逆境对大豆脱落纤维素酶基因时间表达模式的影响

用灵敏度较高的RT—PCR检测培养4周的大豆幼苗的5个不同组织：嫩叶、老叶、茎、离层和根,测得脱落纤维素酶基因的表达量互不相同,离层中表达量最高,茎中表达量最低。选取表达量最高的离层作为逆境处理材料,分别用高温（46C）、干旱、盐（200mmol／L NaCl）处理不同时间后,检测脱落纤维素酶基因的时间表达模式。结果表明：3种逆境条件下,脱落纤维素酶基因的时间表达模式各不相同,但总的来说,高温能抑制脱落纤维素酶基因的表达,干旱和盐都能促进脱落纤维素酶基因的表达。     

大豆基因家族的结构和表达分析

KNOX基因家族编码同源异型盒蛋白,在植物生长发育过程中起重要调控作用。利用生物信息学手段在全基因组水平上对大豆（Glycine Max）KNOX）（家族基因进行鉴定和分类,并分析其基因结构、蛋白同源结构域特征以及基因表达方式。研究结果表明：大豆中的27个GmKNOX基因可以分为GmKNOXl和GmKNOXll两个亚类,其中GmKNOXl类可分为3个主要的进化支,GmKNOXll类分为2个主要的进化支：26个GmKNOX基因不均匀地分布在16条染色体上,GmKNOX27尚无法定位。不同组织表达谱的分析表明：GmKNOXl类基因表达部位比较集中,以茎顶端分生组织中表达量最高：而GmKNOXll类基因的表达特异性较GmKNOXl类低,表达部位更广泛。     

大豆KNOX基因家族的结构和表达分析

KNOX基因家族编码同源异型盒蛋白, 在植物生长发育过程中起重要调控作用。利用生物信息学手段在全基因组水平上对大豆(Glycine max)KNOX家族基因进行鉴定和分类, 并分析其基因结构、蛋白同源结构域特征以及基因表达方式。研究结果表明: 大豆中的27个GmKNOX基因可以分为GmKNOX I和GmKNOX II两个亚类, 其中GmKNOX I类可分为3个主要的进化支, GmKNOX II类分为2个主要的进化支; 26个GmKNOX基因不均匀地分布在16条染色体上, GmKNOX27尚无法定位。不同组织表达谱的分析表明: GmKNOX I类基因表达部位比较集中, 以茎顶端分生组织中表达量最高; 而GmKNOX II类基因的表达特异性较GmKNOX I类低, 表达部位更广泛。     

大豆GmcpSecA基因的克隆及表达特异性

Sec途径是将核编码的叶绿体蛋白输入到类囊体腔的蛋白分选途径之一,对叶绿体正确行使其功能有重要作用。前期研究获得了拟南芥AtcpSecA功能缺失的突变体agyl,其叶片呈黄白色,叶绿体发育缺陷,内部缺少类囊体片层结构。我们从大豆中克隆了拟南芥AtepSecA的同源基因GmcpSecA基因的全长cDNA序列和5’端ATG上游1．5kb的启动子序列,通过RT-PCR的方法对GmcpSecA基因表达的器官特异性进行了初步分析;并构建了GmcpSecA：：GUS和35S：：GmcpSecA融合基因,以农杆菌介导的转化方法获得转基因拟南芥。GUS组织化学染色结果表明：在转基因拟南芥的子叶、叶片、花萼等绿色组织中都有较强的GUS表达,而在非绿色组织中没有GUS表达。通过将过表达载体p35S：：GmcpSecA转化agyl,结果表明GmcpSecA能够部分回补拟南芥agyl突变体的表型。推测GmcpSecA基因具有与AtcpSecA基因相似的功能,在叶绿体发育过程中发挥重要作用。     

