玉米胚胎发生后期丰富蛋白基因的启动子克隆与功能验证

该研究在生物信息学分析的基础上,克隆玉米胚胎发生后期丰富蛋白基因(MGL3)的启动子序列(pMGL3),进行非生物逆境应答元件分析以及实时定量PCR验证其非生物逆境胁迫响应特性,构建了pMGL3启动子驱动报告基因(GUS)表达载体,基因枪法转化玉米愈伤组织,通过GUS染色验证pMGL3启动子在非生物逆境胁迫下的驱动活性。再根据启动子序列分析结果,去除不同的顺式作用元件,构建不同长度pMGL3启动子驱动报告基因GUS表达载体,农杆菌介导法转化烟草叶盘,以确定pMGL3启动子的最短活性序列。结果显示:pMGL3启动子长1 554bp,存在多种与非生物逆境胁迫应答相关的调控元件,在干旱、高盐、低温胁迫及脱落酸、乙烯诱导下驱动MGL3基因增量表达,用以驱动GUS基因转化玉米愈伤组织,在高渗、高盐、低温胁迫及脱落酸诱导下具有驱动活性,且截短至325bp仍可保持驱动活性。研究表明,pMGL3启动子的确有非生物逆境诱导启动活性,进一步验证其作用机理后可运用于玉米抗逆转基因研究。     

海州香薷(Elsholtzia haichowensis Sun)细胞壁转化酶基因启动子(EhcwINVP)的克隆及活性分析

以海州香薷基因组DNA为模板,通过hiTAIL-PCR和walking技术扩增得到其细胞壁转化酶基因启动子(Ehcw INVP)片段,长度为1727 bp。生物信息学分析结果表明,该启动子片段中含有多个对脱落酸、赤霉素、细胞分裂素等激素以及对干旱、低温、重金属铜等逆境胁迫响应相关的顺式作用元件。将通过克隆得到的Ehcw INVP序列替换p CAMBIA1301载体上驱动GUS报告基因表达的Ca MV35S启动子序列,构建Ehcw INVP融合GUS的植物表达载体Ehcw INVP::GUS。转基因拟南芥植株的组织化学分析结果表明,海州香薷细胞壁转化酶基因启动子序列具有驱动GUS基因表达的功能,且在10μmol/L铜胁迫下,转基因拟南芥植株叶和根中的GUS活性分别约是对照组的1.7倍和1.5倍。     

百子莲脱水素基因ApY2SK2逆境应答模式及启动子调控功能研究

在百子莲胚性细胞中筛选到对超低温保存复合逆境具有积极响应的保护类蛋白脱水素(ApY_2SK_2),为探明ApY_2SK_2基因在复合逆境中的应答模式,该研究采用染色体步移技术克隆并分析了ApY_2SK_2编码基因上游1 200 bp的启动子序列。结果表明:(1)序列分析显示,该启动子含有多个与逆境和激素诱导相关的顺式调控元件;实时荧光定量PCR结果表明,ApY_2SK_2基因的表达具有组织特异性,在百子莲的叶和果中表达量较高,且在多种胁迫处理与ABA激素诱导下,其表达量显著升高。(2)成功构建了5个ApY_2SK_2启动子不同缺失片段驱动GUS基因的融合表达载体,经农杆菌转化、抗性筛选和PCR检测鉴定,获得T_3代纯和转基因拟南芥株系。(3) GUS组织化学染色结果显示,GUS基因在拟南芥幼苗全株、成年苗的叶、花和成熟果实中表达活性较强,但在未成熟果实中无明显表达;烟草瞬时表达结果显示,与对照组相比,在脱水胁迫和ABA处理下的ApY_2SK_2启动子不同缺失片段驱动GUS基因表达具有显著差异。(4)转基因拟南芥GUS活性测定结果显示,ApY_2SK_2启动子MBS元件和ABRE元件可响应干旱与渗透胁迫信号;ApY_2SK_2启动子LTR元件参与低温响应;ApY_2SK_2启动子-1 199～-262 bp区域包含多个串联的ABRE顺式调控元件(-373～-211 bp)对响应ABA信号具有主要调控作用。该研究结果揭示了ApY_2SK_2启动子的组织特异性,且启动子上的关键顺式调控元件对不同的胁迫和激素信号响应具有决定性调控作用。     

