优异大麦种质资源的抗性鉴定和评价

1998～1999年,将1997年筛选出的191个农艺性状表现优良的大麦品种进行大麦黄花叶病、大麦白粉病、大麦赤霉病、大麦条纹病及耐盐等抗性的鉴定评价,结果表明,抗及高抗大麦黄花叶病品种60份,抗大麦赤霉病品种59份,高抗大麦条纹病品种89份,抗大麦白粉病品种19份,芽期耐盐品种17份,苗期耐盐品种2份.     

优异大麦种质资源的抗性鉴定和评价

1998～1999年,将1997年筛选出的191个农艺性状表现优良的大麦品种进行大麦黄花叶病、大麦白粉病、大麦赤霉病、大麦条纹病及耐盐等抗性的鉴定评价,结果表明,抗及高抗大麦黄花叶病品种60份,抗大麦赤霉病品种59份,高抗大麦条纹病品种89份,抗大麦白粉病品种19份,芽期耐盐品种17份,苗期耐盐品种2份。     

感染大麦黄花叶病毒(BaYMV)的大麦细胞质内含体及细胞器病变的研究

超薄切片电镜观察表明,在感染大麦黄花叶病毒(BaYMV)的大麦(品种“早熟3号”)叶肉细胞中,液泡周围偶而可看到病毒颗粒束,在发病后期黄化或坏死的叶肉细胞中,可见到散布的病毒颗粒。在所有表现症状的病叶叶肉细胞,表皮细胞和木质部薄壁细胞中均可观察到风轮体、束状体、板状集结体以及膜状体等细胞质内含体,未见 卷简体和细胞核内含体。感病初期细胞中,细胞质丰富,核糖体数量增加,内质网肥大,随着病毒症状发喂,叶绿体、线粒体等细胞器逐渐肿大,外膜破裂直至解体。     

干旱胁迫对不同耐旱性大麦品种叶片超微结构的影响

选用耐旱性不同的3个大麦（Hordeum sativum）品种作为研究对象,分析干旱胁迫对其叶肉细胞叶绿体、线粒体和细胞核超微结构的影响。结果表明,3个大麦品种在非胁迫条件下其超微结构无明显差异。遭受干旱胁迫后,不耐旱大麦品种Moroc9-75叶片细胞核中染色质的凝聚程度高,叶绿体变形,外被膜出现较大程度的波浪状和膨胀,同时基粒出现弯曲、膨胀、排列混乱的现象;线粒体外形及膜受到破坏、内部嵴部分消失等。耐旱大麦品种HS41-1叶片细胞中染色质虽出现凝聚,但凝聚程度低;其叶绿体及线粒体与非胁迫条件下基本相似,多数未见明显损伤。耐旱中等的大麦品种Martin叶片超微结构的变化则介于二者之间。因此,干旱胁迫下叶绿体外形、基粒和基质类囊体膜结构的完整性与基粒的排列次序、染色质的凝聚度和线粒体膜及嵴的完整性与大麦的耐旱性相关,这些特性可作为评价大麦耐旱性强弱的形态结构指标。     

干旱胁迫对不同耐旱性大麦品种叶片超微结构的影响

选用耐旱性不同的3个大麦(Hordeum sativum)品种作为研究对象, 分析干旱胁迫对其叶肉细胞叶绿体、线粒体和细胞核超微结构的影响。结果表明, 3个大麦品种在非胁迫条件下其超微结构无明显差异。遭受干旱胁迫后, 不耐旱大麦品种Moroc9-75叶片细胞核中染色质的凝聚程度高, 叶绿体变形, 外被膜出现较大程度的波浪状和膨胀, 同时基粒出现弯曲、膨胀、排列混乱的现象; 线粒体外形及膜受到破坏、内部嵴部分消失等。耐旱大麦品种HS41-1叶片细胞中染色质虽出现凝聚, 但凝聚程度低; 其叶绿体及线粒体与非胁迫条件下基本相似, 多数未见明显损伤。耐旱中等的大麦品种Martin叶片超微结构的变化则介于二者之间。因此, 干旱胁迫下叶绿体外形、基粒和基质类囊体膜结构的完整性与基粒的排列次序、染色质的凝聚度和线粒体膜及嵴的完整性与大麦的耐旱性相关, 这些特性可作为评价大麦耐旱性强弱的形态结构指标。     

