EMS处理对大白菜种子和幼苗活力的影响及M_2表型变异分析

大白菜突变体的获得是种质创新的有效途径,也是开展功能基因组研究的材料基础。本研究选取自交亲和、易进行小孢子培养的大白菜自交系‘A03’作为构建突变体库的野生型材料。分析EMS种子处理对M1、M2种子和幼苗活力及生理特性的影响,确定适宜诱变方案并构建突变体库,并针对突变体库M2群体结球期、收获期和生殖生长阶段表型性状变异进行了分析。结果表明,以浓度0.4%的EMS浸泡种子16 h,以及连续对两代种子进行诱变处理,均可以构建大白菜突变体库。突变体库M2群体植株在结球期、收获期和生殖生长阶段表型变异丰富,变异频率分别为21.65%、22.40%和25.65%。     

罗布麻EMS突变体库构建及黄酮变异突变体筛选

罗布麻(Apocynum venetum L.)突变体的获得是人工创新种质资源的有效途径,也是开展品种选育、功能基因组研究的基础。本研究以采自东营野生罗布麻种子作为材料,预试验结果表明0.7%的甲基磺酸乙酯(EMS,ethylmethylsulfone)溶液诱变罗布麻种子13 h能够达到半致死剂量。在此浓度和处理时间下构建了一个1452株的突变体群体,对获得的M1植株进行农艺性状和总黄酮含量性状筛选,初步获得125份农艺性状突变材料,其中包括8株白化植株、23株叶型变异株、16株叶色黄纹突变体、32株苗期分枝植株以及46株叶位变异突变体,突变频率分别为0.55%、1.6%、1.1%、2.2%和3.2%。此外,还筛选到2株总黄酮含量明显高于野生型和1株低于野生型的材料。在突变群体中对黄酮代谢途径中编码黄烷酮-3-羟化酶的基因(F3H,flavanone 3-hydroxylase gene)进行测序鉴定,结果鉴定到3株F3H基因的突变体。本研究构建的罗布麻突变体库表型丰富且突变位点可以鉴定,是罗布麻新种质筛选、品种选育以及基因功能研究的良好材料。     

粗糙脉孢菌26 S蛋白酶体三个亚基缺失菌株的构建及表型分析

【目的】通过构建26S蛋白酶体的3个亚基RPN4、RPN7、RPN10的缺失突变菌株,研究这些缺失突变体的表型,进而探究这3个亚基在蛋白酶体中的作用。【方法】采用同源重组基因敲除技术、电转化、粗糙脉胞菌杂交、子囊孢子萌发及PCR鉴定等方法分别获得3个调节亚基的基因缺失突变体。利用racetube和平板生长法进行突变体表型检测。【结果】得到rpn4和rpn10的缺失突变纯合体及rpn7缺失突变异核体菌株。【结论】与野生型相比,rpn7KO(ku70RIP背景)突变体的菌丝生长及产生分生孢子的能力显著减弱;rpn4KO突变体在生长初期的菌丝生长缓慢,而后期的产孢能力与野生型无显著差异;rpn10KO突变菌株的表型介于上述两种突变体的表型之间。这些结果表明26S蛋白酶体的这3个亚基对脉胞菌的生长和发育至关重要。     

EMS诱变西瓜突变体库的构建及表型分析

采用1.0%诱变剂甲基磺酸乙酯(EMS)处理西瓜品系W1-17种子9h,然后对M1和M2代群体单株在叶、花、茎、育性、分支习性等方面进行表型变异观察,同时选取M2代典型变异株系,利用23对西瓜SSR引物进行分析鉴定,构建西瓜突变体库。结果表明:(1)EMS诱变使M1代幼苗形态呈现出叶畸形、叶褶皱、部分黄化、花畸形、雄花不散粉、卷须畸形、矮小、生长缓慢、不育等特异性状,获得由1 252个单株组成的西瓜突变体M1群体,群体总变异频率为18.33%。(2)M2代共筛选到205个突变植株,40种表型变异,表现在子叶性状(黄化、扭曲不对称、折叠等)、叶和茎性状(叶黄化、变小、裂刻变深,茎变细,节间变短,分支少等)、花性状(花变大,花色变浅,两性花,花瓣皱缩、部分退化、数目突变,柱头畸形,雄蕊不成熟等)和其他性状(生长缓慢、不育等)等方面,总的表型突变率达到了19.59%。(3)针对M2代10个典型变异植株,通过SSR引物分析发现有9份材料在DNA水平上有变异。本研究初步构建了含有120个M1代家系及1 051株M2代植株、40种表型变异的西瓜突变体库。     

