植物Nramp基因及其与金属离子转运的关系

概述了植物Nramp基因家族及其序列结构分析;在金属离子转运方面的作用机制;表达调控及亚细胞定位;与植物乙烯信号转导途径的核心组分EIN2基因之间的关系等;对今后的研究重点和应用也做了展望。     

杆状病毒lef基因家族及其功能

病毒基因结构与功能和表达调控的研究是分子生物学领域的热点之一。其核心内容是揭示病毒基因组的复制机理以及早期基因对晚期基因的调控机制。昆虫杆状病毒基因的表达是级联式调控,按其表达的时序可分为极早期基因、早期基因、晚期基因和极晚期基因。早期基因主要为病毒基因组DNA复制、晚期基因的表达提供必需的蛋白因子。     

MADS-box 基因家族基因重复及其功能的多样性

基因的重复(duplication)及其功能的多样性(diversification)为生物体新的形态进化提供了原材料。MADS-box基因在植物(特别是被子植物)的进化过程中发生了大规模的基因重复事件而形成一个多基因家族。MADS-box基因家族的不同成员在植物生长发育过程中起着非常重要的作用, 在调控开花时间、决定花分生组织和花器官特征以及调控根、叶、胚珠及果实的发育中起着广泛的作用。探讨MADS-box基因家族的进化历史有助于深入了解基因重复及随后其功能分化的过程和机制。本文综述了MADS-box基因家族基因重复及其功能分化式样的研究进展。     

微生物基因组序列测量及其重大意义

微生物基因组测序不仅可使人们更好地了解病原微生物的致病机制以及它们与宿主的相互关系,促进寻找更灵敏及特异的病毒原微生物的诊断,分型手段,而且为临床筛选有效的药物及发展疫苗提供参考,此外,它还能提高对人类相关基因功能的认识,为探讨人类遗传性疾病机制提供参考,本文就微生物序列测定重大的理论及应用价值作一简要概述。     

城市绿地微生物及其对城市化的响应

城市绿地微生物的稳定性是城市绿地发挥其重要生态系统功能的重要因素。人类世时代的快速城市化会改变城市绿地土壤理化性质、输入新兴污染物、加剧微生物生态系统潜在风险、改变微生物群落多样性及生态系统功能多样性,深远地影响了城市绿地的生态系统服务功能。本文综述了城市绿地微生物的特征,以及城市化进程对城市绿地微生物组(包括土壤、植物叶际和空气)、抗生素抗性基因、病原微生物和稀有物种群落的影响。与自然微生物相比,城市绿地微生物普遍具有较高的异质性,受人类活动影响大。同时,抗生素抗性基因水平以及人类致病菌数量则显著增加,体现了城市化对城市绿地生态系统健康和功能的扰动。今后研究中应更加关注城市化对于城市绿地微生物的影响,为其对人群健康影响风险评价提供可靠理论支持。     

福氏志贺菌ipaB基因的克隆及其在酵母细胞中的表达

志贺氏菌引起的细菌性痢疾为一种全球性的肠道传染病。据估计,全世界每年感染的人数超过两亿,由该病引起的死亡人数有65万左右[1]。该菌的致病性是由体内含有230kb的毒性大质粒决定的,而大质粒上一个31kb的片段所编码的侵袭质粒抗原(IInvasion plasmid antigen,Ipa)是致病所必需的[2,3]。近年来,国内外有关学者在原核生物中对ipaB基因克隆及功能进行了较广泛的研究[4,5],但在酵母细胞中这方面的研究未见报导。从志贺痢疾杆菌中克隆了ipaB基因,并在酵母细胞中得到了融合表达,为将IpaB应用于双杂交系统研究其在侵袭过程中的分子机制打下了基础。     

葡萄BRX基因家族生物信息学分析

BRX基因家族是一类植物特有的转录因子家族,在拟南芥中参与调节根细胞的增殖与伸长。利用生物信息学方法对葡萄基因组中存在的BRX基因家族进行了电子克隆,并对其进行了基因组的定位、蛋白质的结构、理化性质、二级结构及亚细胞定位的预测与分析,并对其与其它植物进化的亲缘关系进行了研究。基因组定位结果发现:葡萄基因组中6个BRX基因集中分布在3条染色体上,其中Vv BRX1和Vv BRX2分布在第2条染色体上,Vv BRX3和Vv BRX4分布在第9条染色体上,Vv BRX5和Vv BRX6分布在第11条染色体上;编码蛋白的氨基酸数目为360~560个,Vv BRX5的相对分子量(61 884.4)和理论等电点(9.38)均最大,而Vv BRX1的相对分子量(40 239.1)和理论等电点(6.23)均最小。研究显示,不同成员间氨基酸数目、氨基酸序列间存在一定的差异,但都为疏水性蛋白;α-螺旋和无规则卷曲为6个BRX氨基酸序列的主要组成部分;均不存在跨膜域及信号肽。基因结构分析表明,6个BRX基因都含有外显子和内含子结构。亚细胞定位分析表明:6个Vv BRX基因均定位于细胞核。系统进化分析结果表明,Vv BRX1、Vv BRX2基因与胡杨的亲缘关系最近,相似性达96%;Vv BRX3、Vv BRX4与蓖麻、麻疯树、柑橘、可可、大豆聚为一类,说明其进化关系较近;Vv BRX5与其它Vv BRX基因明显分开;Vv BRX6基因与莲的亲缘关系最近。试验结果为葡萄BRX基因家族的克隆和功能分析奠定了一定的研究基础。     

