolyticus strains, whereas there were no amplification products from nine other Vibrionaceae strains and four non -Vibrionaceae strains. An evaluation of detection sensitivities revealed that these four pairs of primers can be used in a PCR assay for the detection of V. parahaemolyticus.

PRACTICAL APPLICATIONS

An automatic BLAST method was developed in this study, by which species-specific sequences can be screened out rapidly. In this way, new and specific genes of Vibrio parahaemolyticus were identified to be used as target sequences for PCR detection. In terms of acceptable specificity and sensitivity, the four pairs of primers were selected by screening, which can be applied in PCR assays and other molecular methods. These kinds of methods might become commercial detection products in the new future. In addition, this method for searching specific DNA sequences can also be used for the mining specific sequences in other genus and species, such as Salmonella , Staphylococcus , etc.     

食物丰容对圈养猩猩行为的影响

于2007年2～4月对成都动物园圈养猩猩铁里进行了两个食物丰容试验,即用PVC+轮胎和圆木+轮胎试验,每期8 d,观察和记录了猩猩在丰容试验前、后以及两种丰容方式中的各种行为发生次数.结果 表明食物丰容有效地恢复了圈养猩猩的多种摄食行为,增加了猩猩的运动相关行为,减少了休息相关行为;但对刻板行为的影响不明显.     

蒺藜皂苷对动脉粥样硬化大鼠动脉壁ICAM-1、VCAM-1、PPARα、PPARγ基因表达的影响

观察全草蒺藜皂苷（tribu saponin from Tribulus terrestris,STT）对实验性动脉粥样硬化（atherosclerosis,AS）大鼠动脉壁中ICAM-1、VCAM-1、PPARα和PPARγ基因表达的影响,以探讨STT抗AS的机制。应用高脂饲料饮食配合注射维生素D,建立SD大鼠AS模型,并设立正常组、模型组、辛伐他汀组和蒺藜皂苷低、中、高剂量组。采用半定量RT-PCR的方法检测各组动物动脉壁中ICAM-1、VCAM-1、PPARα和PPARγ基因的表达,分析造模及各给药大鼠ICAM-1、VCAM-1、PPARα和PPARγ基因表达的变化。与正常组相比,模型组ICAM-1和VCAM-1基因的表达量明显增加（P〈0．01）,而PPARα和PPARγ基因的表达量明显降低（P〈0．01）;与模型组相比,辛伐他汀及各STT药均能降低ICAM-1和VCAM-1基因的表达量（P〈0．01～P〈0．05）,并能增加PPARα和PPARγ基因的表达量（P〈0．01）。提示STT能下调实验性AS大鼠动脉壁ICAM-1和VCAM-1基因的表达及上调PPARα和PPARγ基因表达,这可能是STT抗AS的作用机制之一。     

癫痫相关基因SCN1A启动子区多态性位点的生物信息学分析

SCN1A是多种神经系统疾病的致病基因,该基因的精确表达对于维持神经系统正常功能非常重要.为了认识SCN1A启动子区多态性位点(single nucleotide polymorphisms,SNPs)的保守性及其功能意义,应用生物信息学方法分析了目前已发表位于SCN1A启动子区的11个SNPs,分别命名S1～S11.分析结果表明,S3、S5和S7等位基因频率没有人种差异性,其余SNP等位基因频率均有人种差异性;接近核心启动子的SNPs要比远离核心启动子SNPs的保守程度高,提示靠近核心启动子的SNPs影响SCN1A基因表达的概率可能越大;大部分SNPs祖传等位基因在哺乳动物中是保守的(S3除外),暗示这些SNPs新生等位基因有可能在人类进化过程起到一定的作用:启动子分析软件预测发现,含S2、S4、S8及S9等4个SNPs不同等位基因的同一序列分别存在不同转录因子结合元件,而含S1和S11不同等位基因的同一序列都只能预测到含其中一个等位基因的序列存在转录因子结合元件,这些差异可能是SNPs影响SCN1A表达的重要原因之一.这些分析将为进一步研究SCN1A启动子区SNPs与神经系统疾病的相互关系打下基础.