激发子基因peaT1转化三生烟及其对TMV抗性的提高

通过根癌农杆菌(Agrobactrium tumefaciens)介导转化法,将含有激发子基因peaT1的植物表达载体pCAM-BIA2300-G4AS-peaT1转化三生烟,获得了转基因烟草植株。用PCR检测确认了阳性转化株,用Southern杂交、RT-PCR和Western杂交进一步证实了peaT1基因的整合、转录和表达。对T1代转基因阳性株进行TMV接种试验,结果显示,与非转基因对照相比,表达peaT1的烟草叶片枯斑数量减少,表明蛋白激发子基因peaT1的表达提高了转基因烟草对TMV的抗性。     

转popW基因烟草的构建及相关表型分析

PopW是克隆于青枯劳尔氏菌Ralstonia solanacearum ZJ3721中的一种新的编码harpin蛋白的基因,原核表达的PopW蛋白能够诱导烟草对TMV的抗性、促进烟草生长、提高烟草品质。将popW基因连接到植物表达载体pBI121上,构建成重组转基因载体pB-popW,通过冻融法转化根癌土壤杆菌EHA105,获得阳性转化子。再采用叶盘法转化三生烟Nicotiana tobacum cv.Xanthi nc.,经卡那霉素抗性筛选、PCR检测、RT-PCR分析获得21个株系的T3代阳性植株。PCR及RT-PCR检测结果表明popW基因已经整合到烟草基因组中,并在转录水平正常表达。GUS染色进一步证明popW基因在翻译水平上进行了表达,且不同株系之间表达存在差异。对烟草花叶病毒(TMV)的抗病性测定结果表明,转基因烟草对TMV的抗病性增强,防效最高达54.25%。转基因烟草在生长上也具有一定优势,生长15 d的根长最高为野生型的1.7倍,移栽后60 d的株高、鲜重、干重最高分别为野生型烟草的1.4、1.7和1.8倍。     

转望江南核糖体失活蛋白基因cassin烟草及其对烟草花叶病毒的抗性

通过构建植物表达载体,由农杆菌介导,将望江南核糖体失活蛋白基因cassin转入烟草。PCR和Southern blot杂交结果证明：外源基因已经以单拷贝整合到烟草基因组内,并且在后代发生遗传分离。RT—PCR和Northern blot杂交结果显示：外源基因可以正常转录。用不同浓度的TMV机械摩擦接种转基因T1、T2代各3个自交株系,以非转基因烟草为阴性对照,实验结果表明转基因烟草对TMV表现出不同程度的抗性。     

桃蚜MpAChE基因RNAi表达载体构建及转化

通过害虫取食植物表达害虫发育关键基因dsRNA的转基因植株,分析能否通过抑制害虫特定基因的表达来防控害虫。本研究利用RT-PCR技术从桃蚜中克隆乙酰胆碱酯酶基因383 bp cDNA片段,命名为MpAChE。进一步利用该MpAChE基因片段构建植物RNAi表达载体RNAi-MpAChE,并通过浸花法转化野生型拟南芥,通过卡那霉素抗性筛选转化植株,PCR及Southern杂交进一步鉴定转基因植株。结果表明:克隆的cDNA片段与桃蚜中已克隆的乙酰胆碱酯酶(GenBank登录号AY147797)cDNA序列核苷酸一致性为99%。卡那霉素抗性初步筛选和PCR进一步鉴定,获得25株阳性转基因植株。从25株中随机选择的5株阳性植株,Southern杂交均为阳性。经接种桃蚜初步鉴定,转基因植株对蚜虫的抗性效果不显著。     