猪链球菌2型mrp基因免疫功能片段的克隆、表达及动物试验

根据猪链球菌2型（Streptococcus suis type 2）国外分离株的溶菌酶释放蛋白（Muramidasereleased protein, MRP）的基因序列,设计并合成一对引物,利用PCR技术扩增了江苏分离株的开放阅读框298～827bp间529bp的基因片段,并定向克隆至pET32a(+)表达载体中。重组质粒经限制性酶切鉴定和测序,转化至大肠杆菌BL21,经IPTG诱导,可表达分子量约42kD的蛋白。经过镍亲和层析柱层析,获得纯化的重组蛋白。以重组蛋白免疫Balb/c小鼠,以5LD50猪链球菌强毒株攻击后小鼠的相对存活率达625%。证实所表达的MRP片段为重要的保护性抗原。     

实验动物的微生物质量标准及其在生物医学科研工作中的意义

实验动物在通常条件下生活在微生物的环境中,当动物从母体的无菌的子宫中产出后,立即被周围的微生物所污染。其中有的微生物能从体内排除,而有的则能长期栖居在动物体内,构成共生或寄生的生物学状态。动物的胃肠道内居留着亿万细菌。这些细菌对宿主的生理代谢,组织形态,对疾病的抵抗力,对药物的效应,对致癌物的相互作用等等,都产生重大影响,因此严重干扰动物实验的结果,所以必须把动物体内外的微生物调查清楚,并研究排除和控制这些微生物是极为重要的工作.     

水稻锌铁转运蛋白ZIP基因家族研究进展

锌(zinc, Zn)和铁(iron, Fe)是水稻(Oryza sativa L.)生长必需的矿质元素,也是人体必需的微量元素。水稻体内Zn、Fe含量维持在适宜水平有利于提高其产量和品质,提高稻米中Zn、Fe含量能够在一定程度上解决人体Zn、Fe营养缺乏的问题。因此,研究水稻中Zn和Fe等微量元素转运蛋白的具体功能对于提高水稻产量和稻米品质具有重要意义。锌铁转运蛋白(zinc-regulated transporters and iron-regulated transporter-like protein, ZIP)负责Zn和Fe等离子的吸收、转运和分配,是维持水稻中Zn和Fe平衡的重要转运蛋白,其表达水平受Zn和Fe水平影响。ZIP基因家族在自然群体中具有丰富的等位变异,而且某些单倍型存在明显的籼粳分化,这可能造成了不同品种间籼、粳稻中Zn和Fe积累的差异。目前,已有大量关于ZIP基因家族的研究,但只有OsZIP3的作用机制研究的较为清楚。另外,对Zn、Fe在籽粒中的积累机制研究和自然群体中ZIP基因的等位变异研究还不够深入。因此,ZIP转运蛋白家族仍存在较大的研究空间。本文详细介绍了ZIP转运蛋白在水稻体内的亚细胞定位、表达模式、转运机制以及在自然群体中的等位变异等,以期为研究水稻稻米微量元素的积累提供理论基础,为提高稻米品质提供借鉴。     

Patterns of Gene Duplication and Their Contribution to Expansion of Gene Families in Grapevine

Grapevine is an important fruit crop that has undergone a long history of evolution. Analysis of the whole genome sequence of grapevine has revealed presence of an early palaeo-hexaploid along with three complements. Thus, gene duplication and genome expansion are common in this genome. In this study, we identified 17,922 duplicated genes in the whole grapevine genome. Among these, 2,039; 628; 1,428; 722; and 2,942 were identified respectively as produced by genome-wide, tandem, proximal, retrotransposed, and DNA-based transposed duplications. Analyses of the evolutionary patterns for different types of duplication using non-synonymous and synonymous substitution rates uncovered a series of underlying rules. Thereafter, all the grapevine genes were classified into families, and the contributions of different types of duplication to the expansion of large families were revealed. No duplication type was solely responsible for the formation of any large gene family, but some families showed enrichment of a special type of duplication. On the basis of this study, we believe that uncovering the underlying rules for gene duplications, expansions of gene families, and their evolutionary styles will contribute significantly to a comprehensive understanding of the features of the grapevine genome.     

