根癌农杆菌介导马铃薯试管薯转化体系的优化及AtNHX1基因的导入

以马铃薯栽培品种甘农薯2号的试管薯薄片为转化受体材料,通过根癌农杆菌LBA4404介导拟南芥液泡膜Na /H 逆向转运蛋白基因(AtNHX1)进行转化,获得了抗卡那霉素的再生植株,并对转化植株进行了PCR-Southern检测.结果表明,薯片分化和根再生的卡那霉素选择压为50mg/L;乙酰丁香酮对薯片转化率无影响;优化的试管薯片转化方法是:不经预培养的薯片用OD600值为0.5的菌液侵染8～10min,然后经过2d共培养,在抗性芽分化培养基上生长40d,可获得30%卡那抗性绿苗.对抗性植株的PCR和PCR-Southern检测证明,外源At-NHX1基因已整合到马铃薯基因组中.     

根癌农杆菌介导的CMO基因转化马铃薯的研究

通过根癌农杆菌介导法将强组成型表达启动子CaMV 35S和逆境诱导表达启动子rd29A 驱动的菠菜胆碱单加氧酶(CMO)基因导入马铃薯栽培品种夏波蒂(Shepody)和费乌瑞它( Favorita)中,获得了抗卡那霉素再生植株,对转化植株进行PCR检测初步表明CMO基因已整 合到转基因马铃薯基因组中.并对光照强度对马铃薯试管薯遗传转化的影响进行了研究,结果表明在诱导芽分化的过程中,2 000 lx的光照强度有利于试管薯薄片直接再生出抗性芽.     

豆科植物田著农杆菌转化的研究

本文报道一个简便的豆科植物田著的转化试验。田蓄子叶外值体能被含非致瘤性的Ti质"Y.载体 的根癌农杆菌感染。该载体带有一个嵌合的npr-II基因和胭脂碱合成酶基因。卡那霉素抗性愈伤组 织经胭脂碱测定、N P T-11酶活性检测和DNA分子杂交试验证明外源基因已导入了田蔷细抱。     

Ti质粒T区tms基因的分离及其对高等植物分化的影响

根癌农杆菌Ti质粒的T区DNA带有致瘤基因,其基因1和基因2编码生长素吲哚乙酸生物合成途径中的两个酶。以pGV 354(pBR322质粒中插有Ti质粒C 58 T区DNA的HindⅢ15—HindⅢ22大片段)重组质粒出发,我们分离了基因1和基因2,并构建了带有卡那霉素抗性基因的重组质粒pBZ 692,通过基因载体pGV 3850,我们将基因1和基因2引入了高等植物。结果证明基因1和基因2能促使烟草、向日葵、土豆等转化组织分化长根,转化的根在MS_0培养基上能脱分化形成愈伤组织并自主生长,在转化的组织中有转化标记胭脂碱的存在。     

根癌农杆菌介导的高羊茅遗传转化研究

采用携带卡那霉素抗性基因nptⅡ和Na^ ／H^ 反向运输AtNHX1基因的表达载体pROK2／AtNHX1(带有35S启动子)和pROK2U／AtNHX1(带有ubi1启动子)的根癌农杆菌AGL1和GV3101,对4个品种高羊茅下胚轴来源的胚性愈伤组织进行了遗传转化。胚性愈伤组织经根癌农杆菌感染和共培养后,用50～150mg／L巴龙霉素筛选抗性愈伤组织,获得1126棵再生植株,用10～20mg／L卡那霉素进一步筛选再生植株,总共得到525棵绿色抗性植株。抗性植株的总DNA用AtNHX1基因的特异引物进行PCR检测,其中21棵为PCR阳性,最高转化频率为1．77％。Southern杂交结果证实,外源基因以低拷贝整合到高羊茅的基因组中,实验发现,在不同品种之间转化效率有所差异。     

马铃薯遗传转化体系的优化及玉米淀粉分支酶基因SBEⅡb的导入

以马铃薯脱毒试管苗茎段为转化受体材料,建立并优化了农杆菌介导的马铃薯遗传转化体系。通过农杆菌介导法将玉米淀粉分支酶基因(Starch branching enzyme b,SBEⅡb)的过表达载体转化马铃薯,接种762个茎段,共获得35株抗性植株。经PCR检测获得了4株转基因阳性植株;对转基因植株进一步进行GUS活性组织化学染色,发现转基因植株的茎段与试管薯均被染上蓝色,表明外源SBEⅡb基因已整合到马铃薯基因组,且正常表达。     

Optimization of genetic transformation system of potato and introduction of maize starch branching enzyme gene SBEⅡb into potatoFAN

以马铃薯脱毒试管苗茎段为转化受体材料,建立并优化了农杆菌介导的马铃薯遗传转化体系.通过农杆菌介导法将玉米淀粉分支酶基因(Starch branching enzyme b,SBEⅡb)的过表达载体转化马铃薯,接种762个茎段,共获得35株抗性植株.经PCR检测获得了4株转基因阳性植株;对转基因植株进一步进行GUS活性组织化学染色,发现转基因植株的茎段与试管薯均被染上蓝色,表明外源SBEⅡb基因已整合到马铃薯基因组,且正常表达.     

