Metallothionein Genes in the Nematode Caenorhabditis elegans and Metal Inducibility in Mammalian Culture Cells

Genomic DNAs of metallothionein Ⅰ and Ⅱ in Caenorhabditis elegans (CeMT-Ⅰand CeMT-Ⅱ) were isolated by YAC library/polytene filter hybridization followed by subcloning of corresponding cosmid clones. Both genes are mapped at chromosome V. Although the similarities of 5'-flanking regions and coding regions have shown only 55-58%, the introns are split at the same position in both genes, indicating that these two genes are originally from the same gene. While several metal responsive elements are conserved among eukaryotes, only one metal responsive element was found in the promoter region in CeMT-Ⅱ and not in CeMT-Ⅰ. Indced, neither of 5'-flanking regions of CeMT-Ⅰ nor CeMT-Ⅱ connected to chloramphenicol acetyltransferase reporter gene is responsive to heavy metals in mammalian culture cells by transient transfection analysis. These results would suggest that the metal regulatory factors in C.elegans might be different from those conserved in invertebrates and vertebrates, although the MTs in C elegans revealed the similarities to mammalian MTs in several points

Bioinformatics analysis of metallothionein gene from <i>Agaricus bisporus, Ganoderma lucidum, Taiwanofungus camphorates</i>and <i>Paxillus involutus</i>

Metallothionein (MT) gene has an important role in the detoxification of toxic metals especially some heavy metals. Based on the published sequences of MT genes from Agaricus bisporus, Garnoderma lucidum, Taiwanofungus camphoratus and Paxillus involutus as a type of the edible or medical mushroom in NCBI database, their molecular structures, physiological functions and evolutionary relationship were analyzed using the bioinformatics methods. Results showed that AbMT, GlMT, TcMT and PiMT genes contained complete open reading frame (ORF) and their theoretical points of the last three encoding proteins were higher than 7.0. AbMT, GlMT, TcMT and PiMT were relatively rich in random coil and extended strand, but transmembrane helices and signal peptides were not found. 4 MTs were mainly localized in cell nucleus (over 60%) and their cellular functions might have some relation to central intermediary metabolism. Multiple sequence alignment indicated relatively high identity (more than 52%) and short genetic distances (lower than 0.900) among 4 MT nucleotide sequences. Abundant genetic diversity and strong codon bias were found based on the halotype diversity, average number of nucleotide differences, nucleotide diversity, effective number of codons, codon bias index and scaled chisquare. Simultaneously, we deduced that 4 MT genes during molecular evolution were under positive selection. The present study might provide basis for further investigation of MTs molecular mechanisms and genetic laws.

Regulation of metallothionein gene expression in response to benzo[a]pyrene exposure and bacterial challenge in marine cultured black porgy(Acanthopagrus schlegelii)

Metallothioneins(MTs) are normally considered to be sensitive indicators of heavy metal pollution, but it is less clear whether the MT gene can actively respond to other environmental stresses. In this study, an MT m RNA molecular sequence of 471 bp(full length) was identified in marine cultured black porgy(Acanthopagrus schlegelii), encoding 60 amino acids containing 20 cysteine residues. The MT sequence was highly homologous to that of other fish belonging to the MT superfamily type 1 family. The three dimensional structure of the deduced MT peptide was composed of two metal-binding domains capable of ligating divalent heavy metals. The MT m RNA transcripts were detected in the 11 tested tissues and the highest quantity was present in the liver. Stresses by two factors, benzo[a]pyrene(B[a]p) exposure and bacterial challenge, were evaluated on MT gene expression. The level of MT gene transcripts in the liver significantly declined 24 h post B[a]p exposure and the quantity was significantly correlated with the exposure time during a 24 h period. In contrast, MT gene expression in the liver was significantly increased 48 h post bacterial infection and the quantity was significantly correlated with the infection time during this period of 48 h. Our results indicated that MT gene expression in black porgy liver was sensitive to environmental stresses other than just the heavy metal pollution reported, suggesting that the development of a reliable biomarker for heavy metal pollution will be more complex than expected.

