Analysis and prediction of exon, intron, intergenic region and splice sites for A. thaliana and C. elegans genomes

Although a great deal of research has been undertaken in the area of the annotation of gene structure, predictive techniques are still not fully developed. In this paper, based on the characteristics of base composition of sequences and conservative of nucleotides at exon/intron splicing site, a least increment of diversity al-gorithm (LIDA) is developed for studying and predicting three kinds of coding exons, introns and intergenic regions. At first, by selecting the 64 trinucleotides composition and 120 position parameters of the four bases as informational parameters, coding exon, intron and intergenic sequence are predicted. The results show that overall predicted accuracies are 91.1% and 88.4%, respectively for A. thaliana and C. ele-gans genome. Subsequently, based on the po-sition frequencies of four kinds of bases in regions near intron/coding exon boundary, initia-tion and termination site of translation, 12 position parameters are selected as diversity source. And three kinds of the coding exons are predicted by use of the LIDA. The predicted successful rates are higher than 80%. These results can be used in sequence annotation.

人类基因组非冗余Exon/Intron数据库的构建

以Homo.sapiensRefSeq作为原始数据库来构建EID(Exon/Intron Database)可以克服GenBank所带来的冗余问题.通过分析RefSeq基因组数据库中每个CDS(Coding Sequence,编码序列),获得构建EID的相关的数据(基因的定义、基因标识符、基因序列、蛋白质标识符、蛋白质序列、外显子和内含子的数量、大小、总数、非翻译区(UTR)内含子、内含子相位、内含子剪切位点模式).结果表明,人类24条染色体(22条常染色体和2条性染色体,共计2 870 827355 bps)中含有32 157个基因标识符(gene blocks),其中7 398个基因为假基因,4 014个基因发生了可变剪切(Al-ternative Splicing,AS),15 533个基因含有CDS内含子,765个基因含有UTR内含子,2 585个基因不含有内含子,其他的为异常基因.

外显子周期三行为特征的研究

基因中蛋白质的编码区具有周期三行为这一规律已成为目前基因预测的理论基础,采用功率谱对外显子的周期三行为特征进行了研究,结果表明:大多数外显子独立存在于基因中时并不具有周期三行为,而当基因被剪切后外显子连在一起编码蛋白质的时候才具有周期三行为.并且这种行为特征与外显子的长度、碱基在密码子三个位置上的分布以及氨基酸密码子的使用偏好均有密切关系,同时符合蛋白质翻译次序的外显子也具有对密码子使用的偏好性,这一研究结果对于提高基因预测的准确率以及内含子功能的研究具有重要意义.

Associations of content and gene polymorphism of macrophage inhibitory factor-1 and chronic hepatitis C virus infection

BACKGROUND The expression of macrophage inhibitory factor-1(MIC-1) is increased in peripheral blood of patients with chronic hepatitis and liver cirrhosis. However, whether MIC-1 gene polymorphism is correlated with relevant diseases is not yet reported.AIM To explore the correlation between gene polymorphism in MIC-1 exon region and chronic hepatitis C virus(HCV) infection.METHODS This case-control study enrolled 178 patients with chronic hepatitis C(CHC) in the case group, and 82 healthy subjects from the same region who had passed the screening examination comprised the control group. The genotypes of rs1059369 and rs1059519 loci in the MIC-1 gene exon were detected by DNA sequencing. Also, the MIC-1 level, liver function metrics, liver fibrosis metrics, and HCV RNA load were determined. Univariate analysis was used to compare the differences and correlations between the two groups with respect to these parameters. Multivariate logistic regression was used to analyze the independent relevant factors of CHC.RESULTS The plasma MIC-1 level in the CHC group was higher than that in the control group(P < 0.05), and it was significantly positively correlated with alanine aminotransferase, aspartate aminotransferase(AST), type III procollagen N-terminal peptide(known as PIIINP), type IV collagen, and HCV RNA(P < 0.05), whereas negatively correlated with total protein and albumin(P < 0.05). The genotype and allele frequency distribution at the rs1059519 locus differed between the two groups(P < 0.05). The allele frequency maintained significant difference after Bonferroni correction(Pc < 0.05). Logistic multiple regression showed that AST, PIIINP, MIC-1, and genotype GG at the rs1059519 locus were independent relevant factors of CHC(P < 0.05). Linkage disequilibrium(LD) was found between rs1059369 and rs1059519 loci, and significant difference was detected in the distribution of haplotype A-C between the CHC and control groups(P < 0.05). Meanwhile, we found the MIC-1 level trend to increase among rs1059519 genotypes(P = 0.006) and the level of MIC-1 in GG genotype to be significantly higher than CC genotype(P = 0.009, after Bonferroni correction).CONCLUSION Plasma MIC-1 level was increased in CHC patients and correlated with liver cell damage, liver fibrosis metrics, and viral load. The polymorphism at the MIC-1 gene rs1059519 locus was correlated with HCV infection, and associated with the plasma MIC-1 level. G allele and GG genotype may be an important susceptible factor for CHC.