影响根癌农杆菌介导水稻转化的因素分析

根癌农杆菌与来自水稻成熟种子盾片的愈伤组织共培养,将GUS基因导入水稻愈伤组织,并获得了转基因植株。通过比较影响根癌农杆菌转化频率的各种因素,表明激素配比为2,4-D1mg/L、TDZ0.5mg/L、NAA1mg/L时,可以大大促进籼稻愈伤组织的分化能力;酚类化合物的加入使农杆菌的转化频率提高8.9%-23.5%;共培养时农杆菌的稀释方式及适当调整潮霉素（hygB）的使用浓度影响到农杆菌的转化频率。     

水蛭肽基因的克隆及其转化甘蓝

将合成的水蛭肽基因转入甘蓝,构建了水蛭肽的植物表达载体pBOK-L,使用甘蓝的下胚轴和根癌农杆菌的共培养实现转化,再生植株经卡那霉素筛选,检测结果表明所得到的抗性植株均为转基因植株,获得了转水蛭 肽基因的甘蓝植株。     

甜蛋白基因MBLⅡ对番茄的遗传转化

以5～7d龄的“丽春”番茄无菌苗子叶作为外植体,研究了子叶外植体对抗生素卡那霉素的敏感性,抗生素卡那霉素对番茄筛选的适宜浓度为70mg／L。通过根癌农杆菌(Agrobacterium tumefaciens)介导,成功地进行了马槟榔甜蛋白基因MBLⅡ对番茄的遗传转化,获得转化番茄抗性植株,组织化学法有阳性表现、PCR特异扩增及Southern杂交检测出现特异条带,表明MBLⅡ基因已顺利整合到转基因番茄植株的基因组。     

Entwicklungsgeschichte und Ultrastruktur von Pollenkitt und Exine bei nahe verwandten entomophilen und anemophilen Angiospermensippen derAlismataceae,Liliaceae, Juncaceae,Cyperaceae, Poaceae undAraceae

Some closely related members of the monocotyledonous familiesAlismataceae, Liliaceae, Juncaceae, Cyperaceae, Poaceae andAraceae with variable modes of pollination (insect- and wind-pollination) were studied in relation to the ultrastructure of pollenkitt and exine (amount, consistency and distribution of pollenkitt on the surface of pollen grains). The character syndromes of pollen cementing in entomophilous, anemophilous and intermediate (ambophilous or amphiphilous) monocotyledons are the same in principal as in dicotyledons. Comparing present with former results one can summarize: 1) The pollenkitt is always produced in the same manner by the anther tapetum in all angiosperm sub-classes. 2) The variable stickiness of entomophilous and anemophilous pollen always depends on the particular distribution and consistency of the pollenkitt, but not its amount on the pollen surface. 3) The mostly dry and powdery pollen of anemophilous plants always contains a variable amount of inactive pollenkitt in its exine cavities. 4) A step-by step change of the pollen cementing syndrome can be observed from entomophily towards anemophily. 5) From the omnipresence of pollenkitt in all wind-pollinated angiosperms studied one can conclude that the ancestors of anemophilous angiosperms probably have been zoophilous (i.e. entomophilous) throughout.

     

Identification and Characterization of the First Equine Parainfluenza Virus 5

正Dear Editor,Parainfluenza virus 5 (PIV5), known as canine parainfluenza virus in the veterinary field, is a negative-sense,nonsegmented, single-stranded RNA virus belonging to the Paramyxoviridae family (Chen 2018). The virus was first reported in primary monkey kidney cells in 1954 (Hsiung1972), then it has been frequently discovered in various     

Pathogenic Characterization and Full Length Genome Sequence of a Reassortant Infectious Bursal Disease Virus Newly Isolated in Pakistan

<正>Dear Editor,Infectious bursal disease (IBD) is one of the most important diseases of the poultry. The IBD virus (IBDV), a nonenveloped virus belonging to the Birnaviridae family with a genome consisting of two segments of double-stranded RNA (segments A and B), targets B lymphocytes of bursa of Fabricious leading to immunosuppression. In Pakistan,poultry farming is the second biggest industry and IBD is the second biggest disease threating the poultry sector.However, there is limited genome information of IBDV     

Mink Circovirus Can Infect Minks,Foxes and Raccoon Dogs

正Dear Editor,Mink circovirus (MiCV), which is clustered in the genus Circovirus of the family Circoviridae, was first described in minks from farms in Dalian, China in 2013 (Lian et al.2014). The complete single-stranded circular genome of the virus is 1,753 nucleotides long and contains two major open reading frames (ORFs), designated ORF1 (Rep gene)and ORF2 (Cap gene)(Lian et al. 2014; Ge et al. 2018).Sequence analysis has shown that MiCV is most closely     

CypA Regulates AIP4-Mediated M1 Ubiquitination of Influenza A Virus

Cyclophilin A (CypA) is a peptidyl-prolyl cis/trans isomerase that interacts with the matrix protein (M1) of influenza A virus (IAV) and restricts virus replication by regulating the ubiquitin–proteasome-mediated degradation of M1. However,the mechanism by which CypA regulates M1 ubiquitination remains unknown. In this study, we reported that E3 ubiquitin ligase AIP4 promoted K48-linked ubiquitination of M1 at K102 and K104, and accelerated ubiquitin–proteasome-mediated degradation of M1. The recombinant IAV with mutant M1 (K102 R/K104 R) could not be rescued, suggesting that the ubiquitination of M1 at K102/K104 was essential for IAV replication. Furthermore, CypA inhibited AIP4-mediated M1 ubiquitination by impairing the interaction between AIP4 and M1. More importantly, both the mutations of M1 (K102 R/K104 R) and CypA inhibited the nuclear export of M1, indicating that CypA regulates the cellular localization of M1 via inhibition of AIP4-mediated M1 ubiquitination at K102 and K104, which results in the reduced replication of IAV.Collectively, our findings reveal a novel ubiquitination-based mechanism by which CypA regulates the replication of IAV.