Expression patterns of the rice class I metallothionein gene family in response to lead stress in rice seedlings and functional complementation of its members in lead-sensitive yeast cells

Metallothioneins (MTs) are a group of low molecular mass and cysteine-rich proteins that can chelate heavy-metal ions. In this paper,Northern blot analysis was used to investigate the influence of lead stress on the expression patterns of 10 rice class I MT genes (OsMT-Is) in rice seedlings. With the ex-ception of OsMT-I-3b,the data demonstrate dynamic changes of 9 OsMT-I transcripts in response to Pb2+ treatment in rice seedling roots. Of these genes,transcription of OsMT-I-1a,OsMT-I-1b,OsMT-I-2c,OsMT-I-4a,OsMT-I-4b and OsMT-I-4c increased significantly,while transcription of OsMT-I-2a and OsMT-I-3a increased marginally. In contrast,the expression of OsMT-I-2b was inhibited. Pb2+ induced the expression of 6 OsMT-I genes in seedling shoots,but had no obvious effects on the expression of OsMT-I-1a,OsMT-I-1b,OsMT-I-4a and OsMT-I-4b. All the 10 OsMT-Is had enhanced lead tolerance when heterologously expressed in lead-sensitive yeast mutant cells. These results provide an expression profile of the rice MT gene family in response to Pb2+ stress in rice seedlings and demonstrate in-creased lead tolerance in sensitive yeast mutant cells expressing OsMT-Is. This study lays a foundation for further analysis of the role of the rice MT gene family in respond to Pb2+ stress.

Metallothionein 1 Isoform Gene Expression Induced by Cadmium in Human Peripheral Blood Lymphocytes

Objective To study the gene expression of metallothionein 1 （MT-1） isoforms in human peripheral blood lymphocytes （HPBLs）. Methods The expression of mRNA representing the seven active MT-I genes was determined in HPBLs by quantitative RT-PCR before and after exposure to cadmium. Results Basal expressions of MT-IX, and MT-1A in HPBLs were similar to expression of housekeeping gene. In contrast, the basal gene expressions of MT- 1 H, IF, 1E, and 1G were a little transcripts in human HPBLs. No signal was detected for MT-1B. There was a sex difference （P〈0.05）. in basal gene expression of MT-1E. The levels of gene expression of MT-1A, 1E, IF, 1G, 1H, and 1X increased, but the level of MT-1B did not increase after exposure to cadmium. Conclusions Gene expressions of MT-1 G, MT-1 H, MT-1 F, and MT-1X in HPBLs can be used as a potential biomarker of cadmium exposure.

CLONING AND ORGANIZATION OF BOVINE METALLOTHIONEIN GENES

I. INTRODUCTIONMetallothioneins(MT) are ubiquitously distributed in animal and plant kingdoms. They are cysteine-rich proteins that specifically bind heavy metal ions, such as cadmium, zinc, mercury and copper. The high expression of the MT gene could be induced by heavy metals in vitro and in vivo. The first transgenic mice obtained by Palmiter et al. in 1982 were introduced with an exogenous growth hormnoe gene

Nucleotide Sequence and Characterization of Bovine Metallothionein Gene

1 Introduction Metallothioneins (MTs) are a family of low-molecular weight heavy metal binding proteins, unique in their high cystein content. MTs are ubiquitously distributed in the eukaryote from yeast to human. It is an experimental model emphasized during researching gene expression and regulation of animal cells. In order to provide inducible regulatory elements for transgenosis livestock, we cloned bovine MT genes. At least four members of bovine MT family have been discovered. In this note, one gene (bMTc) of

Evolutionary Mode of Metallothioneins Inferred from Cd-MT Genes of Tetrahymena

From Tetrahymena thermophila （strain BF5）, the coding region of Cd-MT gene was cloned and sequenced. and identified as MTT1 isoform. A serial duplicate structure is discovered in its amino acid sequence, which separates the coding region into three parts （Part 1：7-61; Part 2：64-118; Part 3：122-162）. The alignments among them and comparison with the corresponding parts of MT1 isoform suggest that MT1 and MTT1 isoforms both come from the same ancient gene that is homologous to Part 1, and Cd-MTs of Tetrahymena are aroused by such ancient gene duplication. The prediction of secondary structures and the analysis of the disulfide-bonding state of cysteine show that there are a lot of differences between MT1 and MTT1 isoforms, which maybe relate to their function mechanism.