大麦条纹花叶病毒新疆株血清学及基因同源性检测

在我国新疆从小麦上分离到的大麦条纹花叶病毒(Barley stripe mosaic Virus,BSMV),可以侵染大麦、小麦、玉米等重要粮食作物。主要以带毒种子传播病毒。大麦、小麦种子带毒率达70％以上。BSMV曾一度使世界主要的大麦产区减产25～30％,是影响农业生产的重要病毒。从预防病害流行和探索该种子传RNA病毒作为植物基因工程载体的可     

大麦赤霉病抗扩展性鉴定与评价

利用禾谷镰刀菌单花滴注接种研究了245份大麦品种对赤霉病抗扩展性。结果表明,大麦赤霉病抗性除了抗初侵染外还存在抗扩展类型。比较了接种后7d、14d和21d的病小穗数和病小穗率以覆由不同期病小穗率获得的病程曲线面积等7个指标性状,并对其进行遗传参数分析,发现21d病小穗率指标在品种间具帔大的变幅、遗传变异系数和遗传率,21d病小穗数和病程曲线面积与病小穗率呈极显著正相关。不同大麦品种抗扩展性表现不一,供试品种中以Suyin21、乌金一号、莆846193、盐97001、96AC20-30五个品种21d病小穗率最低,为高抗品种,占全部供试品种的2．04％。     

大麦麦芽总黄铜类化合物含量的测定分析

采用比色法和标准曲线法测定了国内外63份大麦品种子粒总黄酮和发芽后总黄酮的含量变化,结果表明:不同品种大麦中总黄酮含量(mg/100g)有差异,发芽子粒(59.7±1.10)高于未发芽子粒(51.4±0.87);未发芽品种中:裸大麦(56.3±0.97)高于皮大麦(50.0±0.79),多棱大麦(54.4±0.91)高于二棱大麦(51.1±0.81);发芽品种中:裸大麦(63.2±1.64)高于皮大麦(58.7±0.89),二棱大麦(60.0 4±1.00)高于多棱大麦(57.9±1.60),其中发芽大麦青海黄(79.7±0.98)、澳选2号(83.5±0.36)、甘啤3号总黄酮平均含量高,变异系数分别12.98%、11.98%、4.76%.本试验结果为进一步选育富含黄酮类化合物的大麦品种提供了资源和方法.     

糯大麦与非糯大麦颖果发育过程的解剖学与组织化学研究

为了明确糯大麦与非糯大麦颖果发育的差异,该研究以糯大麦代表性品种(‘白青稞’、‘甘垦5号’)和非糯大麦代表性品种(‘扬农啤10号’和‘苏裸麦1号’)为材料,采用体视显微镜观察、组织化学染色、树脂半薄切片和光学显微镜观察等方法,比较研究了糯大麦与非糯大麦颖果及其胚乳淀粉体发育的过程。结果显示:(1)糯大麦和非糯大麦颖果的形态变化,以及鲜、干重和含水率等的变化规律基本一致,生长曲线均呈"S"型。(2)两类大麦颖果胚乳和果皮的I2/KI染色结果不同,糯大麦胚乳的I2/KI染色结果为红褐色,其果皮被染为蓝黑色,而非糯大麦胚乳和果皮均被I2/KI染成蓝黑色,表明糯大麦和非糯大麦的颖果果皮里直链淀粉含量都较高,且糯大麦胚乳内以支链淀粉为主,而非糯大麦的胚乳内以直链淀粉为主。(3)糯大麦胚乳淀粉体的出现时间早于非糯大麦,且其中小淀粉体的比例高于非糯大麦,淀粉体充实状况也好于非糯大麦。(4)与非糯大麦相比,糯大麦表观直链淀粉以及总淀粉含量较低,但可溶性糖含量较高。研究表明,糯大麦颖果生长规律与非糯大麦类似,但内含物淀粉的积累规律不同。     