表达多肽抗生素apidaecin的转基因烟草及其抗病性的初步分析

将多肽抗生素apidaecin基因与病程相关蛋白的信号肽序列融合,构建了apidaecin的分泌型植物表达载体、apidaecin与另一多肽抗生素Shiva\|I的双价分泌型植物表达载体,以本实验室原来构建的Shiva-I分泌型植物表达载体做对照,转化了模式植物烟草。对3种转基因植物进行了分子检测,转化再生苗95%为PCR阳性,Southern杂交结果进一步证明外源基因已经整合到了烟草基因组中,RT-PCR检测表明外源基因可以在转基因烟草内正常转录。对T0代转基因烟草进行烟草野火病的抗病性实验,从3种转基因烟草中都得到了抗病植株,病情指数分析的初步结果显示,双价转基因烟草抗病性最好,apidaecin的次之,Shiva-I的最差。     

大豆Lea5基因过表达提高烟草抗旱和耐盐性的研究

大豆Lea5基因是LEA基因家族成员之一。为分析大豆Lea5基因的功能,构建了大豆Lea5基因植物过表达载体p BI121-Lea5。通过农杆菌介导法转化烟草,获得TL-06、TL-09、TL-17和TL-32等4个转大豆Lea5基因烟草株系。RT-PCR分析表明大豆Lea5基因在4个转基因烟草株系的T2代植株均有不同程度的表达。以转基因TL-09和TL-32株系T2代植株为材料,进行了干旱和盐渍处理,结果表明,2个转大豆Lea5基因烟草株系T2代植株对干旱和盐渍的抗性显著强于野生型烟草,说明大豆Lea5基因可以提高植物抗干旱和盐碱的能力。     

cryIAc基因在转基因玉米中的遗传规律及对抗虫性影响

旨在研究目的基因在转基因植株和后代植株(株系)中的遗传规律及其对转化植株抗虫性的影响。以花粉介导法将cryIAc基因导入玉米自交系‘郑58’和‘昌7-2’,对转化植株及其后代株系进行分子检测和田间抗虫鉴定。结果表明:(1)转化‘郑58’和‘昌7-2’,T1代分别获得转基因植株24和41个,转化率高达20%以上;(2)转基因T2代、杂交F2代及回交1代(B1)的分子检测结果证明,外源基因的遗传符合孟德尔的3∶1、3∶1和1∶1的遗传分离规律;(3)连续多带的分子检测结果还表明,外源基因可稳定遗传并有效表达,表达水平在9.8-14.3 ng/g叶片鲜重之间;(4)抗虫鉴定结果显示,在阴性对照全部感虫情形下,转基因纯合株系仍表现出较高抗虫活性;(5)此外,回交试验结果还证明外源基因通过杂交可传递给下一代;(6)最终经筛选得到SZ003、SZ005、SC001、SC004和SC007五个高抗虫转基因株系。结果表明,花粉介导法是一种高效、快捷的转化方法,cryIAc基因导入玉米自交系植株后赋予和提高了转基因植株的抗虫活性。     

毛头鬼伞真菌具有抗烟草花叶病毒活性的y3基因的克隆及对烟草的转化

【目的】蛋白质Y3具有抗烟草花叶病毒(TMV)活性并由y3基因编码。本文的目的是从真菌毛头鬼伞(Coprinus comatus)中克隆y3基因全长并在植物体中展现其对TMV的抑制活性。【方法】我们利用试剂盒5′-Full RACE Core Set(TaKaRa)扩增了y3基因cDNA5′-端未知序列,通过RT-PCR获得了全长序列,并把该全长序列与CaMV 35 S启动子和NOS终止子一起插入多克隆位点(MCS)构建了植物表达载体pCAMBIA1301-y3,用于农杆菌介导的烟草转化。【结果】y3基因全长534碱基对,包含1个开放阅读框(ORF),编码一条含130个氨基酸残基的肽链(GenBank检索号:GQ859168;EMBL:FN546262)。其cDNA序列和由它推到的氨基酸序列均与已发表的y3基因部分片段有高度相似性(94%)。Northern杂交分析证实了y3基因在转基因烟草中得到表达。接种TMV的转基因植株表现出抗TMV的活性。【结论】我们克隆了y3基因全长并得到了转基因植株。在转基因植株中,由于y3基因的表达改善了植株的抗病毒活性。y3基因的克隆和表达无疑为该基因的进一步研究奠定了基础。     