过量表达分泌型MT3对植物镉富集的影响

金属硫蛋白(metallothionein,MT)MT3是人体中参与重金属解毒的主要蛋白,前期研究表明啤酒酵母(Saccharomyces c erevisiae)α因子信号肽(MF-α)介导重组蛋白EGFP分泌到植物体外。但是目前还没有研究报道转基因植物中过量表达分泌型MT3对植物重金属镉(Cd)的富集能力是否有影响。本研究通过人工方法合成MF-α信号肽、增强型绿色荧光蛋白(enhanced green fluorescent protein,EGFP)和MT3的融合基因MF-α-EGFP-MT3,构建该融合基因的植物表达载体pK-35S-MF-α-EGFP-MT3,转化野生型(WT)烟草和天竺葵获得转基因植物。通过电化学方法检测转基因植物MT3转录水平、转基因植物根系分泌液中EGFP-MT3蛋白的水平。用Cd溶液处理转基因植物,通过表型观察和电化学方法检测根、茎和叶中Cd的含量。结果表明,转基因烟草和天竺葵中都有MT3基因的转录;且根系分泌EGFP-MT3蛋白的量大约为0.45~0.68 mg·g-1(以鲜质量计)。100μmol·L-1的Cd溶液处理转基因烟草植株,表型变化分析发现转基因植株受损情况低于WT,近根部叶片叶绿素含量显著高于WT,说明EGFP-MT3的分泌可降低Cd的毒害作用。转基因烟草植株根、茎和叶片对Cd的富集量比WT高约40%。用50μmol·L-1的Cd溶液处理转基因天竺葵植株,结果表明转基因植株根对Cd的富集量比WT高约30%,茎对Cd的富集量比WT高约4倍。以上结果证明过量表达EGFP-MT3可以提高转基因烟草和天竺葵对Cd的富集能力,可能是EGFP-MT3分泌根系表面增加转基因植物根系对Cd的吸附作用,同时在转基因植物组织细胞内积累的EGFP-MT3也可增加植物组织对Cd的富集作用。

Generation and analysis of expressed sequence tags from the salt-tolerant eelgrass species, Zostera marina

Zostera marina, a monocotyledonous angiosperm, is one of the most important seagrass species. To inves- tigate the salt-tolerance mechanism and discover salt-tolerant genes in Z. marina, a cDNA library was con- structed. Single-pass sequencing of the 5＇ ends of 4 081 clones yielded 4 002 high quality expressed sequence tags （ESTs）, which were assembled into 241 contigs and 1 673 singletons, representing 1 914 unigenes. The average length of the ESTs was 582 bp, with sizes ranging from 100-1 500 bp. Basic Local Alignment Search Tool （BLASTX） analysis revealed that 1 664 unigenes had significant homology to known genes in the Na- tional Center for Biotechnology Information （NCBI） non-redundant （nr） database （E-value≤5-10）. Among them, the two most abundant genes encoded metallothionein （157 ESTs） and chlorophyll a/b-binding pro- tein （38 ESTs）, accounting for 7.1% and 1.7% of the total ESTs, respectively. Using Kyoto Encyclopedia of Genes and Genomes （KEGG）, 1 462 unigenes were assigned to 1 161 pathways （E-value≤5-10）. A total of 938 unigenes were assigned Gene Ontology （GO） terms based on the GO hierarchy analysis, and InterProScan searches recognized 1 003 InterPro families. Three genes for metallothionein in Z. marina that belonged to Class II was identified. Results of this study will improve understanding of the molecular mechanisms of saline tolerance in Z. marina.

Metallothionein:An overview

Metallothioneins (MTs) were discovered in 1957 by Margoshes and Vallee and identified as low-molecular weight and sulphydryl rich proteins. It is not surprising that most mammalian tissues contain age related basal levels of MTs since they are involved in metalloregulatory processes that include cell growth and multiplication. In an effort to understand the biology of this intriguing tumor, various biomarkers such as oncogenes, p53 tumor suppressor gene, waf 1 protein, proliferating cell nuclear antigen, telomerase, microsatellite markers and cytogenetic changes have been examined. One biomarker which has recently shown to be expressed in various human tumors but still less reported in carcinoma is MT. Immunohistochemical detection of MT proteins in cold acetone-fixed paraffin embedded liver sections was performed by the streptavidin-avidin-biotin immuno- peroxidase complex method.

基于GEO数据库筛选滤泡性甲状腺癌关键基因及生物信息学分析

目的 滤泡性甲状腺癌(follicular thyroid carcinoma,FTC)临床上较少见,其在疾病早期即可发生血行转移。本研究利用生物信息学方法探索FTC发生发展的关键基因、发掘FTC的致病机制及治疗靶点。方法 从基因表达综合数据库(gene expression omnibus,GEO)下载基因芯片GSE82208,利用R软件分析以获得差异表达基因(differentially expressed genes,DEGs),利用数据库注释、可视化和综合发现(database for annotation,visualization and integrated discovery,DAVID)在线网站对DEGs进行基因本体论(gene ontology,GO)功能分析和京都基因与基因组百科全书(Kyoto Encyclopedia of Genes and Genomes,KEGG)富集分析。对DEGs行蛋白质–蛋白质相互作用(protein-protein interaction,PPI)分析,并筛选核心基因,对核心基因进行生存分析。结果 共筛选获得74个DEGs,其中表达上调基因61个,表达下调基因13个。GO富集在细胞对锌离子的反应、细胞对镉离子反应、细胞核及金属离子结合等过程。KEGG信号通路富集在矿物质吸收信号通路。通过对PPI网络分析,筛选出核心差异表达基因MT1E、MT1F、MT1G、MT1H、MT1M、MT1X和MT2A共7个金属硫蛋白基因。生存分析发现MT1F和MT1M与甲状腺癌患者预后相关(P<0.05)。结论 金属硫蛋白介导的金属离子代谢紊乱与FTC密切相关,有望成为FTC的诊治靶点。