Tn5介导的致病性副溶血弧菌溶血能力差异突变株表型分析

【目的】构建致病性副溶血弧菌(Vibrio parahaemolyticus,Vp)突变体库,分析溶血能力差异突变株表型特征,为深入挖掘和认识tdh的调控机制提供研究基础。【方法】利用双亲本接合法,将Mini-Tn5-Km2片段随机插入致病性Vp (ATCC 33846)基因组,并以含有卡那霉素(Km)和氨苄青霉素(Amp)的TCBS选择性培养基进行突变株(KmRAmpS)筛选;结合PCR方法对突变菌株进行Km基因筛查,构建在不同基因位点随机插入突变的Vp突变体库。以我妻氏血平板筛选溶血表型变化菌株,并对其生长曲线、菌膜形成能力和运动能力进行测定。【结果】采用双亲本接合法,成功建立包含490株Vp突变株的突变体库,并获得5株溶血表型变化稳定的菌株(2株为溶血能力上调,3株为下调)。5株突变株在生长速率、菌膜形成能力及运动能力方面与亲本株有显著性差异。其中,2株溶血能力上调菌株及1株溶血能力下调菌株在运动能力、生长速率和菌膜形成能力方面较亲本株显著降低(P<0.05);另2株溶血能力下调菌株菌膜形成能力较亲本株显著提高(P<0.05)。【结论】Tn5转座子可用于建立Vp突变体库;Vp溶血能力与其表型特征具有相关性;研究所获得的5株溶血表型突变株为进一步探讨Vp tdh的调控机制奠定基础。     

耐辐射球菌基因DR1709与DR2523的突变分析

摘要：【目的】检测在耐辐射球菌抵抗外来辐射和氧自由基的过程中,锰离子转运蛋白基因（DR1709和DR2523）是否发挥了作用。探讨锰离子、锰离子转运蛋白基因与耐辐射球菌辐射抗性之间的关系。【方法】分别构建这两个基因的突变体。对突变体和野生型进行紫外线照射和过氧化氢处理。对处理后的菌株存活率进行分析。【结果】DR2523被突变以后,耐辐射球菌在tryptone-glucose-yeast extract (TGY)培养液中的生长受影响很小。而DR1709突变体M1709在对数生长阶段的生长速度远低于野生型。     

茎瘤固氮根瘤菌ORS571鞭毛马达基因fliN与fliM的功能分析

【目的】考察茎瘤固氮根瘤菌ORS571中鞭毛马达蛋白FliN、FliM的编码基因分别缺失的突变体表型,初步探究其功能机理。【方法】本研究采用同源重组和三亲本接合转移的方法构建突变体,测定野生型及突变株的生长曲线、趋化性、胞外多糖的分泌、生物膜的形成及细胞絮凝等表型。【结果】三种菌株的生长速率基本无差,与野生型菌株相比突变株鞭毛结构丧失,趋化能力、分泌的胞外多糖和生物膜形成能力均下降,但相同时间内细胞絮凝程度比野生型明显。【结论】实验表明,鞭毛基因fliN、fliM对茎瘤固氮根瘤菌ORS571鞭毛的形成、趋化运动、胞外多糖的分泌、生物膜的形成及细胞絮凝能力等均有调控作用。     

甜瓜突变体库的构建及M2群体表型变异的研究

利用8种不同浓度的甲基磺酸乙酯（EMS）,4种不同的浸种时间,处理甜瓜品系“3-2-2”种子,根据M1代植株发芽率,筛选出适宜的诱变剂量为浓度1.2%,诱变时间为24 h。采用这种方法构建了含有67个M1家系及相应自交M2代种子的甜瓜突变体库。对M1代群体541个单株的表型变异进行了全生育期初步调查,总的表型变异频率达71.53%。对M2代群体603个单株的节间长度、主蔓粗度、叶片长度、叶片宽度、叶柄长度、叶柄粗度共6个表型性状进行形态学调查表明:除节间长度外,其它5个性状和野生型相比均差异显著;不同性状的变异系数不同,叶柄长度的变异系数最大,达15.37%,节间长度的变异系数最小,为7.10%;在M2代中,编号为25的家系叶片出现了黄色和绿色的性状分离。     