CREB3基因启动子区域的突变与肝癌的关系

目的 使用原发性肝癌患者肝癌组织、癌旁组织和正常人外周血 ,通过对环磷酸腺苷反应元件结合蛋白 3(c AMP responsive elem ent binding protein 3,CREB3)基因的单核苷酸多态 (single nucleotide polymorphism ,SNP)进行检测 ,研究 CREB3基因与原发性肝癌的相关性。方法 对 CREB3基因的启动子、外显子以及邻近的内含子区域 ,使用 PCR扩增和 DNA测序方法 ,分别在 2 4例原发性肝癌患者肝癌组织、癌旁组织及 96名正常人外周血进行测序 ,比较其可能存在的差异 ,确定该基因是否与原发性肝癌相关。结果 在正常人的外周血中只出现一个高频 SNP,位于 CREB3基因启动子区 ;该 SNP在肝癌患者癌组织中也呈高频性。在 2 4例肝癌患者的癌组织中 ,发现 CREB3基因启动子区有 6种新突变 ,突变位于基因起始密码上游 - 732～ - 70 2碱基的区域。这 6种突变分别在7例肝癌病人的癌组织中出现 (2 9.2 % ,7/ 2 4 ) ,2 4例癌旁组织中均没有这些突变 ,两组间差异有显著性 (χ2 =6 .0 2 ,0 .0 1<P<0 .0 2 5 )。 CREB3基因的外显子、邻近的内含子区域在肝癌患者癌组织、癌旁组织和正常人外周血均无SNP存在。结论 CREB3基因启动子的 - 732～ - 70

小尾寒羊MyoG外显子2和MyoD 5'侧翼区的多态性研究

采用PCR-SSCP技术分析了小尾寒羊肌细胞生成素Myo G基因外显子2和生肌决定基因Myo D 5'侧翼区的多态性,结果表明:Myo D 5'侧翼区在小尾寒羊中检测到2种基因型(BB、AB),BB和AB基因型频率分别为0.975 0和0.025 0,A和B等位基因频率分别为0.012 5和0.987 5;小尾寒羊的Myo G外显子2不存在多态性。对Myo D 5'侧翼区的BB基因型测序分析发现,其与牛的Myo D1基因序列(XM_592330.2)相比,发生了2处突变,分别是第960位发生了T→C突变、第972位发生了C→A突变。

日本血吸虫8k CaBP基因启动子区的克隆与分析

目的克隆日本血吸虫8kCaBP(Sj8CaBP)基因启动子区并对该序列进行分析。方法提取日本血吸虫基因组DNA,并按ClontechUniversalGenomeWalkerTMKit的操作手册说明,建立日本血吸虫基因组DNA文库。根据手册要求及Sj8CaBP基因的cDNA序列,设计合成该基因染色体步移的特异性引物与试剂盒提供的端子引物进行巢式PCR。将得到的PCR产物克隆测序,测序结果用启动子区的分析软件及与其cDNA序列比对进行分析。结果得到的Sj8CaBP基因长度为1079bp(GenBank登录号AY262018),该基因包含Sj8CaBP基因完整的开放阅读框(ORF),包括1个内含子及2个外显子,在其5'端UTR区具有明显的启动子区,包括TATA盒及CAAT盒,没有发现GC盒及一些血吸虫基因启动子区所常见的AP-1(Activeprotein1)结合位点。结论从日本血吸虫基因组文库中获得一个长1079bp的Sj8CaBP基因片段(GenBank登录号为AY262018),经分析证明,该片段包含一个启动子区,具有TATA盒及CAAT盒的结构及1个内含子2个外显子.

人类pax-5基因外显子1B的5′侧翼区碱基序列分析(英文)

pax 5基因是B细胞生成和B细胞发育中的重要转录因子。为了更好的理解 pax 5基因表达的调节机制 ,对 pax 5基因外显子 1B的 5′侧翼区进行了分离克隆及序列测定。整段碱基序列 (6 6 71bp)分析表明 ,无TATAbox共同序列存在 ,近侧启动子包括 3CATboxs,1SP1和 1Ebox ,上游进一步推测的调节位点显示 6LMO2 COM ,5NFAT ,2LPOLYA B ,3GATA1,2AP4 ,10MZF1,1ETS1 B ,1GATA3,1NKX2 5 ,2RORA1,1LYF1,2Ikaros2 ,2TCF11,1GATA C和 1FREAC7,并确定在序列上。因此 ,pax 5基因外显子 1B的 5′侧翼区与 pax 5表达的调节有关 。

