家蚕微孢子虫
- 网络nosema bombycis;Nosema Bombycis Naegeli
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家蚕微孢子虫PCR检测的研究
Studies on PCR amplification of DNA of pebrine spore Nosema bombycis from silkworm , bombyx mori
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家蚕微孢子虫(NosemaBombycis)表面蛋白提取法研究
Study on the extraction of surface protein of Nosema bombycis
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重度感染家蚕微孢子虫的家蚕丝腺cDNA文库构建及EST测序分析
CDNA Library Construction and EST Analysis of Bombyx mori Silk Gland Heavily Infected by Nosema bombycis
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家蚕微孢子虫cDNA文库的构建及部分EST同源性分析
Construction of Nosema bombycis ( N.b ) cDNA Library and Analysis of ESTs Sequence From Partial Clones
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家蚕微孢子虫(NosemaBombycis)孢壁蛋白提取方法的优化研究
Extraction of Spore Wall Proteins of Nosema bombycis With Improved Methods
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设计1对正、反向引物btubf/btubr,对家蚕微孢子虫(镇江株)基因组DNA的β-微管蛋白(beta-tubulin)基因进行扩增,得到部分片段。
A beta-tubulin DNA fragment of the Zhenjiang strain of Nosema bombycis was obtained by primers btubf / btubr .
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从这55个基因中随机抽取4个进行Southern杂交实验,结果表明这些水平转移基因确实存在于家蚕微孢子虫的基因组上,而非外来污染序列。
We randomly chose four of them to carry out the Southern blot , and the result shows that these genes exist in the genome of N. bombycis rather than the contamination . 2 .
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孢子大小比家蚕微孢子虫(NosemaBombycis)略小。
Compared to Nosema Bombycis , it has a slightly smaller spore size .
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35℃高温对家蚕微孢子虫在BmN细胞中发育、增殖的抑制
Inhibition of 35 ℃ on the Development and Propagation of the Nosema bombycis in BmN Cells
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用铬变素2R法对家蚕微孢子虫孢子染色的研究
Determination of Horseradish Peroxidase Based on Enzymatic Reaction Using Chromotrope 2R as Substrate Study on the Staining of Spores of Nosema bombycis by Chromotrope 2R Method
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serpin基因拷贝与片段重复及转座元件的相关性分析表明,在家蚕微孢子虫11个serpin中,有6个基因与转座元件存在极显著相关性,有两对基因是片段重复产生的多拷贝。
The relative analysis between serpins and segmental duplications and transposable elements indicated that there are six out of eleven serpins have significant correlation to the TEs , and two pairs of serpins were produced by segmental duplication .
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家蚕微孢子虫转宿主果蝇的研究初探
Primary Study on Nosema bombycis Infecting the Insect of Drosophila
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家蚕微孢子虫N.bombycis分离纯化方法的优化
Optimization of the procedures of isolation and purification of Nosema bombycis in silkworm
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家蚕微孢子虫细菌人工染色体文库的构建
Construction and Analysis of Bacterial Artificial Chromosome ( BAC ) Library of Nosema bombycis
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家蚕微孢子虫单抗金银染色法检测技术的研究
Studies on the monoclonal antibody based immunogold-silver staining method for detecting spores of Nosema bombycis
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因此,我们推测家蚕微孢子虫可能在入侵过程中会分泌类枯草杆菌蛋白酶,通过降解昆虫体壁帮助其入侵宿主细胞。
So we speculate that subtilisin-like protease in N. bombycis may participate in the process of invasion .
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家蚕微孢子虫孢壁蛋白的研究有助于阐明微孢子虫的侵染机制,从而可以为微粒子病的防治提供作用靶标。
The research on spore wall proteins is helpful to explain infective mechanism and provide a tool to prevent pebrine .
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截止目前,家蚕微孢子虫的检测经历了以下阶段:显微镜检、分子生物学检测、免疫学检测。
The history of N. bombycis detection experienced the following phases : microscopic examination , molecular biology detection , immunology detection .
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随着家蚕微孢子虫基因组测序的完成,通过序列比对发现在家蚕微孢子虫中也存在类枯草杆菌蛋白酶。
With the completion of genome sequence project of Nosema bombycis , it was found that subtilisin-like protease ( SLP ) also exist in this species .
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目前在家蚕微孢子虫中仅鉴定报道5个孢壁蛋白,因此有待于新的孢壁蛋白鉴定。
To date , just a total of five spore wall proteins have been characterized in Nosema bombycis , thus it is time for us to identify new ones .
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家蚕病原性微孢子虫的超微结构研究
Studies on the Ultrastructure of Microsporidias Pathogenic to Silkworm Bombyx mori
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家蚕3种微孢子虫孢子表面抗原特性的研究
A study on the spore surface antigen specificity of 3 Microsporidians of silkworm
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家蚕病原性微孢子虫孢子表面蛋白的选择性分离与总蛋白比较分析
Selective separation of EXOSPORAL protein and comparative analysis of total Sporal proteins of Microsporidias Pathogenic to silkworm Bombyx mori
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胎牛血清及热处理家蚕体液对家蚕微孢子虫体外增殖的影响
Effects of FBS and Inactived Silkworm Hemolymph on the Development and Multiplication of the Nosema Bombycis in vitro
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本研究就是以快速检测家蚕微粒子病为实验目的,制备家蚕微孢子虫的单克隆抗体,并初步探讨抗体在家蚕微孢子虫的快速检测上的可能应用。
In this study , we prepared monoclonal antibodies ( MAbs ) against N. bombycis and investigated the application of this antibody to rapid detection of silkworm pebrine .
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为促进用PCR法检测家蚕微粒子病的生产应用,对带毒蚕卵中的家蚕微孢子虫DNA提取方法进行了研究。
The method for extracting Nosema bombycis DNA from Bombyx mori eggs infected with Nosema bombycis was studied to approach the feasible application of detecting through PCR .