基于SSA-LSTM-GF的混凝土坝变形预测方法

针对混凝土坝变形分析预测的复杂性,应用相空间重构思想和融合建模理念,提出了一种基于SSA-LSTM-GF的混凝土坝变形分析预测方法。SSA-LSTM-GF方法利用奇异谱分析法(SSA)将变形实测数据序列分解为趋势分量、周期分量和剩余分量,并将剩余分量视为噪声分量予以剔除;采用长短期记忆神经网络(LSTM)模型和高斯拟合(GF)算法分别进行周期分量和趋势分量的分析预测,并将二者结果进行叠加重构,得到最终预测结果。实例验证结果表明,SSA可以达到较好的数据分解和消噪效果,LSTM模型针对周期分量的预测性能优越,GF算法能够很好地实现趋势分量的拟合预测和部分信息的挖掘提取,LSTM模型和GF算法的成果重构效果良好,SSA-LSTM-GF方法具有一定的可行性和应用价值。     

基于荧光SSR标记的紫薇遗传多样性分析

【目的】以收集的239份紫薇属(Lagerstroemia)种质和1份黄薇属(Heimia)种质为材料,开展种质种间特征分析和紫薇种内资源的遗传多样性分析,为进一步优化紫薇种质资源收集保存及合理利用提供科学依据。【方法】基于16对荧光引物鉴定样品基因型,利用GeneMarker软件进行基因型数据的读取;对239份紫薇属种质和1份黄薇属种质进行特征位点分析;并利用Popgene、Cervus、NTSYS和GenAlEx软件对227份紫薇种质进行遗传多样性参数估算、聚类分析和主成分分析。【结果】紫薇(L.indica)种内的特征位点信息最为丰富,其中15个引物所体现出的特征位点信息中,紫薇都有其独特的位点区别于其他6个种,而在福建紫薇(L.limii)、川黔紫薇(L.excelsa)和尾叶紫薇(L.caudata)中也有部分特异的特征位点是紫薇中没有的;16对紫薇SSR荧光引物共检测出143个等位基因,平均每个位点有8.938个等位基因,平均有效等位基因数(N_e)为3.600,Shannon’s信息指数(I)均值为1.459,观测杂合度(H_o)均...     

Morphological,biochemical and molecular changes during ectomycorrhiza development

Summary An ectomycorrhiza, a specialized root organ, is the result of a complex interaction leading to a finely-tuned symbiosis between a plant and a compatible ectomycorrhizal fungus. Ultrastructural observations combined with cytochemical and biochemical studies reveal that structural and metabolic changes in the symbiont cells lead to the final phenotype of the active ectomycorrhiza. In the present review these changes are interpreted as changes in gene expression and discussed within the context of ectomycorrhiza development. Recent genetic data indicate that the continued vegetative growth of the ectomycorrhizal hyphae and the root tissues, and their ability to switch to symbiotic organ formation, is basically controlled by developmentally critical genes. The activity of these symbiotic genes during the differentiation of ectomycorrhizas is associated with extensive changes in the concentration of particular polypeptides and protein biosynthesis. The present state of knowledge about the developmental biology of ectomycorrhizas allows only speculation about the events during their development.Puisant mes forces aux sources des galaxies En buvant la sève des arbres M. Jonasz     

满江红鱼腥藻glnA基因上游调控区的克隆及其序列分析

以满江红鱼腥藻（Ａａｃ）提取总ＤＮＡ为模板,通过ＰＣＲ技术,扩增得到其谷氨酰胺合成酶基因（ｇｌｎＡ）上游区．经酶切得到４０９ｂｐ的片段,并将其连接到ｐＢｌｕｅｓｃｒｉｐｔⅡｋｓ＋上测序．将测序结果与Ａｎａｂａｅｎａ７１２０调控序列比较,有９８２％的同源性．在上游调控中也具有ｎｉｆｌｉｋｅ和Ｅ．ｃｏｌｉｌｉｋｅ启动子,值得注意的是,调节蛋白ＶＦ１的结合位点正好位于ｎｉｆｌｉｋｅ启动子上．所克隆的片段不但对蓝藻固氮、泌氨的基因调控研究具有意义,也对表达载体的构建具有实用价值．     

一种使用非线性循环数列解决堆栈问题的算法

提出了一种使用非线性循环数列解决堆栈问题的算法,对研究栈的性质和求解栈的输出序列具有一定的实用价值。     

扩频系统中自动频率校正单元的设计与实现

针对ＩＳ－９５码分多址蜂窝通信系统标准,给出了一种在从导引信道上提取信道参数并同时获取对载频频差的估计方案,给出了自动频率校正环路的设计方案,及其ＦＰＧＡ实现。该方案简单可行,硬件资源消耗少,且能明显改善移动台接收机的性能。     

Genomic organization of EDSV strain AA-2

The genomic organization of egg drop syndrome virus strain AA-2 isolated in China is reported here. The genome was found to be 32 838 bp in length, approximately 2 kb shorter than those of the human subgenus C adenoviruses. Analysis of open reading frames indicated that the genes for major viral structural proteins (55 K, Penton base, pⅦ, pⅩ, pⅥ, Hexon, 100 K, pⅧ and Fiber), as well as EP, DNA polymerase and ⅣaⅡ are present in the expected locations in the genome. EDSV possesses no identifiable E3 and E4 regions and most proteins encoded by E3 and E4 regions of other adenoviruses genome were not presented in EDSV.     

Cloning, construction of prokaryotic expression vector and expression ofEscherichia coli cytosine deaminase gene

Cytosine deaminase gene ofEscherichia coli strain H-30 was cloned, and its initiation codon of ‘GTG’ was mutated to ‘ATG’ by PCR. Prokaryotic recombinant expression vector pBV220-CD was constructed. Clone with high enzyme activity were selected by detecting their specific activity of cytosine deaminase. 5-FC(5-FC, 5-fluorocytosine) could induce the lethal toxicity to cells containing active CD gene. DNA sequence analysis indicated that there were 16 altered bases and 5 of them resulted in the alteration of amino acids in predicted peptide by comparing DNA sequence of the clone H-30-CD-11 with high enzyme activity with CD gene reported in Gene Bank.     

Research advances in gene therapy for Parkinson's disease

During the long period of time when people have been seeking for an effective therapeutic method for PD, the gene therapy has shown greater and greater advantages over other methods. It can be performed mainly in two ways: ex vivo and in vivo. With the former, TH gene as well as some neurotrophic factor genes (such as GDNF, BNDF genes) can be invited to some cell lines or primary cells thus forming engineered cells and then implanting them into brain. While with the latter, viral vectors including HSV-1, Ad, AAV that can be utilized to construct recombinant viruses, or non-virus vectors can be used to delived DNA into brain directly. The present review summarizes the recent research advances in the gene therapy for PD, and it is reasonable for us to predict a notable progress in prevention and treatment for PD in the next decade.