转双价抗虫基因大白菜新种质的获得及其抗虫性分析

采用超声波辅助花粉介导方法,将双价抗虫基因BmkIT-Chitinase导入早熟型大白菜自交系20-19-3,最终获得了5个转基因大白菜优良自交系纯合株系Z1-5、Z2-7、Z9-6、Z11-6和Z20-13;以转基因大白菜株系和非转基因对照植株为材料,对BmkIT-Chitinase基因在大白菜中的遗传规律、基因表达及抗虫性进行进一步分析。结果显示:(1)转化株后代多代(T_1~T_4)PCR、Southern blotting等分子跟踪检测表明,目的基因已成功导入受体植株,且能够稳定遗传;用该转基因方法对大白菜进行基因转化所获得的转基因植株分析显示,外源基因多数以多拷贝形式整合于核基因组,少部分外源基因以单拷贝形式整合。(2)Elisa分析结果证明,所导入的外源基因可高效表达,T4代株系新鲜叶片中表达产物量最高达到0.069μg·g~(-1)左右。(3)转基因株系田间抗虫性统计分析表明,转化株系与对照在抗虫性方面有显著差异,其对小菜蛾及菜青虫抗性普遍提高2~3级。研究认为,转BmkIT-Chitinase基因大白菜中BmkIT-Chitinase基因的表达可有效提高大白菜的抗虫性。     

农杆菌介导抗储粮害虫转基因小麦(Triticum aestivum L.)的获得及分析

以本实验室选育的小麦优良品系的胚性愈伤组织为材料,采用农杆菌介导将抗虫基因豇豆胰蛋白酶抑制剂基因CpTI转入小麦培养细胞,经筛选获得抗卡那霉素的愈伤组织并再生植株。经PCR和实时PCR检测、PCR-Southern和Southernblot验证,确定了3株独立再生植株为含有CpTI的转基因植株。农杆菌菌浓度、侵染时间及转化处理方式对小麦转化率均有明显影响。3株转基因植株正常可育并结籽,形成转基因株系。外源基因在转基因植株T1代中的分离呈多样性,部分株系(转基因株系T-Ⅰ、T-Ⅲ)表现出孟德尔遗传规律。抗虫试验表明,3株转基因植株T2代籽粒对储粮害虫麦蛾具有一定的抗性,转基因株系T-Ⅰ、T-Ⅱ、T-Ⅲ及非转基因植株的T2代籽粒虫蛀率分别为19·8%、21·9%、32·9%和58·3%。转基因植株T1代群体农艺性状调查显示,3个株系具有良好的农艺性状,为小麦的遗传改良提供了新的种质抗虫材料。     

Effects on Fertility in Transgenic Tobacco by Localized Expression of ipt Gene

The isopenteryl transferase (ipt) gene from Agrobacterium tumefaciens (Smith et Townsend) Conn was driven under the tobacco TA29 promoter and introduced into tobacco ( Nicotiana tabacum L.) plants by A. tumefaciens mediated transformation. PCR and Southern blot analysis confirmed that the ipt gene has integrated into the genomes of tobacco plants. The expression pattern of this chimeric TA29-ipt gene in the transgenic plants was studied, and the endogenous cytokinin level in different organs was assayed by ELISA method. The results showed that the cytokinin content in the androecium of transgenic plants increased 3-4 times as compared with the control, and some changes of the fertility of the TA29-ipt transgenic plants have been observed.     

ipt基因定位表达对转基因烟草育性的影响

杂种优势是生物界的一种普遍现象。作物杂种优势的利用是培育高产、抗逆、优质新品种的重要手段之一。然而 ,常规育种技术获得配套三系的难度很大 ,由此限制了杂种优势利用的发展。近年来应用转基因技术创造雄性不育植株已有不少报道[1- 5] 。有研究表明 ,自然突变的雄性不育株     

