专一性脱硫菌的鉴定及高DBT降解力菌株的选育

从大庆油田土壤中分离得到1株可降解二苯并噻吩(DBT)的脱硫微生物HDBS-1,对该微生物的种属地位进行了鉴定并通过诱变手段提高了该菌株的脱硫能力。经过形态观察、生理生化特征分析及16S rDNA序列测定发现该微生物为坂崎肠杆菌(Enterobacter sakazakii),该菌种可以按特异性脱硫途径(简称4S途径)将DBT转化为2-羟基联苯(2-HBP)。利用紫外线(UV)、硫酸二乙酯(DES)和UV+DES对该菌株复合诱变后,得到菌株HDBS-4,其降解DBT生成2-HBP的能力得到了极大的提高,发酵液中2-HBP生成含量(2.574 mg/L)较原始菌株(0.434 mg/L)提高了5.93倍。     

脱硫菌Fds-1的分离鉴定及其对柴油脱硫特性的研究

从含硫土壤中分离筛选出一株专一性脱硫菌Fds-1,经生理生化指标和16S rRNA序列分析鉴定其属于枯草芽孢杆菌(Bacillus subtilis)。用Gibb’s试剂显色和气相色谱-质谱联用分析表明,该菌株通过“4S”途径脱除有机硫。实验发现Fds-1的最佳脱硫活性在30℃,在此温度下72h内能脱除约0.5mmol/L DBT中的有机硫。Fds-1菌株对有机硫化合物的利用情况和柴油脱硫前后烃组分比较都进一步证明该菌株适合于柴油生物脱硫。利用休止细胞对不同组分柴油的脱硫研究表明,脱硫菌株Fds-1对精制柴油中的DBT类化合物的降解能力强。因此,该菌株对精制低硫柴油的深度脱硫具有应用意义。     

一株高耐镉硫酸盐还原菌的分离及脱硫性能研究

本研究从镉污染稻田水稻根际土壤中分离、纯化出一株硫酸盐还原菌SRB1-1,并对该菌株的生理生态特征、镉和盐耐受性、16S rDNA、脱硫性能及影响因子进行了系列分析。结果表明,该菌为革兰氏阴性菌,菌体弧状,对镉离子的耐受浓度可达200 mg/L,在2%的氯化钠浓度下仍可生长。对其16S rDNA的序列分析表明该菌株属于脱硫弧菌属(Desulfovibrio)。单因子实验考察温度、pH及SO_4~(2-)浓度对该菌脱硫效率的影响,正交实验确定了该菌最佳脱硫工艺条件及影响因子顺序。结果表明最佳脱硫工艺条件为pH 7.5、温度40℃、SO_4~(2-)浓度为1 000 mg/L、培养时间56 h。     

石油生物催化脱硫菌Agrobacterium tumefaciens UP3的分离筛选

从胜利油田被原油污染的土壤中筛选到一株能有效降解模型化合物二苯并噻吩(DBT)的菌株.根据常规的形态分析、生理生化性状及16S rDNA序列分析,将其鉴定为根癌土壤杆菌(Agrobacterium tumefaciens UP3).该菌不能以十二烷、十六烷、液体石蜡和萘作为唯一碳源和能源生长,具有工业应用的潜力.对该菌株DBT降解能力的初步研究表明,54h内可将500mg/L的DBT降解至150mg/L.对降解产物的分析表明,根癌土壤杆菌降解DBT的途径与Kodama路线及4-S路线不同.     

一株脱硫自养菌的鉴定和脱硫特性研究

从无锡市某硫酸厂采集的土样中分离到一株具有脱硫性能的自养菌, 对该细菌的16S rDNA序列进行了测定, 并根据16S rDNA构建了系统发育树, 结合菌落、细菌形态鉴定菌株为那不勒斯硫杆菌(Thiobacillus neapolitanus), 命名为TL-1。同时, 考察了TL-1菌株在不同温度和pH条件下的脱硫效率, 并在反应器中以氧化还原电位(ORP)为控制条件, 对菌株的脱硫效果和生成的单质硫颗粒特性进行了研究, 结果表明, 摇瓶实验中, 30°C、pH 7.5为脱硫最佳条件。反应器运行时, ORP控制在-370 mV条件下运行效果最佳, 系统能够维持95%以上的硫化物去除率和85%以上的单质硫回收率, 随着ORP的增大, 生成的单质硫颗粒粒径有逐渐增大的趋势。     

内蒙古碱湖中紫色非硫光合细菌的分离和鉴定

从内蒙古碱湖水样中分离得到一株紫色非硫光合细菌,命名为JH1-6.对该菌株进行了形态学观察、生理生化鉴定、活细胞吸收光谱以及16S rDNA序列分析.16S rDNA序列分析结果表明该菌株与沼泽红假单胞菌的16S rDNA序列同源性高达99%,结合形态特征和生理生化特性以及活细胞吸收光谱特征等,确定菌株JH1- 6在分类地位上属于沼泽红假单胞菌(Rhodopseudomonas palustris).     