铁蛋白基因表达对烟草耐低铁能力的影响

铁是植物生长发育的必需元素。由于土壤中的三价铁离子不能被植物直接利用。使一些植物经常表现出缺铁症状。为探讨利用铁蛋白基因提高植物耐低铁胁迫的作用,利用农杆菌介导法将大豆铁蛋白基因SoyFer1和内源反义铁蛋白基因NtFer2的cDNA分别导人烟草基因组,采集转基因烟草种子。对T1转基因烟草的卡那霉素抗性分析表明,整合到烟草基因组的外源基因多为单拷贝基因,也有少数为多拷贝基因。对具有卡那霉素抗性的转基因植株进行PCR检测和Northern杂交分析表明,外源基因已整合到烟草基因组中,并且得到了正确表达。将转基因株系移栽到铁离子浓度不同的培养基中生长2个月后进行比较表明,转大豆铁蛋白基因烟草株系的生长量明显高于非转基因烟草株系,而转内源反义铁蛋白基因烟草株系的生长量则明显低于非转基因烟草株系。转大豆铁蛋白基因和转内源反义铁蛋白基因烟草株系的叶绿素含量、丙二醛（MDA）含量和过氧化物酶（POD）活性等生理性状也发生了明显变化,表现为转大豆铁蛋白基因株系的叶绿素含量明显增加,POD活性明显增强,MDA含量明显降低：而转内源反义铁蛋白基因株系的叶绿素含量、POD活性和MDA含量等则表现为与转大豆铁蛋白基因株系的相反。铁蛋白过量表达提高了烟草耐低铁能力,而铁蛋白抑制表达则降低了烟草耐低铁能力。     

大豆转录因子GmNAC2a基因克隆及表达

利用NTT(核蛋白筛选系统)从大豆耐盐品种'铁丰八号'中克隆到1个新的NAC转录因子基因GmNAC2a,该基因DNA片段长度为900 bp,编码299个氨基酸,N端包含1个NAM保守域.系统进化树分析表明,GmNAC2a属于ATAF亚族,GmNAC2a与花生AhNAC1亲缘关系最近,同源性达到76.47%.GmNAC2...     

阜豆GmABC基因的克隆及表达分析

利用RACE技术从大豆品种‘阜豆11号’中克隆到1个ABC转运蛋白基因,该基因cDNA全长为4 693bp,其中开放读码框4 341bp,编码1 447个氨基酸,分子量162.5kD,具有高度保守的ATP结合位点,命名为GmABC。蛋白序列比对结果显示,该基因编码蛋白属于PDR(pleiotropic drug resistance)多向耐药性蛋白家族成员。系统进化树分析显示,GmABC与苜蓿PDR亲缘关系最近,相似性达84%。基因表达分析显示,GmABC受镉诱导表达,当Cd2+浓度达到100mg.L-1时,其表达量最高。研究表明,GmABC可能对阜豆镉胁迫抗性发挥重要作用。     

外源GA3对毛竹实生苗茎秆生长及CesA基因表达的影响

以毛竹实生苗为试验材料,研究不同浓度外源GA₃（0,0.1,0.5,1 μmol·L^-1）对毛竹生长及CesA基因表达的影响。结果表明,与未经GA₃处理相比,施用外源GA₃后,毛竹实生苗茎节间和纤维细胞显著伸长,初生壁纤维素合成相关基因PeCesA2和PeCesA6相对表达量明显上调,次生壁相关基因PeCESA4和PeCESA4-1显著下调,傅里叶红外光谱分析（FTIR）,发现毛竹茎秆纤维素特征峰强度（1 060,1 160及1 373 cm^-1）随着GA₃浓度升高而逐渐增强,表明施用外源GA₃能够影响毛竹茎秆CesA基因表达,PeCesA2和PeCesA6的表达与外源GA₃促进纤维细胞伸长的过程存在一定联系。     

人锰超氧化物歧化酶基因剪接异构体的表达分析

对人锰超氧化物歧化酶(human manganese superoxide dismutase,hMn-SOD)基因剪接异构体进行分析,并检测异构体的表达情况。在GenBank库中检索人锰超氧化物歧化酶基因异构体及编码基因组序列,利用Vector NTI9生物软件进行核酸及蛋白序列比对;利用RT-PCR方法分析锰超氧化物歧化酶基因异构体的表达。结果显示,在GenBank库检索发现有3种人锰超氧化物歧化酶基因异构体,剪接异构的类型为可变的5′剪接位点和外显子盒,各异构体基因内含子均符合"GT-AG"规则。3种基因异构体编码两种异构体蛋白,即222个氨基酸的人锰超氧化物歧化酶蛋白以及中部缺少39个氨基酸的截短型异构蛋白。RT-PCR检测结果表明,剪接异构体hMn-SODb在HEK293T和HSC细胞中的表达比在HepG2细胞中高,未见异构体hMn-SODc的表达。     

