应用代表性差异分析法筛选人癌候选抑癌基因

运用cDNA代表性差异分析法(cDNA representational difference analysis,cDNA RDA),以正常人鼻咽上皮细胞及鼻咽癌HNE1细胞作为比较的样品来源,分离了四个在鼻咽癌中缺失的cDNA片段.以此四个片段作探针,分别进行DNA杂交、RNA杂交,结果显示,这些差异性的cDNA序列确实来自正常人鼻咽上皮且只在其中表达和/或在鼻咽癌HNE1中表达降低,并在鼻咽癌病人中存在不同程度的缺失.序列分析结果表明这些差异性表达的基因为具有相当抑癌基因功能的已知基因和可能与鼻咽癌相关的抑癌基因的新基因.从而说明cDNA RDA是一种高效、敏感、假阳性低的克隆抑癌基因的有效方法.     

Identification of differentially expressed genes by restriction endonuclease-based gene expression fingerprinting.

A novel method for identification of differentially expressed genes has been developed. It is based on the consecutive restriction digestions of 3' terminal cDNA fragments to produce a fingerprint of gene expression. cDNA molecules are synthesized using a biotinylated oligo(dT) primer, digested with a frequently cutting restriction endonuclease and the 3'-terminal restriction fragments are isolated using streptavidin microbeads. After amplification by PCR, cDNA fragments are immobilized again on streptavidin beads, radiolabeled and treated sequentially with a set of restriction endonucleases. The products of individual enzymatic reactions from two or more different RNA populations are resolved by polyacrylamide gel electrophoresis and compared to reveal differentially expressed genes. This strategy enabled us to identify and clone the fragments of five genes expressed differentially in murine thymus and spleen. One of the genes was found to encode terminal deoxynucleotidyl transferase; others are apparently previously unknown genes.     

水稻条纹病毒胁迫下灰飞虱基因的差异表达

水稻条纹病毒(rice stripe virus, RSV)主要由介体昆虫灰飞虱Laodelphax striatellus以循回增殖型方式经卵传播, 目前RSV与灰飞虱间的互作研究很少。为了研究RSV侵染对灰飞虱基因表达的影响, 采用5条随机引物和3条锚定引物, 利用mRNA差异显示(differential display RT-PCR, DDRT-PCR)技术分析了带毒和无毒灰飞虱种群基因表达差异。且利用正交实验优化了DDRT-PCR反应体系中的模板浓度、锚定引物浓度、随机引物浓度、dNTPs浓度、镁离子浓度及Taq酶用量。结果表明: 最佳DDRT-PCR体系(25 μL)为cDNA 3.0 μg, 随机引物2.0 μmol/L, 锚定引物2.5 μmol/L, dNTPs 200 μmol/L, Mg²⁺ 2.0 μmol/L, Taq 酶2.0 U。mRNA差异显示共获得35条差异片段, 选取其中6条经RNA斑点杂交验证, 获得了4条阳性差异片段。其中3条阳性片段为带毒灰飞虱种群特异表达, 分别与5-羟色胺受体1D、 旋转酶B、 60S核蛋白L40高度同源, 无毒灰飞虱种群中特异表达的一条阳性片段在NCBI核酸数据库中比对无同源序列。DDRT-PCR优化体系的建立及部分差异片段的获得为进一步研究灰飞虱与RSV间的互作提供了帮助。     

Suppression subtractive hybridization identifies differentially expressed genes in Brassica napus chlorophyll-reduced mutant

Suppressive subtraction hybridization (SSH) was used to identify differentially expressed genes caused by a chlorophyll-reduced mutation in B. napus. The cDNA fragments, derived from SSH positive subtractive library (tester: normal wild type, driver: mutant) were cloned into pMD18-T vector. Two hundred SSH cDNA clones were screened by dot blot array, and 151 clones were identified as differentially expressed cDNA fragments in Cr3529 line. Thirty-six positive clones which showed marked expression differences were selected and sequenced. After redundant cDNAs were removed, 33 differentially expressed unique cDNA section clones were obtained. Among the 33 clones, two clones possess different parts of the cDNA sequence of the same gene coding geranylgeranyl reductase, four clones belong to unknown proteins, and the rest share homology to genes of diverse class. Sequence analysis showed that at least 12 genes were discovered to be related to the photosynthesis, seven of them coded the proteins which belong to the subunit of photosystem 2. RNA gel blot analysis showed that compared with 3529, the gene expression of the chlorophyll a/b-binding protein Lhcb2 in photosystem 2 declined markedly in the cotyledons and seedling leaves of Cr3529, indicating that the reduced light-harvesting complex 2 accumulation in thylakoid membrane of Cr3529 was due to the decrease of the related gene mRNA level for translation.     