茎瘤固氮根瘤菌环二鸟苷酸代谢相关基因的功能鉴定

【目的】考察茎瘤固氮根瘤菌ORS571中c-di-GMP合成酶AZC-2412的编码基因缺失的突变表型,初步探究其功能机理。【方法】本实验构建基于cre-loxp重组酶系统的根瘤菌基因敲除系统,以及采用三亲接合技术构建突变株。测定野生型和突变株的生长速率、趋化能力、胞外多糖产量、生物膜形成等表型。【结果】突变株与野生型生长速率几乎相同。与野生型相比突变株由于细胞内c-di-GMP水平降低,胞外多糖、生物膜产量等均有所下降。【结论】实验表明,环二鸟苷酸合成酶AZC-2412缺失,使得c-di-GMP水平降低,对胞外多糖生成、细菌的运动能力、生物膜的形成、细胞絮凝、与植物的互作等均有调控作用。     

兽疫链球菌中与透明质酸合成相关新基因的高通量筛选及克隆

【目的】兽疫链球菌(Streptococcus equi subsp. zooepidemicus)中透明质酸主要的生物合成途径和相关基因已经被研究得比较透彻,探究一种挖掘与透明质酸合成相关新基因的策略。【方法】利用自杀质粒pSET4s::sacB在宿主基因组中的随机整合作用,筛选具有表型差异突变菌株构建突变体库,进一步利用连接介导PCR (Ligation mediated PCR,LM-PCR)方法和全基因组重测序,检测质粒整合位点,通过基因无痕敲除和回补实验验证插入位点。【结果】构建了包含150株具有表型差异突变株的突变体库;以荚膜合成能力缺失的1号突变株(M1)作为基础研究对象,检测到自杀质粒整合到基因组458 960位点上,破坏了编码塔格糖-6-磷酸激酶的lacC基因;无痕敲除lacC基因得到ΔlacC,表型分析发现ΔlacC表现为粘性荚膜特性;进一步全基因组重测序发现,除了lacC基因位点存在插入突变,206 613位点存在碱基G缺失,导致编码透明质酸合成酶的hasA基因发生移码突变,且回补hasA基因后,M1恢复粘性荚膜合成能力。【结论】M1突变株粘性荚膜合成能力的缺失由hasA基因功能缺失引起,与lacC基因功能缺失无关。初步建立了兽疫链球菌中高通量筛选与透明质酸合成相关新基因的策略,为今后挖掘新基因奠定了基础。     

Preparation of hair for measurement of elements by inductively coupled plasma-mass spectrometry (ICP-MS)

The preparation of hair for the determination of elements is a critical component of the analysis procedure. Open-beaker, closedvessel microwave, and flowthrough microwave digestion are methods that have been used for sample preparation and are discussed. A new digestion method for use with inductively coupled plasma-mass spectrometry (ICP-MS) has been developed. The method uses 0.2 g of hair and 3 mL of concentrated nitric acid in an atmospheric pressurelow-temperature microwave digestion (APLTMD) system. This preparation method is useful in handling a large numbers of samples per day and may be adapted to hair sample weights ranging from 0.08 to 0.3 g. After digestion, samples are analyzed by ICP-MS to determine the concentration of Li, Be, B, Na, Mg, Al, P, S, K, Ca, Ti, V, Cr, Mn, Fe, Co, Ni, Cu, Zn, Ge, As, Se, Rb, Sr, Zr, Mo, Pd, Ag, Cd, Sn, Sb, I, Cs, Ba, Pt, Au, Hg, Tl, Pb, Bi, Th, and U. Benefits of the APLTMD include reduced contamination and sample handling, and increased precision, reliability, and sample throughput.     