海湾扇贝(Argopecten irradians)金属硫蛋白基因的克隆与分析

金属硫蛋白是一种普遍存在于生物体内的低分子量、半胱氨酸含量丰富、易于被外界刺激诱导的金属结合蛋白。采用表达序列标签法,结合cDNA末端快速扩增技术,首次获得了海湾扇贝金属硫蛋白(AiMT)的全长cDNA序列。该序列全长787bp,5′UTR(UntranslatedRegion)为79bp,3′UTR为270bp,开放阅读框(OpenReadingFrame,ORF)长度为438bp,可编码145个氨基酸。在其编码的氨基酸序列中半胱氨酸含量丰富,甘氨酸含量也较高,芳香族氨基酸含量低,不含组氨酸,存在有无脊椎动物和软体动物金属硫蛋白的特征序列CKCXXX-CXCX,C-末端的氨基酸序列也符合软体动物金属硫蛋白标签序列C-x-C-x(3)-C-T-G-x(3)-C-x-C-x(3)-C-x-C-K。序列特征分析表明,该序列具备金属硫蛋白的典型特征,是金属硫蛋白家族的成员。

铜、锌离子影响丹参金属硫蛋白MT2基因表达

植物金属硫蛋白在金属离子的储存、运输和代谢及降低重金属离子的毒性等方面起着重要作用。本文研究了Cu2+、Zn2+对丹参毛状根中金属硫蛋白基因表达的影响。以6,7-V为液体培养基,分别以缺乏、正常及原培养基100、500、1000倍的Cu2+、Zn2+处理,采用半定量PCR法检测不同时间点时金属硫蛋基因的表达情况。结果发现Cu2+、Zn2+诱导金属硫蛋基因的表达量分别在100倍处理量时的9h和6d达到峰值。Cu2+、Zn2+能显著诱导丹参金属硫蛋白基因的表达,该基因可能在丹参对铜、锌元素的吸收方面发挥着重要的作用。

镉和铜对嗜热四膜虫金属硫蛋白基因的诱导表达

本文在荧光定量PCR优化的基础上,利用该技术考察了不同浓度的重金属镉和铜对嗜热四膜虫金属硫蛋白基因(MTT1)诱导表达的变化规律。结果表明MTT1基因的表达对镉离子的诱导更灵敏,且在一定阈值浓度(≤35.2μmol/L)范围内,镉离子浓度升高会增加MTT1基因表达量,超过该阈值后表达量迅速下降;镉与铜同时诱导时MTT1基因的表达情况与镉单独诱导的类似,但阈值浓度减小为22μmol/L,表明二者的联合毒性为协同作用。镉离子浓度低于22μmol/L时,与铜离子的共同作用会大大增加MTT1基因的表达量,从而增强了四膜虫的解毒能力。

斧文蛤金属硫蛋白基因的克隆与表达分析

金属硫蛋白(Metallothionein,MT)是一类富含半胱氨酸的小分子蛋白质,参与机体重金属解毒、维持金属元素代谢平衡以及清除自由基等生理功能。为了解斧文蛤金属硫蛋白(Ml-MT)的分子生物学特征及其在重金属Cd^(2+)胁迫下的响应机制,本文采用RACE技术从斧文蛤(Meretrix lamarckii)总RNA反转录产物中获得了636 bp的Ml-MT c DNA基因序列。该序列包含65 bp的5′非编码区(UTR)和340 bp的3′非编码区(UTR)以及231 bp的开放阅读框(ORF),可编码76个氨基酸;其中半胱氨酸占27%,不含芳香族氨基酸,含16个MT所特有的Cys-Xn-Cys结构,预测的分子量约为7.704 k D,理论等电点7.138。MT氨基酸序列比对分析表明:斧文蛤金属硫蛋白(Ml-MT)与丽文蛤(Meretrix lusoria)的相似性高达88%,与文蛤(Meretrix meretrix)的同源性为87%。实时荧光定量(q RT-PCR)检测MT在斧文蛤5种组织中均有表达,但存在组织特异性,其中内脏团表达量最高,其次依次为鳃丝、闭壳肌、外套膜、斧足。在Cd^(2+)(0.13 mg/L)胁迫0、6h、12h、24h、48h、72h和96h下,斧文蛤内脏团MT呈现出不同程度的上调表达,具体表现为"高-低-高-低"的波浪式变化,除6h以外,其他时间点均与对照组存在极显著差异(P<0.01)。本研究表明:MT基因在维护机体正常生理功能及斧文蛤抵御重金属Cd^(2+)胁迫过程中发挥着重要的分子调控作用。

