接种大豆根瘤菌(Sinorhizobium fredii)遗传工程菌株LMG101对大豆的增产效应

笔者曾报道带外源肺炎克氏杆菌 (Klebsiellapneumoniae)nifA的大豆根瘤菌 (Sinorhizobium fredii)工程菌株LMG10 1在实验室条件下具有较高的结瘤固氮效率 ,用其接种大豆幼苗可以提高大豆生物量。本项工作通过 3年的田间小区试验 ,对工程菌S .frediiLMG10 1的田间施用效果进行了研究。试验表明 ,接种工程菌S .frediiLMG10 1能有效地提高大豆的结瘤固氮效率和大豆产量。接种工程菌S .frediiLMG10 1的大豆植株固氮酶活力分别比对照和接种出发菌植株高 3.1倍和 2 .1倍 ,与之相应工程菌占瘤率也较高 ,大豆田间产量分别比对照和接种出发菌提高 10 %和 5 %以上 ,统计差异显著 (P <0 .0 5 )。

Proteome Analysis of Inhibitory Effect of Gadolinium on Sinorhizobium fredii

The inhibitory effect of gadolinium on Sinorhizobium fredii USDA 205 was studied on a global scale using twodimensional gel electrophoresis and MALDI-TOF MS. The results indicated that 22 proteins were significantly affected by 1 mmol · L^-1 Gd^3 ＋ treatment when compared with an untreated control. Among these proteins, nine were up-regulated and thirteen were down-regulated. The differently expressed proteins were classified into 8 functional categories based on their functions, including transporters, proteins for cellular defence, and proteins involved in metabolism.

三叶草素基因(tfx)在快生型大豆根瘤菌(Sinorhizobium fredii)H12-2中的表达与稳定性测定

将含有三叶草条基因的重组质粒pT2TFXK和pT2TX3K以接合转移的方式导入快生型大豆根瘤菌H12－2。转移接合子H12－2（pXK）能产三叶草素并具有抑菌活性；H12－2（P3K）表现出对三叶草素的抗性。抑菌谱试验结果表明：82％的供试快生型大豆根瘤菌菌株对三叶草素敏感；所有供试慢生型大豆根瘤菌则表现抗性。稳定性检测结果表明：在共生与人工培养条件下，导入的pXK和p3K质粒均可在宿主菌中稳定存在和表达。

费氏中华根瘤菌(Sinorhizobium fredii)质粒复制基因repC序列多样性的研究

采用质粒快速检测法从供试33株费氏中华根瘤菌中分别检测出2～4个内源大质粒.用根据豌豆根瘤菌的repC基因设计1对引物RC1和RC3,从供试菌株及3株华癸中生根瘤菌和1株大豆慢生根瘤菌中扩增得到repC基因片段,证明在费氏中华根瘤菌中广泛存在repC基因.通过对扩增产物的测序,并与已报道的repC基因序列进行聚类分析,发现供试菌株可分为2个群,群a和群b,群内十分保守,但群间差异明显;其中群b的序列与已知类型的差异明显.

费氏中华根瘤菌(Sinorhizobium fredii)的多样性研究

用大豆品种Willimas和黑龙 33从多年种植大豆未接种根瘤菌的土壤中捕集大豆根瘤菌 ,从分离株中选出 5 0株费氏中华根瘤菌 ,对供试菌株的培养特性、生长速度、耐酸、耐碱性、生长最终pH值、天然抗药性、CN源利用、刚果红吸收强度、产黑色素能力和质粒图谱类型进行了系统的比较研究 ,并通过聚类分析得到树状图谱 ,证实了不同土壤中费氏中华根瘤菌的多样性 .

湖北潜江灰潮土中费氏中华根瘤菌(Sinorhizobium fredii)多样性的研究

用5种代表性大豆为捕集植物从湖北潜江灰潮土中经盆栽试验分离筛选出50株费氏中华根瘤菌，对它们的生长速度、耐盐性、pH生长范围、天然抗药性、碳氮源利用和共生效应等同时进行了比较研究，证实了同一土壤环境中费氏中华根瘤菌群体的多样性。

Extra-copy nifA enhances the nodulation efficiency of Sinorhizobium fredii

Previous investigations have shown that nifA gene is involved in nodulation and symbiotic nitrogen fixation regulation of Rhizobium. We study the role of nifA on nodulation of leguminous plants. We found that Sinorhizo-bium fredii harboring multi-copy plasmid carrying the con-stitutively expressed Klebsiella pneumoniae nifA exhibited an increase of nodulation activity and nodulation competitiveness on soybean plants. The Nod-factor secreted by the rhizobia cells containing the multi-copied nifA was assayed, and preliminary results showed that S. fredii containing the multi-copy plasmid carrying nifA produced higher strength of Nod-factor than the rhizobia containing the same plasmid carrying the vector did.