白桦BpbHLH112基因克隆及其启动子表达特性分析

克隆白桦BpbHLH112基因的编码序列，并进行生物信息学分析。通过实时荧光定量PCR技术分析该基因在不同胁迫处理下的表达模式，进一步克隆了BpbHLH112基因上游1 446 bp的启动子区域，序列分析表明，该区域含有多个逆境响应、激素响应以及信号转导等相关元件，通过构建BpbHLH112启动子片段融合GUS报告基因的表达载体并进行烟草瞬时转化，分析在不同胁迫处理条件下BpbHLH112启动子驱动GUS基因表达的活性，结果表明BpbHLH112启动子的表达能够被一些逆境胁迫因子诱导，本研究结果为深入研究BpbHLH112调控白桦应对非生物胁迫作用的分子机理提供了理论依据。     

白桦BpZFP4基因启动子克隆和逆境响应元件功能分析

前期研究发现白桦锌指蛋白BpZFP4基因响应多种非生物逆境胁迫。为了深入研究其调控机制,本研究利用染色体步移技术克隆了该基因上游1 360 bp的启动子区域,序列分析结果表明该区域含有多个逆境响应顺式作用元件、激素响应元件、光响应以及病原菌和损伤响应元件等。在此基础上,构建了BpZFP4启动子5'-端一系列缺失片段融合GUS报告基因的表达载体。通过对系列缺失突变体在正常条件以及渗透胁迫、盐胁迫和脱落酸（ABA）处理条件下的GUS基因表达分析,鉴定得到BpZFP4启动子对干旱、盐和ABA应答响应的主要调节区域及可能的顺式作用元件。本研究结果为进一步探究BpZFP4基因应答非生物胁迫和信号分子刺激的调控机理提供了重要的理论依据。     

玉米钼辅助因子硫酸化酶基因启动子的克隆与功能验证

为克服组成型启动子启动外源基因过量表达引起的诸多问题,同源克隆(Mo-molybdopterin cofactor sulfurase)基因（ABA3）的启动子(ABA3s)序列,并用PlantCARE软件分析其非生物逆境应答元件, 实时定量PCR检测ABA3基因在非生物逆境诱导下的差异表达后。然后,用该启动子构建启动GUS（β-glucuronidase）基因的表达载体, 基因枪法转化玉米愈伤组织。经组织化学染色法检测其表达后, 在高渗、高盐、低温胁迫处理及ABA诱导下检测GUS酶荧光值与荧光素酶(内参)发光值的比值(GUS/LUC), 以此评价ABA3s启动子在非生物逆境胁迫下的启动活性。结果表明, ABA3基因在模拟干旱、低温、高温、高盐胁迫及ABA、乙稀诱导下差异表达, 说明该基因的启动子(ABA3s)具有非生物逆境诱导活性。序列分析表明, ABA3s启动子全长777 bp, 含有ARE、HSE、MBS、TGA、Circadian等多种非生物逆境胁迫应答元件。用ABA3s启动GUS基因构建的表达载体转化的玉米愈伤组织, 响应干旱、低温、高温、高盐胁迫等多种非生物逆境胁迫, 及ABA和乙稀诱导, GUS检测呈阳性。在8%甘露醇高渗条件下, GUS/LUC比值比空白对照高6倍。上述结果表明, ABA3s启动子具有非生物逆境诱导特性, 经进一步验证其功能后, 可用于玉米抗逆转基因研究。     

白桦BpSPL2基因启动子的克隆及表达分析

SPL(SQUAMOSA promoter-binding protein-like)是植物特有的转录因子,研究表明其在参与发育阶段转变、花和果实发育等方面起着重要作用。利用PCR技术从白桦基因组DNA中扩增获得BpSPL2基因上游1 960 bp启动子序列,使用PLACE和Plant CARE在线软件分析序列,发现BpSPL2基因启动子序列中含有与开花、非生物胁迫及激素响应等相关的顺式作用元件,暗示其在植物的生长发育和胁迫应答中起重要作用。进而构建了BpSPL2基因启动子驱动GUS报告基因的植物表达载体,并利用农杆菌介导将其瞬时转化至白桦和拟南芥,通过GUS组织化学染色检测BpSPL2基因启动子的组织表达特性,结果表明BpSPL2基因启动子具有启动子活性,能够驱动GUS基因在白桦和拟南芥中表达;而其表达活性在白桦的叶片、芽及根部中较强,在拟南芥的花药、雌蕊和叶片较强,为进一步研究白桦BpSPL2基因的表达调控及其功能分析提供参考。     