金属硫蛋白基因在长期水砷暴露小鼠肝组织中的表达

目的探讨金属硫蛋白(MT)-1、2在慢性水砷暴露小鼠肝损伤中的作用。方法将健康清洁级雄性昆明种小鼠随机分成对照组和暴露组,对照组给予普通饲料和自来水(可自由饮用);暴露组给予普通饲料和300mg/L的亚砷酸钠溶液(可自由饮用)。在暴露前,采用150mg/L亚砷酸钠溶液以自由饮用的方式喂养暴露组小鼠,17周后小鼠未出现死亡。染毒10个月后,检测小鼠血清中谷丙转氨酶(ALT)、谷草转氨酶(AST)的活力和球蛋白(Glb)的含量。采用TRIzol-酚-氯仿一步法提取总RNA,采用紫外分光光度法测定RNA在波长为260和280nm时的吸光度值(A260、A280),以A260/A280鉴定RNA的纯度。以实时荧光定量PCR(RT-PCT)技术测定小鼠肝组织中MT-1和MT-2mRNA。并进行肝组织病理学观察。结果对照组小鼠状态良好,毛发光泽;暴露组小鼠毛发粗糙,精神萎靡,动作迟钝,易激惹,进食、进水量明显减少。对照组小鼠体重为(39.10±3.48)g,高于暴露组[(14.00±1.49)g],差异有统计学意义(P<0.05)。与对照组比较,暴露组小鼠血清中ALT、AST的活力和Glb含量较高,肝组织中MT-1和MT-2mRNA的含量较低,差异均有统计学意义(P<0.05)。肝脏病理检查结果可见,对照组肝组织正常;暴露组肝细胞水样变性,脂肪样变性,气球样变性,肝细胞点状、灶状、碎片状坏死,汇管区可见炎细胞浸润,少许纤维增生。结论MT表达的降低可能是亚砷酸钠肝毒性的一个易感因素。

金属硫蛋白-1与p53基因在燃煤型砷中毒患者口腔黏膜脱落细胞中的表达

目的观察金属硫蛋白-1(MT-1)、p53基因、雌激素受体(ERa)基因和甲胎蛋白(AFP)基因在燃煤型砷中毒患者口腔黏膜脱落细胞中的表达。方法收集贵州省兴仁县燃煤型砷中毒患者及非病区正常人口腔黏膜脱落细胞,提取mRNA,以荧光实时定量PCR(RT-PCR)方法检测与肝硬化及皮肤癌相关的MT-1及p53基因等表达。结果燃煤型砷中毒患者口腔黏膜脱落细胞MT-1基因表达与对照组比较明显减少(0.83±0.15、3.86±0.37),抑癌基因p53明显增加(4.35±2.79、0.90±0.58),ERa基因和AFP基因无变化。结论砷中毒患者口腔黏膜MT-1基因表达减少,抑癌基因p53表达增加,可作为燃煤型砷中毒患者皮肤及肝脏病变监测的敏感指标之一,RT-PCR技术可广泛用于砷中毒的防治、监测和科研。

金属硫蛋白和植物螯合肽在植物重金属耐性中的作用

植物螯合肽和金属硫蛋白广泛存在于植物界中 ,它们对植物耐重金属特别重要 ,能够与重金属形成复合物 ,以缓解重金属对植物的危害。本文就这两种金属螯合蛋白的结构、生物合成和基因调控 。

柽柳金属硫蛋白基因的克隆及序列分析

用木麻黄(Casuarina glauca)的金属硫蛋白基因(metallothionein 1)氨基酸序列对柽柳ESTs序列本地数据库进行tBlastn检索,获得了柽柳金属硫蛋白基因全长cDNA序列,去除polyA后该基因全长366 bp,其中5′非翻译区97 bp,3′非翻译区59 bp,开放读码框(ORF)长210 bp,编码70个氨基酸组成的多肽,蛋白分子量为6.793 kD,理论等电点为4.99,含10个Cys,集中分布在肽链的N端和C端。Blast P同源性分析表明该基因与花生同源性最高,与小豆同源性最低。该基因的EST序列在GenBank登录(登录号:CV792539)。