日本血吸虫期别差异表达基因文库的构建及分析

为从期别差异表达基因分析入手研究血吸虫的生长发育机制,应用抑制性消减杂交 (suppressed subtractive hybridization , SSH) 技术首次构建了日本血吸虫尾蚴、虫卵和成虫的期别差异表达基因文库 . 经消减效率分析和三种文库克隆的 EST 的期别差异性鉴定,表明所建文库质量较高,为在整个基因组水平分离血吸虫的差异表达基因提供了重要材料 . 由三个文库选择 257 个插入片段大于 500 bp 的克隆测定了 EST 序列 . 同源性分析结果表明 257 个 EST 代表 182 种血吸虫基因,其中有 22 种为血吸虫已知基因,有 128 种为血吸虫已知 EST ,有 32 种为新发现的血吸虫基因 . 对 EST 编码蛋白的功能预测结果显示：尾蚴消减文库的基因多与运动、能量代谢、转录调节及致病性相关;虫卵消减文库的基因可能参与信号转导、细胞粘附、蛋白质和碳水化合物的代谢以及抗氧化反应;成虫消减文库的基因多参与蛋白质的合成、转运及分解代谢,参与虫体的运动等 . 大规模分离、分析血吸虫期别差异表达基因将对从分子水平去解读血吸虫的生长发育机制,筛选高效疫苗候选抗原、药物靶标及诊断制剂有重要意义 .     

消减杂交筛选2BS细胞衰老过程中差异表达基因

细胞的复制性衰老最终导致不可逆的G1 期阻滞 ,研究此过程中差异表达基因对于阐明衰老发生机制有重要意义 .分别构建年轻和衰老 2BS细胞高表达基因的消减文库 ,经点杂交筛选后共得5 3个差异表达基因 .对其中部分基因的VirtualNorthern印迹分析证实差异表达确实存在 .选择Y1 1 4和S1 1 1片段 ,以Northern印迹分析确证其表达变化 ;并通过对新生儿和老年人白细胞中二者的表达分析 ,显示二者在体内也存在与体外衰老过程相一致的随增龄表达变化 .结果在一定程度上体现了 2BS细胞衰老过程中基因表达谱的变化 ;首次报道了TSSC3(tumorsuppressingsubtransferablecandidate 3)、hnRNPK (heterogeneousnuclearribonucleoproteinK)等基因在成纤维细胞衰老时发生差异表达 ;通过对Y1 1 4和S1 1 1在体内衰老时的表达分析 ,显示体内和体外衰老有一定的相关性     

大菱鲆肌肉组织中的基因差异表达与体长性状的相关性研究

为了揭示出一些影响鱼类生长发育速度方面的遗传信息,本文应用mRNA差异显示技术,以同一批受精卵孵化的同池养殖的两组大菱鲆鱼为试验材料,检测了在相同生长发育条件下两组体长相差悬殊的3月龄大菱鲆肌肉组织的基因差异表达。结果：18对引物组合共显示出723条带,其中有527条带能够重现,差异显示条带的重现率为72.89%;在527条稳定的条带中有21条为差异带,其余506条为共有带（96.02%）。21条差异表达条带中有16条（3.04%）为阳性差异表达cDNA片段。这些差异表达cDNA片段的存在,说明体长差异悬殊的两组大菱鲆之间存在基因表达上的差异。试验结果对于进一步分析各种差异表达基因与大菱鲆的生长性状之间的相关关系奠定了基础;为深入研究大菱鲆的生长发育性状的分子遗传机制奠定了基础。     