Isolation and characterization of a Sinorhizobium fredii mutant that cannot utilize proline as the sole carbon and nitrogen source

Sinorhizobium fredii strain HN01 can use proline as the sole carbon and nitrogen source. A mutant strain GXHN100 unable to catabolize proline was screened from 6000 Tn5gusA5 random insertional mutants of S.fredii strain HN01. Sequencing analysis showed that an open read- ing frame, named pmrA (proline metabolic relative), was inserted by the Tn5gusA5. A positive clone, named pGXHN100 which containing 3.3kb foreign DNA fragment of S.fredii strain HN01, was isolated from a partial gene library of S.fredii HN01 by colony in situ hybridization. Sequence analysis showed that pGXHN100 contained the entire pmrA gene. The 3.3kb DNA fragment of pGXHN100 was cloned into a broad-host-range cosmid vector pLAFR3 to form plasmid pGXHN200 which was subsequently introduced into GXHN100 to form a complemented strain GXHN200. Plant test showed that GXHN100 was effective and no obvious changes in nitrogenase activity comparing with parental strain. But GXHN100 nodulated 2 days later on soybean and its nodulation efficiency and competitiveness were decreased. The complemented strain GXHN200 restored the nodulation efficiency and competitiveness of GXHN100 to the wild type.

A proteomic analysis of bacte-rial strain Sinorhizobium frediiRT19 subjected to salt shock

Sinorhizobium fredii RT19, a strain of free- living bacteria, was subjected to salt shock and its protein expression profiles were analyzed by differential display proteome approaches. The results of separation by two-dimensional polyacrylamide gel electrophoresis (2D PAGE) showed that the number of resolved proteins was 481, 465 and 424, corresponding to salt-free control, 5 and 50 min 1 mol/L salt treatment, respectively. Among the resolved proteins, 82 in total had altered expression in response to salt-shock stress. 26 out of the 82 proteins were induced and 23 were completely inhibited, while 12 were up-regulated and 21 down-regulated in response to salt shock. In addition, the appearance of differentially displayed proteins responding to different salt shock periods is also reported. The identity of the 26 induced proteins was revealed by matrix assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF/MS) followed by database searching. Among them, 20 were assigned to proteins with known functions. Their roles in response to salt shock stress are discussed.

根瘤菌TtsI突变对大豆根瘤菌固氮酶活性的影响及转录组分析

根瘤菌与大豆建立的共生模式为大豆提供了生长发育所必须的氮素,在共生建立时根瘤菌Ⅲ型效应因子是影响结瘤发生的重要信号分子之一。为了解析根瘤菌Ⅲ型效应因子在结瘤中的作用,进行TtsI突变根瘤菌HH103(Sinorhizobium fredii HH103)结瘤鉴定以及根瘤转录组分析,并对差异基因进行富集分析。结果显示:TtsI突变可以降低绥农14根瘤的固氮酶活性,但不影响野生豆ZYD00006的根瘤固氮酶活性。TtsI突变根瘤菌HH103(HH103ΩTtsI)使绥农14根瘤内部分编码氮转运的相关基因以及NLP7下调表达,并且接种HH103ΩTtsI与接种HH103相比,Glyma.11G235200和NLP7在ZYD00006的根瘤中的相对表达没有显著差异。通过GO富集、KEGG富集以及GSEA富集分析显示,差异基因主要涉及信号传导以及代谢进程等,差异基因主要在植物激素信号传导以及MAPK信号通路上富集。研究结果为后续Ⅲ型效应因子的功能和机制的解析以及大豆高效固氮设计提供了新的思路;同时氮转运相关基因的表达差异可为进一步选育高结瘤、高固氮效率以及高氮利用率的大豆品种提供理论支撑。