大麦麦芽总黄酮类化合物含量的测定分析

采用比色法和标准曲线法测定了国内外63份大麦品种子粒总黄酮和发芽后总黄酮的含量变化,结果表明:不同品种大麦中总黄酮含量(mg/100g)有差异,发芽子粒(59.7±1.10)高于未发芽子粒(51.4±0.87);未发芽品种中:裸大麦(56.3±0.97)高于皮大麦(50.0±0.79),多棱大麦(54.4±0.91)高于二棱大麦(51.1±0.81);发芽品种中:裸大麦(63.2±1.64)高于皮大麦(58.7±0.89),二棱大麦(60.0±1.00)高于多棱大麦(57.9±1.60),其中发芽大麦青海黄(79.7±0.98)、澳选2号(83.5±0.36)、甘啤3号总黄酮平均含量高,变异系数分别12.98%、11.98%、4.76%。本试验结果为进一步选育富含黄酮类化合物的大麦品种提供了资源和方法。     

Preparation and primary application of monoclonal antibodies against a novel ribosome-inactivating protein Moschatin from pumpkin seeds

Plant ribosome-inactivating proteins (RIPs) have multiple biological functions, and have been widely used in the studies on biomedical and agronomic applications. Moschatin is a novel single-chain RIP recently purified from pumpkin seeds, and it has been successfully applied to construct the immunotoxin that can selectively kill the cultured human melanoma cells. Six stable strains of hybridomas (2H8, 4A8, 5B6, 6F8, 4H10 and 6C2) that can secrete high specific monoclonal antibodies against Moschatin have been successfully prepared using hybridoma technique. The isotypes of these monoclonal antibodies are IgG1, IgG1, IgG1, IgG1, IgG2a and IgGM. Their affinity constants were determined to be 1.42x10(8), 2.71x10(8), 8.72x10(7), 2.06x10(8), 1.36x10(8) and 1.51x10(8) M(-1) in a sequent order, measured by non-competitive ELISA. The monoclonal antibody 4A8 has been used to detect Moschatin in Western blot. An immunoaffinity gel, which consisted of a monoclonal antibody 4H10 and Sepharose 4B, was prepared and used to purify Moschatin from pumpkin seeds crude extract.     

人凝血因子Ⅶ单克隆抗体的制备与鉴定

目的：制备抗人凝血因子Ⅶ单克隆抗体并鉴定其特性。方法：应用杂交瘤融合技术,以重组人凝血因子Ⅶ为抗原免疫BALB／c小鼠;取免疫小鼠的脾细胞与Sp2／0骨髓瘤细胞融合,经间接ELISA法筛选、融合细胞有限稀释法克隆、克隆化杂交瘤细胞株的亚类鉴定等方法筛选出单克隆抗体杂交瘤细胞株,并对单克隆抗体的特异性进行鉴定;用杂交瘤细胞株诱生小鼠腹水,应用蛋白A亲和层析法进行单抗的纯化。结果：获得了3株可稳定分泌单克隆抗体的杂交瘤细胞3E8、3D2和1C5,诱生的腹水效价分别为1：1×10^7、1：1×10^6和1：1×10^6;亚类鉴定表明388为IgG2a,其余2株均为IgGl;特异性鉴定显示它们与多种血浆蛋白均无交叉反应,表明单抗是特异的;经过亲和层析,获得了纯化的单抗。结论：获得了特异性的人凝血因子Ⅶ单克隆抗体,为建立人凝血因子Ⅶ检测及纯化方法奠定了基础。     

Human alfa-fetoprotein: isolation and production of monoclonal antibodies.