外泌体在白血病中的重要调控作用

目前,白血病复发是患者死亡的主要原因之一。肿瘤细胞和微环境的相互作用,以及隐匿在骨髓中的肿瘤干细胞,促进了白血病的复发和向淋巴组织的转移,因此白血病的治疗、转移和复发问题受到广泛关注。外泌体是由绝大多数细胞分泌的双层脂质膜囊泡,可以调控细胞间的交流和信息传递。在白血病细胞、基质细胞和内皮细胞之间的相互联系中都涉及到外泌体,白血病细胞来源的外泌体存在于白血病患者的血浆中,能把其携带的白血病相关抗原及微小RNA呈递给靶细胞,促进白血病肿瘤细胞的增殖,有助于肿瘤细胞实现免疫逃避,保护白血病细胞抵抗化疗药物导致的细胞毒性作用,促进血管生成及肿瘤细胞的迁移。因此,外泌体与白血病的转移、治疗及预后密切相关,可以用来检测和监测白血病的进展。本文综述了外泌体的来源、形成与分泌机制,以及外泌体在白血病发生前、发展中、预后和免疫治疗中所扮演的重要角色。     

日本北海道虻类雌性外生殖器形态(双翅目：虻科)(英文)

【目的】利用日本北海道虻类评估和验证外生殖器在分类学上的意义。【方法】将虻类成虫标本浸渍在生理盐水中并置于双目显微镜下通过针和镊子在培养皿中进行解剖并绘图,观察第9背板、第10背板、尾叶、第8腹板、受精囊、受精囊管及生殖叉器的形态特征。【结果】在日本北海道共记录了虻科(Tabanidae) 3亚科7属38种。我们观察并描述了3亚科其中的6属24种的雌性外生殖器的主要特征。亚科之间存在明显差异;然而在一般情况下属之间很难建立一种方法来确定共同点;种之间只有在斑虻属Chrysops中有相似之处,其他属中则比较多样化。因此,亚科鉴定根据第9背板、第8腹板及受精囊足以进行区分,属及种鉴定需要结合第9背板、第10背板、尾叶、第8腹板、受精囊、受精囊管及生殖叉器各自的特征组合在一起才能区分开来。我们也制作了虻类外生殖器的检索表。【结论】和许多其他昆虫一样,外生殖器是虻科的重要分类特征,对于促进分类学和系统学的发展具有重要意义。本研究首次对分布在日本北海道的虻科雌性外生殖器进行了系统研究。     

Ecological importance of sedges: a survey of the Australasian Cyperaceae genus Lepidosperma

Background

Sedges (Cyperaceae) form an important ecological component of many ecosystems around the world. Sword and rapier sedges (genus Lepidosperma) are common and widespread components of the southern Australian and New Zealand floras, also occurring in New Caledonia, West Papua, Borneo, Malaysia and southern China. Sedge ecology is seldom studied and no comprehensive review of sedge ecology exists. Lepidosperma is unusual in the Cyperaceae with the majority of species occurring in dryland habitats.

Scope

Extensive review of ecological literature and field observations shows Lepidosperma species to be important components of many ecosystems, often dominating understorey and sedge-rich communities. For the first time, a detailed ecological review of a Cyperaceae genus is presented.

Conclusions Lepidosperma

species are long-lived perennials with significant abundance and persistence in the landscape. Speciation patterns in the genus are of considerable interest due to complex biogeographical patterns and a high degree of habitat specificity. Potential benefits exist for medicinal products identified from several Lepidosperma species. Over 178 organisms, including 26 mammals, 42 birds, six reptiles, five amphibians, eight arachnids, 75 insects, three crustaceans and 13 fungi, are found to be dependent on, or making use of, Lepidosperma species. A significant relationship exists between Lepidosperma species and the moth genus Elachista. Implications for the conservation and ecology of both sedges and associated species are discussed.     

Literature based species occurrence data of birds of northeast India

The northeast region of India is one of the world's most significant biodiversity hotspots. One of the richest bird areas in India, it is an important route for migratory birds and home to many endemic bird species. This paper describes a literature-based dataset of species occurrences of birds of northeast India. The occurrence records documented in the dataset are distributed across eleven states of India, viz.: Arunachal Pradesh, Assam, Bihar, Manipur, Meghalaya, Mizoram, Nagaland, Sikkim, Tripura, Uttar Pradesh and West Bengal. The geospatial scope of the dataset represents 24 to 29 degree North latitude and 78 to 94 degree East longitude, and it comprises over 2400 occurrence records. These records have been collated from scholarly literature published between1915 and 2008, especially from the Journal of the Bombay Natural History Society (JBNHS). The temporal scale of the dataset represents bird observations recorded between 1909 and 2007. The dataset has been developed by employing MS Excel. The key elements in the database are scientific name, taxonomic classification, temporal and geospatial details including geo-coordinate precision, data collector, basis of record and primary source of the data record. The temporal and geospatial quality of more than 50% of the data records has been enhanced retrospectively. Where possible, data records are annotated with geospatial coordinate precision to the nearest minute. This dataset is being constantly updated with the addition of new data records, and quality enhancement of documented occurrences. The dataset can be used in species distribution and niche modeling studies. It is planned to expand the scope of the dataset to collate bird species occurrences across the Indian peninsula.     