基于转录组测序的慈竹笋木质素基因筛选及其表达分析

慈竹（Bambusa emeiensis）纤维素含量丰富,是较好的造纸原料,但竹茎中木质素影响着制浆生产及纸浆质量。目前,对慈竹木质素生物合成机制所知甚少,这限制了遗传调控竹木质素的研究。本文以拟南芥、水稻等植物的已知木质素基因作为查询序列,通过BLASTp和系统进化分析,从10、50、100和150 cm慈竹笋转录组数据中筛选到351个木质素生物合成相关Unigenes,包括51个LAC,37个4CL、26个PAL、34个CCR和25个CAD相关转录子,其数量高于其他已报道的竹类植物。转录丰度和定量基因表达分析发现16个木质素基因,包括2个PAL、5个CCR、3个4CL、2个CADH2和4个LAC,随着笋发育而表达上调,表明其可能与发育性木质素积累相关。     

苹果中磷酸蔗糖合酶家族基因的表达特性及其与蔗糖含量的关系

磷酸蔗糖合酶(sucrose phosphate synthase,SPS)是植物中蔗糖合成的主要限速酶,影响植物的生长发育和果实中蔗糖的含量。为探明苹果中SPS基因家族特性及其在蔗糖合成中的作用,该研究从苹果基因组中分离了MdSPS家族基因,分析了它们的进化关系以及mRNA表达特性与酶活性和蔗糖含量的关系。结果显示:(1)在苹果基因组中有8个SPS家族基因表达,它们分别属于双子叶植物的3个SPS亚家族。(2)荧光定量PCR分析显示,苹果C类的MdSPS6基因和A类的MdSPS1a/b基因是苹果中表达丰度最高的SPS基因成员,其中MdSPS6在苹果成熟果中表达丰度最高,其次是成熟叶片,而MdSPS1a/b在不积累蔗糖的幼果中表达丰度最高。(3)在果实发育过程中,除MdSPS1a/b之外,其它5个苹果MdSPS家族基因均随果实的生长表达丰度增加,与SPS活性和蔗糖含量明显呈正相关关系。研究表明,C类家族MdSPS6是苹果果实发育后期和叶片中蔗糖合成的主要SPS基因。     

Role of MAP kinase activation in Nramp1 mRNA stability in RAW264.7 macrophages expressing Nramp1(Gly169)

Nramp1 (natural resistance-associated macrophage protein 1) is a phagosomal iron transport molecule. In addition to its anti-microbial activity, Nramp1 exerts a wide range of pleiotropic effects, including increased stability of Nramp1 mRNA and a variety of other mRNA species. Previously, we showed that the increased stability of Nramp1 mRNA is regulated by an oxidant-generated signaling pathway that requires PKC. In the current study, we show that inhibition of ERK1,2 and p38 MAP kinase activities decreases Nramp1 mRNA stability in Mycobacterium avium infected RAW264.7 cells expressing Nramp1(Gly169) but not in RAW264.7-Nramp1(Asp169) cells. Phosphorylation of ERK1,2 and p38 MAP kinases, which could be inhibited by the anti-oxidant BHA and a protein kinase C inhibitor, was higher in M. avium infected RAW264.7-Nramp1(Gly169) cells than in RAW26.47-Nramp1(Asp169) cells. These results suggest that generation of oxidants by Nramp1 iron transport activates MAP kinase signaling cascades that result in stabilization of Nramp1 mRNA.     

Haplotype Analyses of DNA Repair Gene Polymorphisms and Their Role in Ulcerative Colitis

Ulcerative colitis (UC) is a major clinical form of inflammatory bowel disease. UC is characterized by mucosal inflammation limited to the colon, always involving the rectum and a variable extent of the more proximal colon in a continuous manner. Genetic variations in DNA repair genes may influence the extent of repair functions, DNA damage, and thus the manifestations of UC. This study thus evaluated the role of polymorphisms of the genes involved in DNA repair mechanisms. A total of 171 patients and 213 controls were included. Genotyping was carried out by ARMS PCR and PCR-RFLP analyses for RAD51, XRCC3 and hMSH2 gene polymorphisms. Allelic and genotypic frequencies were computed in both control & patient groups and data was analyzed using appropriate statistical tests. The frequency of ‘A’ allele of hMSH2 in the UC group caused statistically significant increased risk for UC compared to controls (OR 1.64, 95% CI 1.16–2.31, p = 0.004). Similarly, the CT genotype of XRCC3 gene was predominant in the UC group and increased the risk for UC by 1.75 fold compared to controls (OR 1.75, 95% CI 1.15–2.67, p = 0.03), further confirming the risk of ‘T’ allele in UC. The GC genotype frequency of RAD51 gene was significantly increased (p = 0.02) in the UC group (50.3%) compared to controls (38%). The GC genotype significantly increased the risk for UC compared to GG genotype by 1.73 fold (OR 1.73, 95% CI 1.14–2.62, p = 0.02) confirming the strong association of ‘C’ allele with UC. Among the controls, the SNP loci combination of hMSH2:XRCC3 were in perfect linkage. The GTC and ACC haplotypes were found to be predominant in UC than controls with a 2.28 and 2.93 fold significant increase risk of UC.     