豌豆根瘤菌共生基因在S.fredii中的表达及共生质粒间的相互作用

通过两亲本接合转移 ,将豌豆根瘤菌 ( Rhizobium leguminosarum bv. viciae) 12 2 9的约 2 5 5 0 kb的共生质粒 p Sym12 2 9分别转入费氏中华根瘤菌 ( Sinorhizobium fredii) HN0 1SR及其消除了共生质粒的菌株 HND10 0中 .在人工培养条件下 ,用 1 4C标记的薄层层析 ( TL C)技术检测转移接合子的结瘤因子 ( L COs)的结果表明 ,转移接合子 HND10 0 ( p Sym12 2 9)产生的 L COs与豌豆根瘤菌 12 2 9相同 .植物盆栽结瘤试验结果表明 ,HND10 0( p Sym 12 2 9)能够在豌豆品种 Nigra上形成白色球状的无效根瘤 ,而豌豆根瘤菌 12 2 9则形成正常的长圆柱状的有效根瘤 .将 p Sym 12 2 9转入 HN 0 1SR后 ,部分接合子表现出与 HND10 0 ( p Sym 12 2 9)相同的结瘤性状 ,而另一部分接合子的结瘤性状与 HN0 1SR相同 ,显示了 HN0 1SR与 12 2 9两菌株异源共生质粒之间结瘤功能的抑制关系 .

S.fredii WGF03 SiR基因的功能鉴定

亚硫酸盐还原酶催化亚硫酸盐还原为硫化物，参与了生物硫循环。为了明确亚硫酸盐还原酶在S船捌WGF03中是否与亚硫酸盐同化途径有关，通过分子克隆技术，采用同源双交换的方法，利用质粒pKl8mobsaeB构建SiR基因缺失突变体SiRI。用不同硫源的液体MM培养基培养检测，发现互补菌株CSiRI与野生型菌株能够利用亚硫酸盐作为唯一硫源，而突变体SiRI却不能，结果证实了亚硫酸还原酶确实与亚硫酸盐同化途径有关。植株试验表明突变株SiRI比野生菌株WGF03推迟结瘤2～3d，固氮酶活比野生菌株低12％左右，但在瘤数，瘤重，植株干重的平均值却差异不大。

根瘤菌HH103ΩNopAA/T/C三重突变体构建及结瘤表型鉴定

为提高豆科-根瘤菌共生固氮的效率,研究中华根瘤菌HH103菌型各效应因子突变体对大豆结瘤的影响,以其效应因子NopAA、NopT和NopC为研究对象,采用三亲杂交的方法获得突变体HH103ΩNopAA/T/C,PCR鉴定后,以绥农14为材料进行结瘤表型分析,发现突变体HH103ΩNopAA/T/C可以影响大豆结瘤数量以及结瘤重量,但对瘤大小没有明显影响;降低平均结瘤数和瘤鲜重干重,与突变体HH103ΩNopC有显著差异。上述结果说明效应因子NopAA、NopT和NopC相互调控,在大豆-根瘤菌共生体系建立过程中发挥重要作用。

pH对土壤中土著快、慢生大豆根瘤菌结瘤的影响

The effect of pH on the nodulation of Sinorhizobium fredii and Bradyrhizobium japonicum was examined by analy- zing the indigent soybean rhizobia,predominant indigent rhizobia,and specific rhizobia,respectively.The results showed that very acid and very alkaline environment could retard the nodulation and inhibit the growth of the rhizobia.Sinorhizohium fredii could endure environment more strongly than Bradyrhizobium japonicum,and had a high competitive nodulation capacity.Bradyhizobium japonicum could endure acid environment more strongly than Sinorhizobium fredii.In very acid and very alkaline environment,the nodulation capacity of S.fredii and B.japonicum was mainly determined by their physiological characteristics.

一株能在苜蓿上结瘤的费氏中华根瘤菌

费氏中华根瘤菌 (Sinorhizobiumfredii) 0 4 2BS分离自新疆的苜蓿根瘤 ,通过交叉结瘤试验 ,发现它既可在苜蓿上又可在大豆上结瘤固氮。 1 6SrDNAPCR RFLP分析表明 ,0 4 2BS与费氏中华根瘤菌模式菌株USDA2 0 5的 4种限制性酶切图谱完全一致。其G +Cmol%为 60 0 ,与费氏中华根瘤菌USDA2 0 5和USDA1 91的DNA同源性分别为 84 9%和89 6% ,表明 0 4 2BS属于费氏中华根瘤菌。应用绿色荧光蛋白基因标记 0 4 2BS ,得到重组菌株 0 4 2BSG。将其接种保定苜蓿和北引 1号大豆 ,并重新分离出根瘤菌 ,利用激光共聚焦荧光显微镜检测到标记基因的表达 ,从而确证了 0 4 2BS能在苜蓿和大豆上结瘤。而且 ,0 4