Characterization of citrus pectin samples extracted under different conditions: influence of acid type and pH of extraction

Background and Aims

Pectin is a complex macromolecule, the fine structure of which is influenced by many factors. It is used as a gelling, thickening and emulsifying agent in a wide range of applications, from food to pharmaceutical products. Current industrial pectin extraction processes are based on fruit peel, a waste product from the juicing industry, in which thousands of tons of citrus are processed worldwide every year. This study examines how pectin components vary in relation to the plant source (orange, lemon, lime, grapefruit) and considers the influence of extraction conditions on the chemical and macromolecular characteristics of pectin samples.

Methods

Citrus peel (orange, lemon, lime and grapefruit) from a commercial supplier was used as raw material. Pectin samples were obtained on a bulk plant scale (kilograms; harsh nitric acid, mild nitric acid and harsh oxalic acid extraction) and on a laboratory scale (grams; mild oxalic acid extraction). Pectin composition (acidic and neutral sugars) and physicochemical properties (molar mass and intrinsic viscosity) were determined.

Key Results

Oxalic acid extraction allowed the recovery of pectin samples of high molecular weight. Mild oxalic acid-extracted pectins were rich in long homogalacturonan stretches and contained rhamnogalacturonan I stretches with conserved side chains. Nitric acid-extracted pectins exhibited lower molecular weights and contained rhamnogalacturonan I stretches encompassing few and/or short side chains. Grapefruit pectin was found to have short side chains compared with orange, lime and lemon. Orange and grapefruit pectin samples were both particularly rich in rhamnogalacturonan I backbones.

Conclusions

Structural, and hence macromolecular, variations within the different citrus pectin samples were mainly related to their rhamnogalacturonan I contents and integrity, and, to a lesser extent, to the length of their homogalacturonan domains.     

The Rumen Ciliate Fauna of Domestic Sheep (Ovis ammon aires) from the Turkish Republic of Northern Cyprus

ABSTRACT. Concentration and composition of ciliate protozoa in the families Ophryoscolecidae and Isotrichidae were determined in rumen contents of domestic sheep ( Ovis ammon aries ) from Cyprus. A total of five genera of Ophryoscolecidae were identified, Metadinium, Enoploplastron, Polyplastron, Epidinium , and Ophryoscolex , which included six species: Metadinium affine, Enoploplastron triloricatum, Polyplastron multivesiculatum, Epidinium ecaudatum, Epidinium graini, and Ophryoscolex purkynjei. Eight separate forms of Epidinium were identified ( E. ecaudatum f. ecaudatum, E, e. f. caudatum, E. e. f. bicaudatum, E. e. f. tricaudatum, E. e. f. quadricaudatum, E. graini f. graini, E. g. f. caudatricoronatum , and E. g. f. caudaquadricoronatum ), along with five forms of Ophryoscolex purkynjei (O. p. f. purkynjei, O. p. f. bifidobicinctus, O. p. f. bifidoquadricinctus, O. p. f. bicoronatus, O. p. f. tricoronatus , and O. p. f. quadricoronatus). Three species of Isotrichidae were observed, Isotricha intestinalis, I. prostoma , and Dasytricha ruminantium. This study reports new host records for three forms of Epidinium graini and Ophryoscolex purkynjei f. bifidobicinctus. The rumen fauna in the family Ophryoscolecidae from Cypriote domestic sheep appear to have limited diversity compared to those from Turkish and Far Eastern (Chinese/Japanese) sheep, while they are more diverse than those found in Western European (Scottish) and North American (Canadian/Alaskan) sheep.     