一株基因克隆干扰菌的鉴定及其发酵液降解DNA活性分析

旨在寻找导致基因克隆失败的原因,检测整个电泳环境中是否存在对DNA有强降解力的菌株。依据菌体形态,革兰氏反应以及16S rDNA序列对DNA降解菌株进行鉴定,琼脂糖凝胶电泳分析菌株对DNA的降解活性。结果显示,从DNA电泳槽中分离到了一株菌,革兰氏染色鉴定为阴性菌,对该菌进行液体培养,利用质粒pUC19作为底物,检测该菌发酵液对DNA的降解能力,发现该菌发酵液能够迅速并彻底地降解DNA,其最佳降解温度为45℃,将该菌命名为DD(DNA degrading)。对该菌的16S rDNA进行测序比对后,发现其与粘质沙雷氏菌(Serrtia marcescens)的16S rDNA序列同源性高达100%。结合菌体形态,革兰氏反应以及16S rDNA序列结果,DD菌株为一株粘质沙雷氏菌,DNA降解活性分析显示其具有很强的DNA降解能力。     

一株新的胡萝卜软腐欧文氏菌的分离和鉴定

从大白菜软腐组织中分离出一株软腐病细菌BC1,经过形态观察、生理生化特性分析、致病性检测和16S rDNA序列分析,该分离物被鉴定为胡萝卜软腐欧文氏菌胡萝卜亚种（Erwinia carotovora subsp. carotovora, Ecc）的一个新菌株,编号为BC1。这是首次从16S rDNA序列水平上对在我国分布的软腐欧文氏菌进行鉴定。Ecc BC1的16S rDNA序列与其它软腐欧文氏菌株的16S rDNA序列之间同源性达987%～993%,而且在系统发育树中独立于Ecc其它菌株。序列分析结果表明,Ecc BC1具有至少2种不同的16S rDNA序列,它们都在第459位和473位（相对于大肠杆菌16S rDNA序列）发生碱基突变,同一基因中两个突变位点之间彼此互补,处于16S rRNA螺旋H17颈部,而且这两处碱基变异只存在于BC1菌株中。通过与其它软腐欧文氏菌亚种和菌株16S rDNA序列进行比对分析,还进一步鉴定出一些BC1菌株特异的16S rDNA碱基突变位点。本文报道的Ecc BC1两个16S rDNA序列在GenBank中的登录号分别为AY309068和AY309069。     

石油生物催化脱硫菌Agrobacterium tumefaciens UP3的分离筛选

从胜利油田被原油污染的土壤中筛选到一株能有效降解模型化合物二苯并噻吩（DBT）的菌株。根据常规的形态分析、生理生化性状及16S rDNA序列分析,将其鉴定为根癌土壤杆菌（Agrobacterium tumefaciens UP3）。该菌不能以十二烷、十六烷、液体石蜡和萘作为唯一碳源和能源生长,具有工业应用的潜力。对该菌株DBT降解能力的初步研究表明,54h内可将500mg/L的DBT降解至150mg/L。对降解产物的分析表明,根癌土壤杆菌降解DBT的途径与Kodama路线及4_S路线不同。     

红球菌SDUZAWQ对有机硫和无机硫的耐受性研究及脱硫基因的克隆

以筛选得到的红球菌SDUZAWQ为对象,研究其在不同浓度的有机硫化合物二苯并噻吩(DBT)存在下的脱硫能力,以及在0.2mmolLDBT和不同浓度Na2SO4同时存在下的脱硫情况。当DBT浓度高达6mmolL时,菌株仍能生长,而且检测出产物2-羟基联苯(2-HBP)的存在,说明该菌株具有耐受较高浓度DBT的能力。当DBT和Na2SO4同时存在时,DBT为菌株SDUZAWQ所利用,并且也检测出2-HBP,并非如文献所报道的红球菌在无机硫存在下不代谢DBT,表明该菌株能够耐受一定浓度的无机硫酸盐。对相关脱硫基因的克隆和测序结果显示,完整脱硫基因dszABC、其上游调控序列和dszD的序列与模式菌株RhodococcuserythropolisIGTS8的同源性分别是99%、100%和100%。     

Sulfur-selective desulfurization of dibenzothiophene and diesel oil by newly isolated Rhodococcus sp. strains