RTN4基因外显子区拷贝数变异与鼻咽癌的相关性研究

目的探讨RTN4基因(54972187-55137831)外显子区9个目的片段拷贝数变异(copy number variant,CNV)与鼻咽癌的相关性研究。方法采用多重基因拷贝数检测技术(Accu Copy TM)对179例鼻咽癌样本和200例健康体检者样本进行RTN4基因外显子区9个目的片段拷贝数检测,观察两组样本基因拷贝数变异情况,运用数理统计比较两组拷贝数分布的差异性。结果鼻咽癌患者和健康体检者的RTN4基因外显子区的拷贝数主要以2个拷贝为主,经分析发现这两组的拷贝数比较差异无统计学意义(P均>0.05)。结论 RTN4基因(54972187-55137831)外显子区拷贝数变异可能与鼻咽癌发生发展无相关性。

非小细胞肺癌表皮生长因子受体基因突变274例分析

目的:研究非小细胞肺癌(NSCLC)患者表皮生长因子受体(EGFR)基因突变情况及其与临床指标的相关性,为NSCLC患者表皮生长因子受体酪氨酸激酶抑制剂(EGFR-TKI)的个体化给药提供参考。方法:选取2015年1月-2017年12月我院收治的苏北地区NSCLC患者274例,采用扩增阻滞突变系统与TaqMan探针相结合的方法检测其肺组织中EGFR基因的突变情况,回顾性分析突变情况与患者性别、年龄、吸烟状态、临床分期、肿瘤分化及病理类型等临床指标的相关性;同时与相关文献数据进行对比,分析EGFR基因突变的地区差异。结果:274例NSCLC患者中,发生EGFR基因突变的有112例,总突变率为40.88%;其中,外显子19、21、20、19+21突变的分别有50、57、3、2例,突变类型包括delE746-A750、L858R、insH773-V774H等。非吸烟、早期、高分化、腺癌患者EGFR基因外显子19、21的突变率分别为52.50%、47.24%、46.36%、45.00%,均分别显著高于吸烟(28.57%)、晚期(27.03%)、低分化(31.71%)、鳞癌(27.66%)患者(P<0.05);而男性与女性、≥65岁与<65岁患者EGFR基因外显子19、21的突变率比较,差异均无统计学意义(P>0.05)。苏北地区NSCLC患者EGFR基因的突变率显著高于上海地区(P<0.05),与云南地区无显著差异(P>0.05)但突变类型不同。结论:苏北地区NSCLC患者EGFR基因突变类型以外显子21突变最多,外显子19突变次之,外显子20突变和外显子19+21双突变少见,且存在明显的地区差异。EGFR基因外显子19、21的突变率与NSCLC患者的吸烟状态、临床分期、肿瘤分化及病理类型有关,非吸烟、早期、高分化、腺癌患者更可能在EGFR-TKI靶向治疗中获益。

Molecular cloning and analysis of the partial sequence of Rhinopithecus roxellanae growth hormone gene

Growth hormone gene (GH) ofRhinopithecus roxellanae was amplified by PCR based on the sequences of the reported mammalian growth hormone gene for the first time. The amplified fragment was about 1.8 kb. It was cloned and its upper stream was sequenced. This sequencing region consists of a 5′flanking regulatory region, exon I and part of exon II, intron I of growth hormone gene. Comparing the corresponding sequences of growth hormone gene betweenRhinopithecus roxellanae and the porcine, we concluded that the homology reached 81% in the region, and there was high conservation in the 5′flanking sequence. The kinds of amino acids of exon I and exon II for about 90% were the same to those in pig. Many mutations occurred in the degenerate site of the triplet code. In the nucleotides of intron I, there were only 72% homologies with those in pig. It means that introns and 3′flanking sequence maybe play an important part in growth hormone gene regulation of the different animals.

The Unexpected Existence of Coding and Non-Coding Fragments along the Eukaryotic Gene