OsEBP-89启动子中应答茉莉素信号的必需DNA区域的分析

水稻OsEBP-89基因的表达受乙烯（ET）、脱落酸（ABA）、茉莉素等激素和干旱、低温等逆境胁迫处理的诱导．本研究中,克隆该基因启动子和预测应答胁迫与激素信号相关顺式作用元件的基础上,通过农杆菌注射法介导的瞬时表达证实了该启动子在烟草叶片中驱动GUS报告基因的表达受茉莉素的诱导．为了进-步确定该启动子中应答茉莉素信号的重要DNA区域,对该启动子进行了-系列的缺失突变,并将相关的缺失启动子片段与GUS报告基因融合．烟草叶片中GUS报告基因瞬时表达分析表明,该启动子中位于-1200bp和-800bp的碱基是该基因应答茉莉素信号的必需DNA区域,其中在-1127bp处有一个G—box元件;结合已有的研究结果,发现应答茉莉素信号的必需DNA区域不同于该基因应答ACC处理的必需DNA区域（在-562bp处存在一个ERE元件）．总之,本研究结果有助于探讨该基因应答不同胁迫信号表达的分子机制．     

桑树磷脂酶MaPLA1-2D亚型4个基因的克隆与胁迫应答分析

磷脂酶(phospholipase)是一类在植物生长发育和胁迫应答中起重要调控作用的磷脂水解酶,也是一类重要的信号转导酶。而磷脂酶A1(PLA1)在植物应答生物胁迫和非生物胁迫中的功能研究鲜见报道。研究从桑树(Morus alba L.)中克隆了磷脂酶PLA1的1个亚型MaPLA1-2D基因,对其进行了序列分析、组织表达、胁迫诱导表达和蛋白亚细胞定位分析。结果表明,桑树PLA1-2D亚型基因包括4个成员,命名为MaPLA1-2D.1~MaPLA1-2D.4。4个基因在桑树根和叶中高水平表达,蛋白亚细胞定位在叶绿体。序列和进化分析表明MaPLA1-2D基因4个成员与拟南芥AtDAD1基因的保守结构域序列具有较高相似度且进化关系紧密。MaPLA1-2D基因4个成员的启动子含有多种胁迫应答顺式元件和激素响应元件;胁迫诱导表达模式分析表明MaPLA1-2D基因表达受干旱和脱落酸处理显著诱导。以上结果说明,MaPLA1-2D基因与拟南芥DAD同源,可能在桑树非生物胁迫应答中发挥重要功能。     

大豆转录因子GmERF5启动子的克隆及活性分析

乙烯响应因子(Ethylene-responsive factors,ERFs)广泛参与植物对生物和非生物胁迫的应答。从大豆吉林32的基因组DNA中分离到GmERF5的启动子片段,全长1 924 bp。该区段含有9种与逆境相关的顺式作用元件,即G-box、GT-1、LTRE-1、W-box、TL1、DPBF、MYB、MYC和BIHD10S。将该启动子构建到植物表达载体pCAMBIA1301上与葡萄糖苷酸酶(GUS)基因融合,注射法转化烟草叶片,并进行干旱、高盐和低温处理,通过GUS组织化学染色和GUS荧光值的测定分析启动子的启动活性。结果表明,在未处理条件下,该启动子能驱动下游GUS基因的表达。干旱和低温处理10 h能明显增强GmERF5P的启动活性。     

Comparative study of Bifidobacteriumanimalis, Escherichiacoli, Lactobacilluscasei and Saccharomycesboulardii probiotic properties

The present work investigates some probiotic properties of four different microorganisms (Bifidobacterium animalis var. lactis BB-12, Escherichia coli EMO, Lactobacillus casei and Saccharomyces boulardii). In vitro and in vivo tests were carried out to compare cell wall hydrophobicity, production of antagonistic substances, survival capacity in the gastrointestinal tract of germ-free mice without pathological consequence, and immune modulation by stimulation of Küpffer cells, intestinal sIgA and IL-10 levels. In vitro antagonism against pathogenic bacteria and yeast was only observed for the probiotic bacteria B. animalis and L. casei. The hydrophobic property of the cell wall was higher for B. animalis and E. coli EMO, and this property could be responsible for a better ability to colonize the gastrointestinal tract of germ-free mice. Higher levels of sIgA were observed mainly for S. boulardii, followed by E. coli EMO and B. animalis, and only S. boulardii induced a significant higher level of IL-10. In conclusion, for a probiotic use, S. boulardii presented better characteristics in terms of immunomodulation, and B. animalis and L. casei for antagonistic substance production. The knowledge of the different probiotic properties could be used to choice the better microorganism depending on the therapeutic or prophylactic application.     

Non-specificity of a colorimetric method for the estimation of N-acetyl-d-glucosamine

The colorimetric method of Reissig et al. for the estimation of N-acetylamino sugars, is often used as a specific method for the quantification of the N-acetyl-d-glucosamine. Although this assay is more sensitive to the monomer, it recognizes all soluble N-acetyl-d-glucosamine oligomers. This result is very important because this method is extensively used in biology for the estimation of chitinolytic activity.     