New desulfurizing bacteria able to convert dibenzothiophene into 2-hydroxybiphenyl and sulfate were isolated from contaminated soils collected in Mexican refineries. Random amplified polymorphic DNA analysis showed they were different from previously reported Rhodococcus erythropolis desulfurizing strains. According to 16S rRNA gene sequencing and fatty acid analyses, these new isolates belonged to the genus Rhodococcus. These strains could desulfurize 4,6-dimethyldibenzothiophene which is one of the most difficult dibenzothiophene derivatives to remove by hydrodesulfurization. A deeply hydrodesulfurized diesel oil containing significant amounts of 4,6-dimethyldibenzothiophene was treated with Rhodococcus sp. IMP-S02 cells. Up to 60% of the total sulfur was removed and all the 4,6-dimethyldibenzothiophene disappeared as a result of this treatment.     

抗草甘膦转基因大豆PCR检测及问题探讨

转基因植物的检测具有重要的意义。用抗草甘膦转基因大豆中的外源CaMV35S启动子、CP4 EPSPS和巢式PCR引物,应用PCR方法,从中扩增出预期大小的DNA片段。将扩增产物回收后测序,经同源性分析扩增产物为CaMV35S启动子和CP4 EPSPS的一部分序列。与常规PCR相比,巢式PCR在检测转基因大豆中具有更高的特异性。讨论了PCR检测过程中假阴性和假阳性的原因。     

北戴河海洋沉积物中L-半胱氨酸脱硫细菌的多样性及其特性

【背景】脱硫细菌对有机硫的脱硫作用在硫的生物地球化学循环以及脱硫工业中都起着重要的作用。【目的】了解海洋沉积物中可分解有机物产生硫化氢的细菌多样性。【方法】对我国北戴河海洋沉积物中可培养的L-半胱氨酸脱硫细菌进行分离与筛选,通过对其16SrRNA基因序列测定与分析,构建系统发育树,并对其脱硫、脱氮能力进行检验。【结果】从海洋沉积物中分离得到97株细菌,从以L-半胱氨酸为硫源的培养基中筛选出62株有机脱硫专一型细菌。根据脱硫细菌的形态及其特征,从中选取12株作为典型代表做进一步分析,它们分别属于芽孢杆菌属(Bacillus)、赖氨酸芽孢杆菌属(Lysinibacillus)、动性球菌属(Planococcus)和红球菌属(Rhodococcus)。结果表明,这12株细菌均可产生半胱氨酸脱巯基酶,能够将半胱氨酸分解为丙酮酸、硫化氢和氨,即同时具备脱硫与脱氮的能力。其中有5株菌脱硫能力较强,分别属于赖氨酸芽孢杆菌属、动性球菌属和芽孢杆菌属。【结论】海洋沉积物中存在着丰富的L-半胱氨酸脱硫细菌,为进一步研究海洋中硫的生物地球化学循环提供了素材。     

S16, a novel S-RNase allele in the diploid species Solanum chacoense.

Wild potato species have a gametophytic self-incompatibility system controlled by a single multiallelic S locus. In the style, the S-RNase gene codes for an allele-specific ribonuclease that is involved in the rejection of pollen that carries the same S haplotype. This gene has 5 conserved regions (C1-C5) and highly variable regions outside of these areas that play a role in S-RNase allele specificity. In this work, PCR-mediated amplification of genomic DNA from 2 Solanum chacoense accessions was performed using primers designed on the basis of the C1 and C4 conserved regions. By sequencing the PCR products, a new S-RNase allele (S16) was identified in 1 plant of the QBCM argentinian accession. Comparison of the partial sequence (from C2 to C3) of S16 RNase with those of 11 S-RNase genes of other Solanaceae species showed the highest and the lowest similarity scores within the same plant species (respectively, 71% with the S11 and S13 RNase and 35% with the S2 RNase). Differences at the nucleotide level between S16 and S11 RNase alleles are discussed.     

Development of broad-spectrum insect-resistant tobacco by expression of synthetic cry1Ac and cry2Ab genes

Efficacy of two newly synthesized cry1Ac and cry2Ab genes was checked in tobacco before their expression in cotton. Both genes were artificially synthesized and codon optimized with respect to cotton-preferred codon usage. These genes were cloned in a plant expression vector and then transformed into tobacco. Fifty-eight putative transgenic plants were recovered from the selected explants. Successful integration of both genes in plant genome was confirmed by PCR amplification. Expression of transgenes was confirmed by PCR amplification from total plant RNA. Detached leaf insect bioassays were conducted with Helicoverpa armigera and Spodoptera exigua larvae. About 12 % of the transgenic plants showed significantly high resistance to S. exigua. Significant mortality (62 %) of H. armigera was recorded within 24 h of bioassays. Both toxins showed synergistic effect in tobacco and broadened the spectrum of plant activity against insects.     