The Role of a Novel TRMT1 Gene Mutation and Rare GRM1 Gene Defect in Intellectual Disability in Two Azeri Families

Cognitive impairment or intellectual disability (ID) is a widespread neurodevelopmental disorder characterized by low IQ (below 70). ID is genetically heterogeneous and is estimated to affect 1–3% of the world’s population. In affected children from consanguineous families, autosomal recessive inheritance is common, and identifying the underlying genetic cause is an important issue in clinical genetics. In the framework of a larger project, aimed at identifying candidate genes for autosomal recessive intellectual disorder (ARID), we recently carried out single nucleotide polymorphism-based genome-wide linkage analysis in several families from Ardabil province in Iran. The identification of homozygosity-by-descent loci in these families, in combination with whole exome sequencing, led us to identify possible causative homozygous changes in two families. In the first family, a missense variant was found in GRM1 gene, while in the second family, a frameshift alteration was identified in TRMT1, both of which were found to co-segregate with the disease. GRM1, a known causal gene for autosomal recessive spinocerebellar ataxia (SCAR13, MIM#614831), encodes the metabotropic glutamate receptor1 (mGluR1). This gene plays an important role in synaptic plasticity and cerebellar development. Conversely, the TRMT1 gene encodes a tRNA methyltransferase that dimethylates a single guanine residue at position 26 of most tRNAs using S-adenosyl methionine as the methyl group donor. We recently presented TRMT1 as a candidate gene for ARID in a consanguineous Iranian family (Najmabadi et al., 2011). We believe that this second Iranian family with a biallelic loss-of-function mutation in TRMT1 gene supports the idea that this gene likely has function in development of the disorder.     

Carbon Flux and Carbohydrate Gene Families in Pineapple

The recently sequenced pineapple genome was used to identify and analyze some of the key gene families involved in carbohydrate biosynthesis, breakdown and modification. Gene products were grouped into glycosyltransferases (GT), glycoside hydrolases (GH), carbohydrate esterases (CE), and polysaccharide lyases (PL) based upon predicted catalytic activity. Non-catalytic carbohydrate-binding modules (CBM) and enzymes involved in lignification were also identified. The pineapple genes were compared with those from two and five monocot and eudicots species, respectively. The complement of pineapple sugar and cell wall metabolism genes is similar to that found in rice and sorghum, though the numbers of GTs and GHs is often fewer. This applies to a lesser extent to the genes involved in nucleotide-sugar interconversion, with both pineapple and papaya having a minimum complement. Interestingly, pineapple does not appear to contain mixed linkage β-glucan in its walls while possessing cellulose synthase-like (Csl), J and H genes. Pineapple and papaya have less than half the number of GT1 genes involved in small molecule glycosylation compared to Arabidopsis and tomato, and fewer members in GH families than Arabidopsis. The ratio of rice and sorghum to pineapple genes in GH families was more variable than in the case of GTs and it is unclear why pineapple GH gene numbers are so low. Rice, sorghum and pineapple have far fewer CE8, PL1 and GH28 genes related to pectin metabolism than most eudicots. The general lower number of cell wall genes in pineapple possibly reflects the absence of a genome duplication event. The data also suggests that pineapple straddles the boundary between grasses (family Poaceae) and eudicots in terms of genes involved in carbohydrate metabolism, which is also reflected in its cell wall composition.     

Alcohol Dehydrogenases: Identification and Names for Gene Families

Plant gene products that have been described as `alcohol dehydrogenases' are surveyed and related to their CPGN nomenclature. Most are Zn-dependent medium chain dehydrogenases, including `classical' alcohol dehydrogenase (Adh1), glutathione-dependent formaldehyde dehydrogenase (Fdh1), cinnamyl alcohol dehydrogenase (Cad2), and benzyl alcohol dehydrogenase (Bad1). Plant gene products belonging to the short-chain dehydrogenase class should not be called alcohol dehydrogenases unless such activity is shown.