The pathways leading to synthesis and post-synthetic modification of DNA employed methionine as donor of atoms: the carbon that came from its –CH3 served for DNA replication and repair either in bacteria or humans;its entire –CH3 served instead for building N6-methyladenine and 5-methylcytosine on bacterial DNA and 5-methylcytosine alone on human DNA. In humans, although a slight extra-S asymmetric methylation appeared de novo yielding on parental DNA 5’-m5CpC-3’/ 3’-GpG-5’, 5’-m5CpT-3’/3’-GpA-5’ and 5’-m5CpA-3’/3’-GpT-5’ monomethylated dinucleotide pairs, a heavy symmetric methylation involved in S semiconservatively newly made DNA to guarantee genetic maintenance of –CH3 in 5’-m5CpG-3’/3’-Gpm5C-5’ dimethylated dinucleotide pairs. In this framework, an inverse correlation was found between bulk genomic DNA methylation occurring in S and bulk polyA-containing pre-mRNA transcription taking place in G1 and G2. Thus, probes of 1 × 106 Daltons (constructed using sheared by sonication newly made methylated DNA filaments) revealed a modular organization in genes: after the hypermethylated promoter, they exhibited an alternation of unmethylated coding and methylated uncoding sequences. This encouraged the search for a language that genes regulated by methylation should have in common. An initial deciphering of restriction minimaps with hypomethylatable exons vs. hypermethylatable promoters and introns was improved when the bisulfite technique allowed a direct sequencing of m5C. In lymphocytes, where the transglutaminase gene is inactive, its promoter exhibited two fully methylated CpG-rich domains at 5’ and one fully unmethylated CpG-rich domain at 3’, including the site +1 and a 5’-UTR. At variance, in HUVEC cells, where the transglutaminase gene is active, in the first CpG-rich domain of promoter few doublets lost their –CH3. Such an inverse correlation suggested new hypotheses especially in connection with repair-modification: UV radiation would cause demethylation in given loci of a promoter by chance, whilst even a partial demethylation in this promoter would be able to resume a previously silent pre-mRNA transcription.

Preliminary study on the molecular structure of 3' region of Duchenne muscular dystrophy (DMD) gene in Chinese

Number and order of HindⅢ exon-containing fragments (Hd) at 3' region of DMD gene were studied systematically using 16 partly-overlapping cDNA subprobes which were produced from dystrophin cDNA 9- 14 with each of 9 restriction endonudeases. There are 25 Hd fragments corresponding to cDNA 9 -14 in DMD gene. Since then, the exact length and the new order of Hd fragments are established. A new 2.1 kb fragment (Hd 55) is revealed, a 5.2 kb fragment (formely designated as Hd 59) is excluded and the existence of a controversial 3.2 kb fragment (Hd 64) is confirmed. Besides, three new exons were revealed by comparing the PvuⅡ and the XbaⅠ hybridization patterns with the Hindlll hybridization patterns for these cDNA subprobes. It is concluded that there are at least 66 Hd fragments, or 79 exons in DMD gene basing on the discovery of three additional exons. The corresponding relationship between the 66 Hd fragments and the SfiⅠ large scale physical map has been studied, and at least 17 Hd fragments or 19 exons were shown to be distributed in the last fragment (LI fragment) of the SfiⅠ map of DMD gene.

Dravet综合征患者电压依赖性钠通道α1亚基基因5’-非翻译区外显子的遗传变异

目的筛查Dravet综合征患者的电压依赖性钠通道α1亚基（voltage—gated sodium channel α1—subunit，SCN1A）基因5’-非翻译区外显子突变位点，分析并预测其致病易患性。方法收集24例Dravet综合征患者的外周血，抽提基因组DNA，采用直接测序法进行SCN1A基因5’-非翻译区外显子突变位点的筛查；用生物信息学方法分析SCN1A基因5’-非翻译区外显子变异位点邻近序列的保守性及潜在的转录因子结合元件，推测其致病易患性。结果发现位于外显子h2u上的突变位点166．642．520G〉A，先证者1为新生突变，而先证者2的突变来自临床表型正常的母亲，该突变位点在100名健康对照者中均未发现。突变位点在哺乳动物中呈中度保守（62．5％），人与其他哺乳动物之间在突变位点邻近序列的平均同源率高达88．5％；166．642．520野生型位点的序列上预测得到一种转录因子结合元件，而突变型位点的序列上预测得到两种转录因子结合元件。结论突变位点166．642．520G〉A与Dravet综合征存在一定程度的相关性，其致病机制有待于进一步实验证实。

果蝇核糖体蛋白基因中潜在转录协同作用模体的统计分析

首先基于频率分析方法抽提出果蝇核糖体蛋白(RP)基因外显子上游直至第1个内含子结束的序列(称为启动子)中潜在的调控模体,这些模体中有85%与实验上的转录因子匹配.然后将抽提出的模体两两配对,运用超几何分布找出出现条数比例在RP基因中显著高于在背景启动子中的模体对,并进一步用K-S检验提取出它们在RP基因中的距离分布与背景距离分布有显著差异的模体对,这些模体对被认为具有转录协同作用.它们中的一部分与实验结果匹配.分析提取出的模体对在序列中的位置分布,发现它们主要的协同作用区域是上游区,而上游和内含子之间的协同作用也是一种重要的组合调控形式,同时发现模体对的模体间距离大部分位于300bp以内,并且在第一外显子附近较为集中.这些结果将有助于对RP基因转录调控机制的认识.