Alfa-fetoprotein from human cord serum was purified in a single step by hydrophobic interaction chromatography on Phenyl Sepharose CL-4B with a final recovery of alfa-fetoprotein of about 90% and a purification factor of 900. The purified preparation was homogeneous on SDS-PAGE and native PAGE running with a relative molecular weight of 72,000. Monoclonal antibodies against this purified preparation were raised by hybridoma technology using Sp2/0 myeloma cells as a fusion partner. 50% of culture wells exhibited hybrid growth and 7% of these wells contained anti-AFP secreting hybrids. Positive hybrid cells were cloned twice by the limiting dilution method and 8 clones were obtained that secreted monoclonal antibodies. Five of these cell lines (3F6H10, 3F6H4, 3F6H1, 3F6G5 and 3F6G10) were selected at random for purification and characterization purposes. All 5 cell lines secreted monoclonal antibodies of IgG1 subclass which were purified by affinity chromatography on Protein A- Sepharose CL-4B column with a final recovery of 80% and a purification factor of about 13. The purified preparations were homogeneous on SDS-PAGE, native PAGE and IEF. The monoclonal antibodies were highly specific for human alfa-fetoprotein as determined by Western blotting. The affinity constants (K) of these Mab ranged from 10(6) to 10(9) l/mol.     

抗传染性法氏囊病病毒VP5蛋白单克隆抗体的制备与初步应用

原核表达的IBDVGx-VP5蛋白经纯化后免疫8周龄的BALB/c雌性小鼠,三次基础免疫后,融合前加强免疫,取脾细胞在PEG(MW1500)的作用下与SP2/0小鼠骨髓瘤细胞融合,经过三次亚克隆筛选,获得稳定分泌抗VP5蛋白的杂交瘤细胞,分别命名为4B4、6D12、3E8,以三株杂交瘤细胞制备的腹水ELISA效价分别为5×104、3.5×104、3×104,特异性实验表明三株单抗能与IBDVGt株反应。以单抗介导的间接免疫荧光检测表达Gt-VP5的VeroE6细胞,可以见到特异的荧光,能做为特异性的检测VP5蛋白的工具,为今后IBDVVP5蛋白的研究打下基础。     

Production and characterisation of monoclonal anti-idiotype antibody to Vibrio anguillarum

Seven monoclonal anti-idiotype antibodies (mab2) were raised against mouse monoclonal antibody (mab1) 4A6. Identification of subclass showed that 1H5, 1D1, 2B12 and 2F12 belonged to IgG2b, 2H12 and 1H12 to IgG2a and lE10 to IgG3. The titres of these mab2 ascitic fluids ranged from 1 x 10(-4)-1 x 10(-6). The capacity of the mab2 to inhibit the binding between the corresponding rabbit antiserum and Vibrio anguillarum was investigated with the competitive inhibition ELISA. The results showed that mab2 1D1, 1E10, 1H5 and 1H12 were able to inhibit this binding. Another experiment demonstrated that mab2 1D1, 1E10 and 1H5 might induce Balb/c mice to produce Ab3 and these Ab3 competed the same antigen epitopes with Ab1. These results indicate that mab2 1D1, 1E10 and 1H5 are likely to represent an internal image of V. anguillarum and may thus be described as Ab2-beta anti-idiotype antibodies. In protection experiments, Japanese flounders vaccinated with mab21D1, 1E10 and 1H5 showed significantly enhanced survival from challenge with V. anguillarum. Thus. mab21D1, 1E10 and 1H5 may have use as idiotype vaccines for fish in aquaculture.     

Monoclonal antibodies for a comparative serological study of strains of Vibrio anguillarum

Murine monoclonal antibodies against characteristic determinants of heat stable somatic antigens of typical serovar I (820/15/8 Kop) and serovar II (134/82/1 Kiel) of European Vibrio anguillarum strains were produced. Three stable hybridoma cell lines, called aVaI/1F4, aVaI/6F4 and aVaI/2H5, produced monoclonal antibodies each against a typical serovar I determinant of strain 820/15/8 Kop. One hybridoma cell line (aVaII/5A4) producing monoclonal antibodies against Vibrio anguillarum strain 134/82/1 Kiel (serovar. II) was established. Fourteen Vibrio strains and Aeromonas salmoniáda strains were serologically compared by Enzyme-Linked Immunosorbent Assay (Elisa ).     