以绿荧光蛋白基因为报告基因的广宿主启动子探针载体的构建和应用

将以绿荧光蛋白基因（ ｇｆｐ） 的ｃＤＮＡ 为模板，用人工合成引物经ＰＣＲ 扩增获得的０－９ｋｂＤＮＡ 片段克隆到表达载体ｐＥＴ１１Ｃ 上构建成ｇｆｐ 表达载体ｐＨＮ１１５ 。从ｐＨＮ１１５ 上切下的不含启动子，但保留了ＳＤ 序列的ｇｆｐ 基因经克隆载体ＳＫ（ ＋ ） 和ｐＩＪ２９２５ 亚克隆后再克隆到广谱稳定性质粒ｐＴＲ１０２ 上构建成广谱、稳定、可视的启动子探针载体ｐＨＮ１２７ 。并用它从费氏中华根瘤菌ＨＮ０１ 的总ＤＮＡ 中成功地钓出组成型和诱导型表达的启动子。

费氏中华根瘤菌与耐盐有关基因的克隆及其在大肠杆菌中的表达

费氏中华根瘤菌（Ｓｉｎｏｒｈｉｚｏｂｉｕｍ ｆｒｅｄｉｉ）ＲＴ１９与耐盐有关的４．４ｋｂ ＤＮＡ片段含有３个相间的开放阅读框，经亚克隆及功能检测，证实其中的ＯＲＦ２与耐盐有关。将ＯＲＦ２分别克隆到表达载体以ｐＴＨｉｏＨｉｓＡ、Ｂ和Ｃ上，得到３个重组质粒ｐＧＡ、ｐＧＢ和ｐＧＣ，转化大肠杆菌（Ｅｓｃｈｅｒｉｃｈｉａ ｃｏｌｉ）ＤＨ５α。经ＩＰＴＧ诱导后和作ＳＤＳ－ＰＡＧＥ分析，发现只有ｐＧＣ编码的融合蛋白获得了表达。其分子量为５３ｋＤａ，恰好是ｔｒｘＡ基因编码的硫氧还蛋白与推测的蛋白质分子量之和。Ｗｅｓｔｅｒｎ印迹证实，表达的蛋白质是ｔｒｘＡ基因和目的基因编码的。

16株快生型大豆根瘤菌生物学与分子生物学特性的比较研究

以快生型大豆根瘤菌标准菌株ＵＳＤＡ２０５为对照，对自我国吉林省和湖北省土壤中分离的１５株快生型大豆根瘤菌的培养特性，碳氮源利用、生长速度、耐盐性、ｐＨ适应范围、天然抗药性、质粒图谱、Ｇ＋Ｃ克分子％、血清学特性和共生固氮效率进行了系统的比较研究。

导入四碳二羧酸转移酶基因对费氏中华根瘤菌共生固氮效率的影响

将来自苜蓿中华根瘤菌 (Sinorhizobiummeliloti)的四碳二羧酸转移酶基因(dctABD)经 pIJ2 92 5克隆到广宿主、稳定性质粒 pTR10 2上 ,获得诱导型表达的重组质粒 pHN2 0 2。在此基础上再引入来自 pDB30所含的发光酶基因 (luxAB)作分子标记 ,以 pTR10 2为基础构建成带有dctABD和luxAB的重组质粒 pHN2 0 5。经三亲本接合转移 ,将重组质粒 pHN2 0 5导入费氏中华根瘤菌 (Sinorhizobium fredii)HNO1,GR3和YC4。与出发菌相比较的盆栽试验结果表明 :HN0 1(pHN2 0 5)和GR3(pHN2 0 5)分别在宁镇一号和川早一号大豆上能显著提高植株地上部分干重 (生物量 )和总氮量 ,YC4 (pHN2 0 5)在黑龙 33大豆上能同时显著提高植株地上部分干重 (生物量 ) ,总氮量和根瘤鲜重。本研究结果表明 :导入dctABD基因对共生固氮效率的增效性与受体根瘤菌和大豆品种等因素有关。以luxAB为报告基因进行的转移接合子培养条件下分离单菌落和共生条件下形成根瘤的发光活性检测结果表明 :pHN2 0 5可在供试费氏中华根瘤菌中稳定遗传。

低湿耕地综合治理对土壤微生物生态影响及大豆增产的研究

本文报道了三江平原低湿耕地综合治理后对土壤微生物生态的影响及对大豆增产的明显效果。4年来开发试验研究的结果表明,低湿耕地经过综合治理并栽培大豆等作物以后,土壤中大豆根瘤菌数量及自生固氮菌的数量明显增加;低湿耕地综合治理后接种高效固氮大豆根瘤菌,经配对选优及结合施用启动氮的高光效高固氮大豆-根瘤菌共生固氮体系的生物技术措施,使大面积的大豆增产12.3％,达到接近岗平地耕作条件下生物技术措施的水平,对今后的生产实践或科学理论都具有重要意义。