抗CⅡTA核糖核酸酶P抑制Daudi细胞表面MHC-Ⅱ类抗原的

探讨抗MHC-Ⅱ类分子转录激活因子(CⅡTA)的核糖核酸酶P对Daudi细胞表面MHC-Ⅱ类分子表达的抑制作用.M1-RNA 是核糖核酸酶P的催化活性单位.以pTK117质粒为模板,PCR扩增带有抗CⅡTA第452及629位点的引导序列的M1-RNA (M1-452-GS 及M1-629-GS),再分别插入pUC19载体(pUC19-M1-452-GS和pUC19-M1-629-GS).从Raji细胞中克隆CⅡTA基因DNA片段 (114～800)后插入pGEM-7zf(+)质粒.将重组M1-RNA与靶基因的mRNA进行细胞外共孵育,显示仅pUC19-M1-629-GS可特异性地切割靶基因mRNA.再将M1-629-GS克隆入psNAV载体(pA629)并稳定转染Daudi细胞株,RT-PCR检测其CⅡTA的mRNA水平,流式细胞术检测其HLA DR、DP、DQ抗原表达.与对照组比较,M1-629-GS阳性Daudi细胞的CⅡTA mRNA含量减少90.19%(P<0.05),其HLA DR、DP、DQ抗原表达分别降低91.97%、90.19%、92.36%(P<0.05).研究表明,抗CⅡTA的核糖核酸酶P可通过抑制CⅡTA 的转录而降低Daudi细胞表面的MHC-Ⅱ类分子的表达.     

Mutation spectra of TA*, the major photoproduct of thymidylyl-(3'5')-deoxyadenosine, in Escherichia coli under SOS conditions.

The biological activity of TA*, the major photoproduct of thymidylyl-(3',5')-deoxyadenosine, has remained speculative since it was identified a decade ago. To determine the mutagenicity of TA* in Escherichia coli, we constructed the replicative form of an M13mp18-derived phage containing TA* in the (-)-strand by polymerase-catalyzed elongation of a TA*-containing 49mer opposite a uracil-containing (+)-strand of the phage. The in vitro synthesis mixture was transfected into an ung+, phr- E.coli host and the progeny were screened with a hybridization probe unique for the (-)-strand. TA* was found to block DNA replication substantially in the absence of SOS, but under SOS, TA* was bypassed more efficiently and was highly mutagenic. Among 56 analyzed (-)-strand progeny from two transfections, 46 (82%) were mutants, including six (11%) tandem mutants. The most abundant mutation was a 3'A-->T substitution (31/46, 56%). The possible biological consequences of TA* formation in the highly conserved TATA box consensus sequence on gene expression are discussed in light of the mutagenicity of TA*.     

2-[3-(2-Thioxopyrrolidin-3-ylidene)methyll-tryptophan,a novel yellow pigment in salted radish roots

The structure of the yellow pigment found in salted radish roots was studied. It was found that 1-(2-thioxopyrrolidin-3-yl)-1,2,3,4-tetrahydro-beta-carboline-3-carboxylic acid (TPCC) was unstable under neutral pH, and was easily converted into the yellow pigment. The yellow pigment was isolated and identified as 2-[3-(2-thioxopyrrolidin-3-ylidene)methyl]-tryptophan (TPMT) by IR, MS, 1H-, and 13C-NMR spectroscopy. In addition, we proved that this compound was the main yellow pigment in salted radish roots. This compound induced no mutagenicity in Salmonella typhimurium TA98 and TA100, either with or without prior activation.     