Effects of MULTIFOLIATE-PINNA, AFILA, TENDRIL-LESS and UNIFOLIATA genes on leafblade architecture in Pisum sativum

In order to dissect the genetic regulation of leafblade morphogenesis, 16 genotypes of pea, constructed by combining the wild-type and mutant alleles of MFP, AF, TL and UNI genes, were quantitatively phenotyped. The morphological features of the three domains of leafblades of four genotypes, unknown earlier, were described. All the genotypes were found to differ in leafblade morphology. It was evident that MFP and TL functions acted as repressor of pinna ramification, in the distal domain. These functions, with and without interaction with UNI, also repressed the ramification of proximal pinnae in the absence of AF function. The expression of MFP and TL required UNI function. AF function was found to control leafblade architecture multifariously. The earlier identified role of AF as a repressor of UNI in the proximal domain was confirmed. Negative control of AF on the UNI-dependent pinna ramification in the distal domain was revealed. It was found that AF establishes a boundary between proximal and distal domains and activates formation of leaflet pinnae in the proximal domain.     

Presence of Rhizobium Etli bv . Phaseoli and Rhizobium Gallicum bv . Gallicum in Egyptian Soils

Seven bean rhizobial strains EBRI 2, 3, 21, 24, 26, 27 and 29 identified as Rhizobium etli, and EBRI 32 identified as Rhizobium gallicum, isolated from Egyptian soils and which nodulated Phaseolus vulgaris efficiently, were subjected to hybridization with a nifH probe in order to estimate the copy number of this gene. Seven strains (EBRI 2, 3, 21, 24, 26, 27 and 29) which were only able to nodulate Phaseolus vulgaris, contained three copies of the nifH gene, consistent with their identification as Rhizobium etli bv. phaseoli. Only one strain (EBRI 32) which nodulated both Phaseolus vulgaris and Leucaena leucocephala, had one copy of nifH gene. This confirmed the classification of this strain as Rhizobium gallicum bv. gallicum.     

Characterisation of cell wall polysaccharides, arabinogalactans-proteins (AGPs) and phenolics of Cola nitida, Cola acuminata and Garcinia kola seeds

Many Cola plant species are endemic to West and Central Africa. Cola acuminata and Cola nitida are used as masticatory when fresh, while the dried nuts are used for beverages and pharmaceutical purposes in Europe and North America. Garcinia kola seeds, that serve as a substitute for the true kola nuts, are used in African traditional medicine for the treatment of various diseases, including colic, headache and liver cirrhosis. Seeds extracts of G. kola are also known for their anti-inflammatory, antimicrobial and antiviral properties. To gain information on the chemical properties of the kolas, we have isolated and analyzed cell wall polysaccharides, arabinogalactan-proteins and phenolic substances from the seeds of the three kola species. The sugar composition of cell wall material of C. acuminata, C. nitida and G. kola revealed that Gal (up to 30%), Ara, GalA and Glc as the predominant monosaccharides, representing approximately 90% by mol of the total hydrolysable sugar present in this material. In Ammonium oxalate cell wall fraction, GalA was found to be the major sugar present in all kola species. In the alkali-soluble fraction, there were significant differences in the level of Glc and Gal. The level of Glc was high in C. acuminata and C. nitida while the level of Gal and Xyl were high in C. nitida and G. cola. Isolation and quantification of arabinogalactan-proteins demonstrate that G. kola seeds contained four to eight times more of these proteoglycans than the seeds of the other two species. Finally, analysis of soluble phenolic substances shows that caffeine and catechin were largely represented in C. acumina and C. nitida seeds, with caffeine accounting for 50% of all soluble phenolics. These findings indicate that the three Kola seeds are highly enriched in pectins and proteoglycans and that C. acuminata and C. nitida can be used as a possible source of caffeine and catechin.     