抗鳗弧菌独特型单克隆抗体的制备及鉴定

利用具有中和活性的抗鳗弧菌单克隆抗体 4A6作为免疫原 ,通过单克隆抗体技术制备出 7株分泌抗独特型单抗的杂交瘤细胞。以ELISA竞争抑制实验及诱导Ab3的功能实验证实 ,其中 4株属于Ab2 β,有可能用于疫苗生产。     

胰腺癌潜在肿瘤标志物的探索及在胰腺癌中的应用

目的:探索胰腺癌新的潜在标志物,建立夹心法ELISA体系,并初步应用于胰腺癌患者的血清检测。方法:应用基质辅助激光解吸电离飞行时间质谱(MALDI-TOF-MS)技术对胰腺癌患者术前后血清进行分析,提纯分析差异蛋白并命名为DAP44,通过杂交瘤技术制备出抗DAP44单克隆抗体,用HRP标记法标记抗体,间接ELISA法检测抗体滴度,用制备出的抗体对胰腺癌组织和癌旁组织进行组化染色,采用夹心ELISA(DAS-ELISA)法制备抗DAP44检测试剂盒,检测胰腺癌病人和正常人血清DAP44值,比较两者差异。结果:对差异蛋白进行肽段测序和生物信息分析,并融合了3株能稳定分泌抗DAP44单克隆抗体的杂交瘤细胞(2D6H5,1E4D6,5B8H12),3株杂交瘤细胞分泌的抗体效价均在107以上,通过抗体配对筛选确定以2D6H5为包被抗体,1E4D6为酶标抗体时,DAS-ELISA法敏感性最高。两株抗体组化染色结果显示:癌组织DAP44表达量远高于癌旁。DAS-ELISA法标准曲线线性范围在0.78-25 ng/mL,检测下线为0.78 ng/mL,此方法检测到的胰腺癌病人和正常人血清DAP44平均含量分别为19.707±1.464和10.653±2.221,两者之间有统计学差异(P0.001)。结论:DAP44可能作为潜在的胰腺癌肿瘤标志物,建立的抗DAP44 DAS-ELISA法体系能够初步用于胰腺癌的临床诊断和疗效评估指标。     

抗吡虫啉单克隆抗体的制备及鉴定

为制备灵敏度高,特异性强的抗吡虫啉单克隆抗体,建立经济、快速、准确的吡虫啉残留免疫学分析方法,采用分子模拟技术分析吡虫啉及其类似农药的电荷分布后,选择1-[6-(2-羧乙硫基-3-吡啶)甲基]-N-硝基-2-咪唑啉亚胺 (H1) 作为免疫半抗原,1-(6-氯-3-吡啶甲基)-3-羧丙基-N-硝基-2-咪唑啉亚胺 (H2) 作为包被半抗原,利用NHS酯法将H1和H2分别与牛血清蛋白 (BSA) 和卵清蛋白 (OVA) 偶联合成免疫原与包被原。免疫BALB/c小鼠后,采用常规杂交瘤技术共获得2株稳定分泌抗吡虫     

Preparation and preliminary application of monoclonal antibodies against Trichokirin-S1, a small ribosome-inactivating peptide from the seeds of Trichosanthes kirilowii

Trichokirin-S1,a small ribosome-inactivating peptide recently purified from the seeds ofTrichosanthes kirilowii,has potential clinical applications because of its small molecular mass.Two stablestrains of hybridomas (1F11 and 2A5) that can secrete highly specific monoclonal antibodies (mAbs) againstTrichokirin-S1 have been developed using the hybridoma technique.The isotypes of these two mAbs,1F11and 2A5,were determined to be IgG_(2a) and IgG_1,respectively.The affinity constants,which were measuredby non-competitive ELISA,were found to be 2.3×10~8 M~(-1) and 2.8×10~8 M~(-1),respectively.An immunoaffinitymethod using 2A5-coupled Sepharose 4B was successfully developed to purify Trichokirin-S1.These twoantibodies have also been used to detect Trichokirin-S1 in Western blot.