Micromanipulation of Gene Expression in the Adult Zebrafish Brain Using Cerebroventricular Microinjection of Morpholino Oligonucleotides

Manipulation of gene expression in tissues is required to perform functional studies. In this paper, we demonstrate the cerebroventricular microinjection (CVMI) technique as a means to modulate gene expression in the adult zebrafish brain. By using CVMI, substances can be administered into the cerebroventricular fluid and be thoroughly distributed along the rostrocaudal axis of the brain. We particularly focus on the use of antisense morpholino oligonucleotides, which are potent tools for knocking down gene expression in vivo. In our method, when applied, morpholino molecules are taken up by the cells lining the ventricular surface. These cells include the radial glial cells, which act as neurogenic progenitors. Therefore, knocking down gene expression in the radial glial cells is of utmost importance to analyze the widespread neurogenesis response in zebrafish, and also would provide insight into how vertebrates could sustain adult neurogenesis response. Such an understanding would also help the efforts for clinical applications in human neurodegenerative disorders and central nervous system regeneration. Thus, we present the cerebroventricular microinjection method as a quick and efficient way to alter gene expression and neurogenesis response in the adult zebrafish forebrain. We also provide troubleshooting tips and other useful information on how to carry out the CVMI procedure.     

Design and Use of Multiplexed Chemostat Arrays

Chemostats are continuous culture systems in which cells are grown in a tightly controlled, chemically constant environment where culture density is constrained by limiting specific nutrients.^1,2 Data from chemostats are highly reproducible for the measurement of quantitative phenotypes as they provide a constant growth rate and environment at steady state. For these reasons, chemostats have become useful tools for fine-scale characterization of physiology through analysis of gene expression^3-6 and other characteristics of cultures at steady-state equilibrium.⁷ Long-term experiments in chemostats can highlight specific trajectories that microbial populations adopt during adaptive evolution in a controlled environment. In fact, chemostats have been used for experimental evolution since their invention.⁸ A common result in evolution experiments is for each biological replicate to acquire a unique repertoire of mutations.^9-13 This diversity suggests that there is much left to be discovered by performing evolution experiments with far greater throughput. We present here the design and operation of a relatively simple, low cost array of miniature chemostats—or ministats—and validate their use in determination of physiology and in evolution experiments with yeast. This approach entails growth of tens of chemostats run off a single multiplexed peristaltic pump. The cultures are maintained at a 20 ml working volume, which is practical for a variety of applications. It is our hope that increasing throughput, decreasing expense, and providing detailed building and operation instructions may also motivate research and industrial application of this design as a general platform for functionally characterizing large numbers of strains, species, and growth parameters, as well as genetic or drug libraries.     

A Microplate Assay to Assess Chemical Effects on RBL-2H3 Mast Cell Degranulation: Effects of Triclosan without Use of an Organic Solvent

Mast cells play important roles in allergic disease and immune defense against parasites. Once activated (e.g. by an allergen), they degranulate, a process that results in the exocytosis of allergic mediators. Modulation of mast cell degranulation by drugs and toxicants may have positive or adverse effects on human health. Mast cell function has been dissected in detail with the use of rat basophilic leukemia mast cells (RBL-2H3), a widely accepted model of human mucosal mast cells^3-5. Mast cell granule component and the allergic mediator β-hexosaminidase, which is released linearly in tandem with histamine from mast cells⁶, can easily and reliably be measured through reaction with a fluorogenic substrate, yielding measurable fluorescence intensity in a microplate assay that is amenable to high-throughput studies¹. Originally published by Naal et al.¹, we have adapted this degranulation assay for the screening of drugs and toxicants and demonstrate its use here.Triclosan is a broad-spectrum antibacterial agent that is present in many consumer products and has been found to be a therapeutic aid in human allergic skin disease^7-11, although the mechanism for this effect is unknown. Here we demonstrate an assay for the effect of triclosan on mast cell degranulation. We recently showed that triclosan strongly affects mast cell function². In an effort to avoid use of an organic solvent, triclosan is dissolved directly into aqueous buffer with heat and stirring, and resultant concentration is confirmed using UV-Vis spectrophotometry (using ε₂₈₀ = 4,200 L/M/cm)¹². This protocol has the potential to be used with a variety of chemicals to determine their effects on mast cell degranulation, and more broadly, their allergic potential.