转Cry1Ac/1Ab基因棉花对异色瓢虫生长发育及其捕食功能的影响

【目的】为探究转Cry1Ac/1Ab基因棉花对异色瓢虫生长发育及其捕食功能的影响。【方法】以转Cry1Ac/1Ab基因棉与其亲本常规棉为实验材料,利用取食不同棉花品种叶片的棉铃虫饲喂异色瓢虫幼虫。【结果】与常规亲本棉相比,取食饲喂转基因棉花叶片的初孵棉铃虫幼虫的异色瓢虫幼虫从1龄发育至化蛹期时间延长0.77 d,但差异不显著;除1龄幼虫体重增加(0.0773 mg)外,其余各龄期幼虫体重均有所下降,但差异均不显著;异色瓢虫1、2、3、4龄幼虫对初孵棉铃虫捕食量均随棉铃虫密度的增加而增加,捕食功能反应均符合HollingⅡ圆盘方程。【结论】转Cry1Ac/1Ab基因棉花对异色瓢虫生长发育无显著影响,饲喂取食转Cry1Ac/1Ab基因棉花的棉铃虫对异色瓢虫捕食功能无显著差异。     

Characterization of recA genes and recA mutants of Rhizobium meliloti and Rhizobium leguminosarum biovar viciae

Summary DNA fragments carrying the recA genes of Rhizobium meliloti and Rhizobium leguminosarum biovar viciae were isolated by complementing a UV-sensitive recA ^– Escherichia coli strain. Sequence analysis revealed that the coding region of the R. meliloti recA gene consists of 1044 by coding for 348 amino acids whereas the coding region of the R. leguminosarum bv. viciae recA gene has 1053 bp specifying 351 amino acids. The R. meliloti and R. leguminosarum bv. viciae recA genes show 84.8% homology at the DNA sequence level and of 90.1% at the amino acid sequence level. recA ^– mutant strains of both Rhizobium species were constructed by inserting a gentamicin resistance cassette into the respective recA gene. The resulting recA mutants exhibited an increased sensitivity to UV irradiation, were impaired in their ability to perform homologous recombination and showed a slightly reduced growth rate when compared with the respective wild-type strains. The Rhizobium recA strains did not have altered symbiotic nitrogen fixation capacity. Therefore, they represent ideal candidates for release experiments with impaired strains.The accession numbers: X59956 R. LEGUMINOSARUM REC A ALAS-DNA; X59957 R. MELITOTI REC A ALAS-DNA     

Analysis of urinary N-acetyl-S-(N-methylcarbamoyl)cysteine, the mercapturic acid derived from N,N-dimethylformamide

Human biotransformation of the industrial solvent N,N-dimethylformamide gives raise to N-acetyl-S-(N-methylcarbamoyl)cysteine (AMCC) which has the longest half-life (about 23 h) among urinary metabolites of N,N-dimethylformamide. It could be used for monitoring industrial exposure over several workdays, by measuring it in urine samples collected at the end of the working week. This is consistent with the suggestions of the American Conference of Governmental Industrial Hygienists, which established a limit of 40 mg/l for the year 2000. An easy, cheap and user-friendly method has been developed for determination of urinary AMCC. Unlike currently available methods, it requires neither a time-consuming preparation phase nor gas chromatographic analysis with a nitrogen-phosphorus or mass detector. The method uses high-performance liquid chromatography (HPLC), with an UV detector at 436 nm. A 10-μl volume of urine is added to a carbonate–hydrogen carbonate buffer and mixed with a dabsyl chloride solution in acetonitrile. The reaction between AMCC and the reagent is performed at 70°C for 10 min. The ‘dabsylated’ product is stable for at least 12 h. After brief centrifugation, the solution is ready for HPLC analysis using a C₁₈ column (250×4.6 mm, 5 μm). The method is sensitive (detection limit 1.8 mg/l) and specific. It identified urinary AMCC in urine of 40 subjects not exposed to N,N-dimethylformamide with a median concentration of 3.9 mg/l. In urine samples from 20 workers exposed to N,N-dimethylformamide (5–40.8 mg/m³), AMCC concentrations ranged from 16 to 170 mg/l. Industrial toxicology laboratories with limited instrumentation will be able to use it in the biological monitoring of workers exposed to N,N-dimethylformamide.     

Application of petG-trnP sequence to systematic study of Chinese Cupressus species

Chinese Cupressus L. includes five species. The molecular phylogenetic relationship of the Cupressus species and Chamaecyparis L. were determined by comparing 417–479 bp of chloroplast petG-trnP intergenic spacer sequence. In PAUP^* analysis, Platycladus orientalis was used as the functional out group. By using the maximum likelihood method 1 077 trees were examined and the result showed that one tree had a best score of -Ln=2 232.47. The phylogenetic tree clearly showed that Chamaecyparis nootkatensis was diverged from other Chamaecyparis species. Based on the results, together with evidences from other aspects, we consider that Cupressus funebris and Chamaecyparis nootkatensis should be placed in the genus Cupressus. The use of cpDNA intergenic spacer petG-trnP in Cupressus was also discussed. __________ Translated from Journal of Sichuan University (Natural Science Edition), 2005, 42(5): 1033–1037 [译自: 四川大学学报 (自然科学版) 2005, 42(5): 1033–1037]