水稻淀粉分支酶基因5′上游区缺失对基因表达的影响

为研究水稻淀粉分支酶基因 (sbe1) 5′上游调控区中存在的顺式作用元件 ,我们将水稻sbe1基因翻译起始点 (ATG) 5′上游区 1.2kb(- 10 96～ 74bp)片段经过不同限制性内切酶消化及外切核酸酶ExoIII部分消化 ,得到 4个 5′端缺失的片段。将这些缺失片段分别与 gus基因编码区连接 ,构建成融合质粒 ,经土壤农杆菌 (Agrobacterium)介导引入水稻 ,定量测定转基因水稻植株未成熟种子中的 gus酶活力。结果表明 ,- 5 16～ 6 4bp的sbe1启动子片段可以驱动gus基因的高表达 ,其它 3个启动子片段 (- 10 96～ 74bp ,- 2 95～ 74bp ,- 146～ 6 4bp)驱动 gus基因表达的能力较低。推测在sbe1基因 5′上游区 - 5 16～ - 2 95bp片段中可能存在能使 gus基因高表达的增强元件     

Effects of Melatonin on Growth,Physiology and Gene Expression in Rice Seedlings Under Cadmium Stress

Melatonin (MLT) is a hormonal substance found in many organisms and can improve plant stress resistance. In this study, the japonica rice variety Y32 and indica rice variety NJ6 were cultivated in hydroponics under different concentrations of CdCl₂ at the two-leaf stage. The growth, physiological and biochemical responses of the seedlings and the expression of cadmium (Cd)-related genes under exogenous melatonin (MLT) treatment were assessed. The results indicated that Cd stress destroyed the dynamic balance between reactive oxygen species (ROS) production and removal, resulting in ROS accumulation, membrane lipid peroxidation, and impaired growth and development. Following the application of exogenous MLT to rice seedlings, increases in plant biomass including both underground and above-ground areas were observed. MLT also scavenged the inhibition of superoxide dismutase (SOD) and peroxidase (POD) in a concentration dependent manner in response to Cd stress. Catalase (CAT) activity and malondialdehyde (MDA) expression also decreased following MLT treatment. Amongst the six Cd-related genes assessed, five genes were down-regulated and one was up-regulated in response to MLT treatment. Taken together, these data demonstrate that MLT improves the resilience of rice seedlings at the biochemical, physiological, and molecular levels, and diminishes the damage caused by Cd stress.     

用gfp基因标记法研究大豆根瘤菌在大豆根部定殖结瘤情况

采用三亲本杂交的方法,将绿色荧光蛋白基因(gfp)转入高效、抗逆、广适应性的快生大豆根瘤菌Sinorhizobium frediiCCBAU 01287中,获得含gfp基因的转基因菌株CBAU 01287(G);平板传代和共生检测表明:外源质粒在CCBAU 01287中能够自我复制,稳定遗传。进一步研究表明,gfp标记菌CCBAU 01287(G)可用于实时监测根瘤菌在大豆根部的早期定殖情况和定殖密度的测定;标记菌株对大豆的生长及生物量的积累与出发菌株的效果无显著差异。     

GUS Expression in Protoplasts of Immature cotyledons of Soybean

The E. coli beta-glucuronidase (GUS) gene was used in gene expression experiments with the protoplasts isolated from immature cotyledons of soybean (Glycine max L.). Transient expression of GUS gene could be detected in 1—6 days after DNA incorporation into soybean protoplasts by using a fluorogenic substrate MUG. Stable transformation was observed by histochemical localization with the use of a substrase X-Gluc. Some factors such as PEG toxicity and protoplast stability affecting PEG-mediated transformation were discussed.     