2-[3-(2-Thioxopyrrolidin-3-ylidene)methyl]-tryptophan,a Novel Yellow Pigment in Salted Radish Roots

The structure of the yellow pigment found in salted radish roots was studied. It was found that 1-(2-thioxopyrrolidin-3-yl)-1,2,3,4-tetrahydro-β-carboline-3- carboxylic acid (TPCC) was unstable under neutral pH, and was easily converted into the yellow pigment. The yellow pigment was isolated and identified as 2-[3-(2-thioxopyrrolidin-3-ylidene)methyl]-tryptophan (TPMT) by IR, MS, ¹H-, and ¹³C-NMR spectroscopy. In addition, we proved that this compound was the main yellow pigment in salted radish roots. This compound induced no mutagenicity in Salmonella typhimurium TA98 and TA100, either with or without prior activation.     

Conformational solution studies of the anti-microbial temporin A retro-analogues by using NMR spectroscopy.

Temporin A (TA) is a small, basic and highly hydrophobic peptide, isolated from the skin of the European red frog, Rana temporaria. The TA (FLPLIGRVLSGIL-NH2) displays a broad spectrum of anti-microbial activity against Gram-positive bacteria and fungi Candida albicans. In this study we investigate the solution structure of two TA retro-analogues, (6-1)(7-13)-TA (GILPLFRVLSGIL-NH2) and retro-TA (LIGSLVRGILPLF-NH2) by using nuclear magnetic resonance (NMR). The 3D solution structure of the analogues was established by using inter-proton distances and vicinal coupling constants in the Simulated Annealing (SA) calculations (XPLOR program). The NMR conformational studies show the existence of the helical structure in the middle part of the (6-1)(7-13)-TA peptide and an unordered structure of the retro-TA analogue under the D3-TFE/H2O (3:7, v/v) conditions. Our investigations have shown that the hydrophobic cluster at N-terminus with the Pro amino acid residue in position 3 or 4, the helical structure and the amphipathic character of the peptide are responsible for the anti-microbial activity of the TA analogues.     

Effect of electrode location on EMG signal envelope in leg muscles during gait.

The aim of the study was to assess the variability of EMG signal envelope with electrode location during gait. Surface EMG signals were recorded from 10 healthy subjects from the tibialis anterior (TA), peroneus longus (PL), gastrocnemius medialis (GM), gastrocnemius lateralis (GL), and soleus (SO) muscles. From TA, PL, GL and GM, signals were acquired using a two-dimensional grid of 4 x 3 electrodes (10 x 15 mm in size, as used in most gait laboratories) with 20-mm interelectrode distance in both directions. A similar grid of 3 x 3 electrodes was used for SO. EMG envelope was characterized by its peak value, area after normalization by the peak value, and time instant corresponding to the maximum. The maximum relative change in peak value with electrode location, expressed as a percentage of the peak value in the central location, was (mean+/-SD) 31+/-18% for TA, 29+/-13% for PL, 25+/-15% for GL, 14+/-8% for GM, and 26+/-14% for SO. The maximum relative change in area was 29+/-13% for TA, 73+/-40% for PL, 31+/-23% for GL, 35+/-20% for GM, 20+/-13% for SO, and in the position of maximum, computed as distance from the maximum position in the central channel, it was 5+/-10% of the gait cycle for TA, 26+/-16% for PL, 3+/-2% for GL, 3+/-1% for GM, 3+/-3% for SO. A crosstalk index, defined on the basis of the expected intervals of muscle activation for healthy subjects, indicated that estimated crosstalk was present between TA and PL, in an amount which depended on electrode location. It was concluded that the estimate of muscle activation intensity during gait from surface EMG is variable with location of the electrodes while timing of muscle activity is more robust to electrode displacement and can be reliably extracted in those cases in which crosstalk is limited. These results are valid for healthy subjects, where the level of muscular activity during gait is much lower than maximum.     