酿酒酵母海藻糖—６—磷酸合成酶基因克隆及植物表达载体的构建

从耐热性极强的酿酒酵母菌株ＡＳ２．１４１６中分离纯化出总ＲＮＡ和mRNA,以ＡＭＶ逆录酶合成cDNA,采用保守引物,从该cDNA中扩增克隆出tps1基因,对该基因的全序列分析表明,该基因含有１５０７个核苷酸,与国外报道相关基因的同源性达９９．６５。利用ＢamＨⅠSacⅠ切点将tps1基因插入植物表达载体pBin438多克隆位点上,得到tps1基因植物表达载体重组质粒。     

番茄叶片胞壁转化酶cDNA克隆及反义沉默表达分析

参考GenBank登录的植物胞壁转化酶基因序列,设计1对PCR引物,以番茄(‘中蔬四号’)叶片总RNA的反转录产物为模板,扩增出长为416bp的cDNA片段,Blast结果表明,其为番茄胞壁转化酶基因LIN6片段;将其反向插入双元载体pBinAR的CaMV 35S启动子和OCS终止子间,构建反义植物表达载体pBinAR-aLIN6。通过农杆菌EHA105介导转化番茄MicroTom,PCR和Southern斑点杂交检测表明,共获得5株转基因番茄;生化检测表明,5个转化植株叶片胞壁转化酶活性分别比未转化植株下降67.9%、13.4%、73.5%、85.6%和58.0%。     

Theoretical and Practical Approaches to Evaluate Suitable Primer Sets for the Analysis of Soil Fungal Communities

Six published fungal specific primer sets (NS1/NS2, SSU‐0817/SSU11‐96, SSU‐0817/SSU‐1536, EF4/EF3, EF4/fung5 and FR1/FF390) were examined for their applicability to the analysis of soil fungal communities using bioinformatic tools as well as real PCR systems. Virtual primer matching for EF4/EF3 and EF4/fung5 revealed good matching with zygomycetous, ascomycetous and basidiomycetous 18S rDNA database entries. Whereas primer EF4/EF3 had no cross matches in the rDNA databases for plant and invertebrate, primer EF4/fung5 gave one signal with the corresponding database. Similar results were obtained for the primer set SSU‐0817/SSU‐1536. Two matches with plant rDNAs and 22 or 12 matches with the invertebrate database could be identified for the primer sets SSU‐0817/SSU‐1196 and FR1/FF390, respectively. Primer pair NS1/NS2 showed only a 70% match with fungal 18S rDNA sequences, but a 75% to 90% match with non‐fungal sequences. Alignments of 2000 eukaryotic sequences using “ARB” confirmed that PCR fragments obtained by the primer sets EF4/EF3, EF4/fung5, SSU‐0817/SSU‐1536 and FR1/FF390 were supposed to include hypervariable regions (V4, V7, V9), whereas the others included regions which were more phylogenetically conserved. Practical PCR approaches affirmed fungal specificity as predicted by virtual primer matching for EF4/EF3, EF4/fung5 and FR1/FF390. However FR1/FF390 amplified only 60% of the fungal samples under investigation. All other primer sets amplified fungal as well as non‐fungal samples.     

Development of group-specific PCR-DGGE fingerprinting for monitoring structural changes of Thauera spp. in an industrial wastewater treatment plant responding to operational perturbations

A Thauera-specific nested-PCR denaturing gradient gel electrophoresis (DGGE) method was developed, and its usefulness was demonstrated by monitoring the structural shifts of Thauera spp. in an anaerobic-anoxic-oxic fixed-biofilm coking wastewater treatment plant (WWTP) responding to operational perturbations. The specificity of the PCR method was confirmed by the fact that all 16 S rRNA gene sequences, cloned from the amplicons of a biofilm sample, belonged to Thauera genus. 16 S rRNA gene V3 region was then amplified from the first round Thauera-specific PCR product and applied for DGGE analysis. All Thauera clones, with 13 different V3 regions, migrated into 10 positions on DGGE gel, which demonstrated the high resolution of this DGGE method. When the WWTP experienced a gradual deterioration in chemical oxygen demand (COD) removal function due to a mechanical failure of the recirculation pump, biofilm samples were collected from the reactor and analyzed by this method. Principal component analysis (PCA) of the DGGE fingerprinting data showed that the composition of Thauera group exhibited a time related trajectory when the plant's COD removal rate decreased from 84.1+/-2.7% in the first 4 weeks to less than 75% at week 5 and 6, suggesting a concomitant shift of Thauera composition and the system's COD removal function. This group-specific PCR DGGE fingerprinting technology has the potential to be a profiling tool for monitoring structural shifts of Thauera spp. in industrial WWTPs.