大豆胞囊线虫抗性基因定位与克隆研究进展

大豆胞囊线虫（soybean cyst nematode,SCN）是大豆生产上一种危害严重的世界性害虫,能给大豆生产造成极大损失。大豆抗性品种选育是防治其措施中最经济、有效的方法。大豆SCN抗性的分子遗传学研究是开展大豆SCN抗性分子育种的理论基础,本文针对SCN抗性基因定位和克隆两个方面的研究现状进行了综述,并对当前研究中存在的问题及发展前景进行了讨论与展望。     

外源水杨酸对NaCl胁迫下大豆种子萌发和幼苗生长生理的影响

以大豆种子、幼苗为试验材料,采用砂培的方法,研究了0.2mmol·L-1外源水杨酸(SA)对100mmol·L-1 NaCl胁迫下大豆种子萌发、幼苗形态及生物量、膜脂过氧化和抗氧化酶活性的影响。结果显示:NaCl胁迫下,大豆种子萌发和幼苗生长受到显著抑制,且随着胁迫时间的延长(0~3d),大豆幼苗相对电解质渗漏率、硫代巴比妥酸活性产物(TBARS)含量显著升高,超氧化物歧化酶(SOD)、过氧化氢酶(CAT)、抗坏血酸过氧化物酶(APX)活性均明显降低。外源SA促进NaCl胁迫下大豆种子萌发和根茎生长,增加幼苗生物量积累,降低幼苗叶片相对电解质渗漏率和TBARS含量,增强其叶片SOD、CAT、APX活性。研究表明,NaCl胁迫能显著抑制大豆种子萌发和幼苗生长,而一定浓度的外源SA能有效提高NaCl胁迫下大豆种子活力及幼苗抗氧化酶活性,减轻膜脂过氧化程度,缓解NaCl胁迫所造成的伤害,提高大豆幼苗抗盐胁迫的能力。     

Gene Expression and Polymorphism of Myostatin Gene and its Association with Growth Traits in Chicken

Myostatin is a member of TGF-β super family and is directly involved in regulation of body growth through limiting muscular growth. A study was carried out in three chicken lines to identify the polymorphism in the coding region of the myostatin gene through SSCP and DNA sequencing. A total of 12 haplotypes were observed in myostatin coding region of chicken. Significant associations between haplogroups with body weight at day 1, 14, 28, and 42 days, and carcass traits at 42 days were observed across the lines. It is concluded that the coding region of myostatin gene was polymorphic, with varied levels of expression among lines and had significant effects on growth traits. The expression of MSTN gene varied during embryonic and post hatch development stage.     

锰对植物毒害及植物耐锰机理研究进展

含锰矿渣的排放造成了严重的土壤锰污染。揭示锰毒害和植物的耐锰机制对于污染土壤治理具有重要意义。研究表明,高浓度的Mn2＋能够抑制根系Ca2＋、Fe2＋和Mg2＋等元素的吸收及活性,引起氧化性胁迫导致氧化损伤,使叶绿素和Rubisco含量下降、叶绿体超微结构破坏和光合速率降低。而锰超累积植物则具有多种解毒或耐性机制,如区域化、有机酸螯合、外排作用、抗氧化作用和离子交互作用等。根系主要通过有机酸的螯合作用促进植物对Mn^2＋的转运解毒,同时能够将过量的Mn^2＋区域化在根细胞壁中;叶片可通过酚类物质或有机酸螯合Mn^2＋,并将其区域化在叶片表皮细胞和叶肉细胞的液泡中（或通过表皮毛将Mn^2＋排出体外）。其中,金属转运蛋白在植物对Mn^2＋的吸收、转运、累积和解毒过程中发挥着重要作用。     

Inheritance and Gene Mapping of Resistance to Soybean Mosaic Virus Strain SC14 in Soybean