Influence of high-intensity exercise training and anabolic androgenic steroid treatment on rat tissue glycogen content

To increase tissue glycogen content many athletes use anabolic androgenic steroids (AAS). However, the literature concerning the effects of androgens on glycogen metabolism is conflicting. This study aimed to determine the influence of training and AAS on body weight (bw), triglycerides, glucose, tissue glycogen and transaminases levels. Male Wistar rats, randomized into four groups (sedentary vehicle (SV), sedentary AAS (SA), trained vehicle (TV) and trained AAS (TA)), were treated with nadrolone (5 mg/Kg, 2x/week, i.m.) or vehicle. Trained rats performed jumps into water (4 sets, 10 repetitions, 30 sec rest) carrying a 50-70% body wt-load strapped to the chest (5 days/week,6 weeks). Two days after the last session, the animals were killed (bifatorial ANOVA+Tukey test; P < 0.05). Trained animals presented lower bw (TV:345+/-7 vs. SV:380+/-7 and TA:328+/-4 vs SA:370+/-11 g) and triglycerides levels (TV:77+/-3 vs. SV:98+/-4 and TA:79+/-3 vs. SA:98+/-8 mg/dL) and higher glycogen content in liver (TV:5.3+/-0.2 vs. SV:3.9+/-0.1 and TA:5.3+/-0.3 vs. SA:4.6+/-0,2 mg/100 mg) and in gastrocnemious (TV:0.70+/-0.02 vs. SV:0.49+/-0.01 and TA:0.73+/-0.03 vs. SA:0.57+/-0.02 mg/100 mg) than sedentary ones. In the cardiac muscle, the association between training and AAS increased glycogen content (TA:0.19+/-0.01 > SV:0.13+/-0.01=TV:0.13+/-0.01=SA:0.14+/-0.01 mg/100 mg). In the soleus AAS increased glycogen (SA:0.53+/-0.03 vs. SV:0.43+/-0.01 and TA:0.58+/-0.02 vs. TV:0.48+/-0.01 mg/100 mg). Exercise training and AAS had no effect on blood glucose and transaminases levels. Training and AAS effects on glycogen supercompensation are tissue-dependent and the effects of association between them were only observed in the cardiac muscle. These data emphasize the necessity of more studies to confirm greater effects of AAS than those promoted by physical exercise.     

Investigation of polyethylenimine‐grafted‐triamcinolone acetonide as nucleus‐targeting gene delivery systems

Background

Nuclear membrane is one of the main barriers in polymer mediated intracellular gene delivery. To improve the transgenic activity and safety of nonviral vector, triamcinolone acetonide (TA) as a nuclear localization signal was conjugated with different molecular weight polyethylenimine (PEI).

Methods

Different molecular weight PEI [600, 1800, 25 000 (25k)] was conjugated with TA to synthesize PEI‐TA by two‐step reaction. Their physicochemical characteristics, in vitro cytotoxicity and transfection efficiency were evaluated. To investigate the difference of transfection efficiency of various molecular weight PEI‐TA, their transfection mechanism was further investigated by confocal microscopy and competition assay. Transgenic expression in vivo was evaluated by injection into hepatic portal vein of mice.

Results

All PEI‐TA could form nanosize polyplexes with DNA and their physicochemical properties resemble each other. Their cytotoxicities were negligible compared to PEI 25k. The order of transfection efficiency was PEI 1800‐TA > PEI 600‐TA > PEI 25k‐TA. A transfection mechanism study displayed that TA could inhibit considerably the transgenic activity of PEI 1800‐TA and PEI 600‐TA, but that of PEI 25k‐TA was not inhibited. It was suggested that PEI 1800‐TA and PEI 600‐TA might translocate into the nucleus. Confocal microscopy investigation verified this suggestion. The data strongly suggested that the transfection efficiency of PEI 1800‐TA in vivo was much higher than that of PEI 25k, which was consistent with the results obtained in vitro.

Conclusions

Low molecular weight PEI‐TA could translocate into the nucleus efficiently. PEI 1800‐TA presented higher transgenic activity and it has a great potential for gene therapy as a nonviral carrier. Copyright © 2010 John Wiley & Sons, Ltd.