差异显示法分离水稻抗稻瘟病相关基因

采用mRNA差异显示技术,分析水稻稻瘟病抗源材料“地谷”叶片受稻瘟病菌侵染前后的基因的表达差异,获得87个差异片段。对这87个差异片段进行了回收、重扩增与克隆,并对其中的81个片段进行了杂交鉴定。斑点杂交结果证实其中6个片段受稻瘟病菌诱导表达。进一步克隆测序并进行数据库比对分析表明其中一个与水稻4号染色体中一推测的苹果酸合成酶高度同源,一个与水稻11号染色体上的RPR1基因高度同源,RPR1基因具有保守的NBS-LRR结构,并与水稻防卫反应的信号传导有关;另一个与水稻第6号染色体上一推测的硫氧还蛋白高度同源,其余3个为新的cDNA片段。     

水稻愈伤组织形态发生中的MADS盒基因的差异表达

采用MADS(MCM1-Agamous-Deficiens-SRF)盒基因家族功能区保守序列PCR引物,将水稻(Oryzasativa L.ssp indica)“珍汕97B”悬浮细胞、愈伤组织、分化愈伤组织和再生试管苗等不同形态发生的组织的mRNA反转录后选择性放大,经测序胶分离鉴定出一组差异表达的cDNA。对命名为RM1 cDNA的5＇端序列测定表明,RM1与典型的MADS基因——拟南芥agamous蛋白保守区一级结构同源性达63％,模拟二级结构相似性显著,初步确认RM1属于MADS基因家族成员。分子杂交证实,RM1在悬浮培养细胞中不表达,而在愈伤组织、分化愈伤组织和再生试管苗中活跃表达。     

差异显示法分离赤霉素调控的水稻(Oryza sativa)cDNA(英文)

赤霉素(gibberellins)是植物生长发育过程中一类重要的调节激素。本文运用反转录和聚合酶链式反应建立了一套旨在分离差异表达cDNA的差异显示方法。以籼稻珍汕97 B为材料,将赤霉素GA_3处理后的苗期水稻与对照的cDNA片段进行比较,鉴定了15个差异cDNA,并将它们从测序胶中回收和再次扩增获得差异表达的cDNA;用其中一个差异cDNA片段DDF1为探针的Southern和northern杂交证实,DDF1所对应的基因是一个单拷贝基因,可被高浓度的GA_3诱导并获得高水平表达。     

Estrogen-dependent and cell-specific regulation of gene expression in RUCA-I endometrial adenocarcinoma cells

Estrogens are believed to play a crucial role in growth regulation and differentiation of the normal endometrial tissue as well as in the carcinogenesis of the endometrium. Therefore, the influence of estrogens and antiestrogens on gene expression in the estrogen receptor-positive rat endometrial adenocarcinoma cell line RUCA-I was investigated. Differentially expressed genes were detected by differential display PCR of RNA of untreated, estradiol-treated and antiestrogen-treated RUCA-I cells. By means of the PCR technique, 14 differentially expressed fragments could be detected. Three of these 14 differentially expressed fragments were confirmed by Northern blotting. The steady state mRNA levels of the three gene fragments named AH41, AH42 and AH44 were downregulated by the antiestrogen ICI 164384. Further characterization revealed that the fragment AH41 is not expressed in stromal cells but in the human and rodent epithelial cell lines, BG-1 and RUCA-II. A comparison of the cDNA sequence of fragment AH41 with the EMBL database showed no high homology to known genes. Therefore, fragment AH41 has to be regarded as a fragment of a novel, estradiol-sensitive gene.     

Screening and comparison of differentially expressed genes between one MDR-TB strain and the virulent M. tuberculosis H37Rv

To screen and compare the differentially expressed genes between one MDR-TB strain separated from one child patient and the virulent Mycobacterium tuberculosis H37Rv, suppression subtractive hybridization (SSH) technology was used to build a library of cDNAs that were differentially expressed in the MDR and H37Rv. From this cDNA library, genes that were expressed in the MDR-TB but not in the H37Rv were selected for gene sequencing and homology analysis; 113 positive clones were obtained, their cDNA fragments were sequenced, and homology analysis was performed. Four novel sequences were identified. The results provide a partial list of genes differentially expressed in MDR-TB and four novel genes were found. Identification of these genes may contribute to our understanding of MDR-TB development.     