Soybean mosaic virus (SMV) is one of the most broadly distributed diseases worldwide. It causes severe yield loss and seed quality deficiency in soybean (Glycine max (L.) Merr.). SMV Strain SC14 isolated from Shanxi Province, China, was a newly identified virulent strain and can infect Kefeng No. 1, a source with wide spectrum resistance. In the present study, soybean accessions, PI96983, Qihuang No. 1 and Qihuang No. 22 were identified to be resistant (R) and Nannong 1138‐2, Pixianchadou susceptible (S) to SC14. Segregation analysis of PI96983 x Nannong 1138‐2 indicated that a single dominant gene (designated as R_SC14) controlled the resistance to SC14 at both V₂ and R₁ developmental stages. The same results were obtained for the crosses of Qihuang No. 1 × Nannong 1138‐2 and Qihuang No. 22 × Nannong 1138‐2 as in PI96983 × Nannong 1138‐2 at V₂ stage, but at R₁ stage, the F₁ performed as necrosis (a susceptible symptom other than mosaic), F₂ segregated in a ratio of 1R:2N:1S, and the progenies of necrotic (N) F₂ individuals segregated also in R, N and S. It indicated that a single gene (designated as R_SC14Q, to be different from that of PI96983) controlled the resistance to SC14, its dominance was the same as in PI96983 × Nannong 1138‐2 (without symptoms) at V₂ stage and not the same at R₁ stage. The tightly linked co‐dominant simple sequence repeat (SSR) marker Satt334 indicated that all the heterozygous bands were completely corresponding to the necrotic F₂ individuals, or all the necrotic F₂ individuals were heterozygotes. It was inferred that necrosis might be due to the interaction among SMV strains, resistance genes, genetic background of the resistance genes, and plant development stage. Furthermore, the bulked segregant analysis (BSA) of SSR markers was conducted to map the resistance genes. In F2of PI96983 × Nannong 1138‐2, five SSR markers, Sat_297, Sat_234, Sat_154, Sct_033 and Sat_120, were found closely linked to RSC14, with genetic distances of 14.5 cM, 11.3cM, 4.3cM,3.2cM and 6cM, respectively. In F₂ of Qihuang No. 1 × Nannong 1138‐2, three SSR markers, Sat_234, Satt334 and Sct_033, tightly linked to R_SC14Q with genetic distances of 7.2 cM, 1.4 cM and 2.8 cM, respectively. Based on the integrated joint map by Cregan et al. (1999), both RScMand R_SC14Q were located between Sat_234 and Sct_033 on linkage with group F of soybean, with their distances from Sct_033 at the same side being 3.2 cM and 2.8 cM, respectively. Therefore, RSC14and R_SC14Q might be on a same locus. The obtained information provides a basic knowledge for marker‐assisted selection of the resistance gene in soybean breeding programs and fine mapping and map‐based cloning of the resistance gene. (Managing editor: Li‐Hui Zhao)     

人Mn—SOD cDNA的克隆及高效表达

用逆转录－聚合酶链反应（ＲＴ－ＰＣＲ）,以人肝细胞株（Ｌ０２）总ＲＮＡ为模板,扩增了人锰超氧化物歧化酶（ｈＭｎ－ＳＯＤ）的ｃＤＮＡ。重组到Ｔ７启动子控制下的表达载体ｐＥＴ－２４ａ（＋）中,构建表爱质粒ｐＥＴ－ＭｎＳＯＤ,并转化大肠杆菌ＢＬ２１（ＤＥ３）。ＳＤＳ－ＰＡＧＥ及蛋白质印迹分析表明,经１ｍｍｏｌ／Ｌ异丙基硫代－β－Ｄ－半乳糖苷（ＩＰＴＧ）诱导后,可高效表达一分子量为２２ｋＤ的蛋白质,与抗人     

人胰岛素生长因子Ⅰ基因的人工合成,克隆及其表达

采用固相亚磷酸三脂法,化学合成了人胰岛样生长因子Ｉ结构基因的两个１２９聚体长单链ＤＮＡ片段,通过其中的２３ｂｐ互补配对和Ｋｌｅｎｏｗ酶酶促补齐成为ＩＧＦ－Ｉ中进行ＤＮＡ全序列测定分析及寡核苷酸引导的定向点空变校正,获得了人工合成的ＩＧＦ－Ｉ结构基因。进一步分别重组构建了在Ｐｌａｃ和ＰＬＰｒｏｍｏｔｅｒ控制下的人工合成ＩＧＦ－Ｉ基因表达质粒ＰＨＭ５９０和ＰＢＬＥ０１１,在大肠杆菌中进行了表达研究。经