A study on differentially expressed gene screening of Chrysanthemum plants under sound stress

Environmental stress can induce differential expression of genes of flower plants. It had been found that sound stimulation had an obvious effect on the growth and development of flower plants, but it is not reported on the differentially expressed genes and their expressing characteristics under sound stimulation. This is one of the few reports in terms of using the DDRT-PCR technique for screening the differentially expressed cDNA fragments responding to sound-wave stress on Chrysanthemum. Six differentially expressed cDNA fragments were obtained. Molecular weight of fragments was from 200 to 600 bp, respectively. Among differential fragments acquired, three of them (SA3, SG7-1, and CA2) were found to be positive fragments by northern dot hybridization, whose molecular weight are 270, 580 and 370 bp, respectively. SA3 was differentially expressed and SG7-1 was preferably expressed, while CA2 was restrained by the sound wave. These results indicated that expression of some genes was turned on, meanwhile the stress restrained some genes from expression under the mode of sound-stress stimulation.     

Systematic comparison of gene expression through analysis of cDNA fragments within or near to the protein-coding region.

Life is controlled by the timely and ordered expression of genes. Identification of important genes involved in specific physiological and pathological conditions requires efficient methods to analyse differential gene expression. We describe a novel strategy, namely complete comparison of gene expression (CCGE), for a systematic assessment of differentially expressed genes. Using the CCGE method, double-stranded cDNA is digested with two restriction enzymes that cut with different frequencies, the representative cDNA fragments are generated within or near to the protein-coding region. After being flanked by two different types of adapters, and amplified by a nested suppression PCR, the selected cDNA fragments, representing entire cDNA population, can be divided into 256 subsets; amplified and compared in a systematic manner.     

A novel strategy for identifying differential gene expression: An improved method of differential display analysis.

We propose a novel alternative approach, an advanced method for recently developed strategies, for identifying differentially expressed genes. Firstly, double-stranded cDNAs were digested using Sau3AI and the 3'-end restriction fragments of the cDNA were ligated to a double-stranded adapter. Next, the restriction fragments were directly amplified using several combinations of adapter-specific primers and FITC-labeled oligo dT primers. The selected cDNA fragments were displayed on a polyacrylamide gel. Neither nested PCR nor purification of 3'-end fragments are necessary. We examined the validity of this approach by evaluating gene expression changes during granulocytic differentiation of HL-60 cells. This method can theoretically detect almost all gene expression changes more rapidly and through simpler manipulations than by any other approach.     

宏基因组技术在开拓天然产物新资源中的应用

微生物代谢产物具有巨大的化学多样性,是多种抗生素和其它药物的重要来源。由于现有培养手段的局限性,可培养的微生物不到微生物总数的1％,使绝大部分微生物资源的开发利用受到制约。近年来．直接提取环境样品中混合微生物总基因组DNA,利用可培养的宿主细菌构建宏基因组文库,通过筛选目的克隆,寻找活性代谢产物,取得瞩目进展。对这一新领域的研究进展结合我们的研究概况进行了简要综述。     

利用cDNA-AFLP技术分析旱作促进水稻种子根伸长过程中的基因表达

短期旱作促进水稻种子根的伸长。利用cDNA—AFLP技术分析种子根根尖在旱作条件下差异表达的基因,同时比较这些基因在种子根尖、侧根和不定根原基区的表达差异。在1640个片段中,70个在种子根根尖中受旱作诱导,其中24个被克隆并测序。2个基因分别编码丙酮酸脱氢酶激酶(PDK)和腺嘌吟转磷酸核糖基酶(APRT),并用电子拼接技术获得水稻的APRT全长cDNA;另一个经cDNA末端快速扩增法延长后仍无同源序列。Northern杂交验证了这3个基因的cDNA—AFLP表达谱。这是首次报告使用cDNA—AFLP技术研究水稻根组织的差异表达基因。