面向养殖水体分布差异的COD光谱法检测研究

面向养殖水体，传统光谱法对化学需氧量（Chemical Oxygen Demand，COD）检测模型构建的基础：源域（现有样本库）与目标域（检测地水体）间光谱数据独立同分布。但是当源域与目标域分布间存在差异时，由源域得到的低误差模型常在目标域上表现下滑。针对该问题，提出面向UV Vis光谱的域对抗训练网络（DAUVwpNet），将分布不同的源域和目标域数据映射至相同分布的特征空间中，使其在该空间的分布距离尽可能接近，从而在特征空间中对源域训练的目标函数也可以迁移至目标域上，以降低模型在目标域的误差。试验表明：面向同一批测试数据，DAUVwpNet的预测误差为0.78，要低于传统模型的预测误差（0.85）；DAUVwpNet预测值与实测值间相关系数为0.95，要高于传统模型的相关系数（0.89）。表明了该网络能够较好对齐两域特征空间数据分布，降低因分布差异带来的COD检测误差。     

空间矩阵的线性空间性研究

针对矩阵函数求导时产生的情形,提出立体矩阵这一概念,建立起立体矩阵的初步理论知识体系,并总结了立体矩阵的运算的一系列基本性质,构造了实矩阵域,而后考虑了立体矩阵在实数域和矩阵线性空间。     

人工改造野生大豆GsDREB2基因对植物耐盐和耐渗透胁迫能力的影响

DREB (dehydration responsive element binding protein)转录因子是一个干旱应答元件的结合蛋白,它能特异结合启动子中含有DRE/CRT顺式元件,激活逆境诱导基因的表达,调控植物对干旱、低温、高盐、高温等胁迫的耐逆性。大量研究表明DREB转录因子在信号传导、作用机理及基因表达方面存在复杂性。为了野生大豆来源GsDREB2基因能更有效地发挥功能,人工突变该基因的负向调节结构域(negative regulatory domain, NRD,140~204),经改造命名为GsDREB2-mNRD。在酵母中比较全长基因(FLDREB2)和GsDREB2-mNRD转录激活和与DRE元件结合的能力,并验证GsDREB2-mNRD核定位情况。分别将FLDREB2和GsDREB2-mNRD转化拟南芥,通过拟南芥幼苗期盐胁迫和渗透胁迫试验,比较GsDREB2-mNRD和FLDREB2在提高植物耐盐和渗透胁迫方面的差异。结果表明,GsDREB2基因内部存在着负向调节结构域(NRD),抑制了GsDREB2转录激活功能和DRE元件结合的特性;经改造的GsDREB2基因依然能定位在细胞核;超量表达GsDREB2-mNRD基因的拟南芥耐盐和渗透胁迫能力明显强于非转基因对照,也高于FLDREB2基因超表达的拟南芥;野生大豆来源的GsDREB2基因NRD结构域的缺失可增强该基因在植物耐盐、渗透胁迫等逆境胁迫下的功能。     

Identification of the core motif of the BRCA2 C-terminal RAD51-binding domain by comparing canine and human BRCA2

Mammary tumors are the most common tumors in women and non-spayed female dogs. One of the reasons for mammary tumors is mutations of the tumor suppressor gene, BRCA2. BRCA2 participates in homologous recombination repair by interacting with the RAD51 recombinase. BRCA2 has two RAD51-binding domains, consisting of BRC repeats and the C-terminal RAD51-binding domain, respectively. Although several studies have addressed the function of the C-terminal RAD51-binding domain of human BRCA2, the amino acid sequences required for the RAD51-interaction activity remain unclear. In this study, the C-terminal RAD51-binding domains of canine and human BRCA2 were compared; the canine domain displayed a weaker interaction with RAD51. This difference was attributed to the C-terminal portion of the domain via a comparison between canine and human domains. Furthermore, peptides shorter than those previously reported displayed RAD51-interacting activity, and a core motif of this domain consisting of 25 amino acids was identified. Since a mutation (S3323N) was reported in the core motif of this domain, the effect of this mutation was evaluated. The mutant exhibited similar RAD51-binding activity as that of the wild-type protein, suggesting that the mutation was functionally neutral. These data suggested that the C-terminal portion of the BRCA2 C-terminal RAD51-binding domain influenced its RAD51-interaction activity, and a minimum core motif of 25 amino acids was identified in this domain. These data may help clarify BRCA2 function, as well as the tumorigenic effects of BRCA2 mutation.     

Prokaryotic Expression and Antigenicity Analysis of Porcine Japenese Encephalitis Virus Envelope Protein Domain Ⅲ

In order to analyze the antigenicity of porcine Japanese encephalitis virus (JEV) E protein domain Ⅲ, which was expressed by pET-28a vector with His-tag and purified through Ni-NTA, the BALB/c mice were immunized with the purified protein.We identified the antigenicity of domain Ⅲ of E protein and the anti-mice and anti-porcine JEV E Ⅲ protein specific antibody titers by SDS-PAGE, Western blotting, indirect ELISA and IFA.SDS-PAGE results showed the expressed target protein existed mainly in the form of inclusion body.Western blotting, ELISA test results showed that the protein had good reactivity with anti-serum.The mice immunized with the purified JEV E Ⅲ protein generated 1×10⁵ anti-JEV E Ⅲ protein specific antibody titers by ELISA, and the porcine immunized with the porcine JEV generated 5.1×10⁴ anti-JEV specific antibody titers.The IFA results showed that JEV E Ⅲ protein anti-serum could identify JEV antigen.The above results showed that the recombinant JEV E Ⅲ had good antigenicity.These results provided important basis for development of diagnostic antigen for JEV.     

Simulation Propagation of Partial Discharge UHF Signals in Transformer

Many factors affect the propagation of ultra high frequency(UHF) signals caused by partial discharge(PD) on the waveforms and energy of signals in transformer.To investigate the relationshi Pof factors and UHF signals,simulation model of transformer for PD study are established.UHF signals in simulation model of transformer caused by PD are calculated using finite difference time domain method.By means of amplitude and cumulative energy plot of simulation signals,and combing the measured result,the following factors:distance between PD source and detection position,different metallic conductor position around detection position and iron core and winding are researched,which contribute to comprehend the propagation characteristic of UHF signals and detect UHF signals accurately.     

机床传动误差测量中的空域法分析

从空间域的角度讨论了信号处理的一种特殊方法，介绍了它的特点，建立了空域傅氏变换数学模型，并且给出了实用效果。实践证明空域分析法应用于机床传动链一类的特殊场合是有效的。     

基于本体的农业信息服务系统

领域信息服务系统是人工智能领域的一项研究热点.为了让用户及时准确地得到解决方案,解决搜索引擎返回信息过多及问答系统知识瓶颈的问题,提出建立一个用户与专家非实时交流的平台,实现问题咨询与解决方案的双向对应.为此,较全面地分析了农业信息服务系统的系统框架与功能,对其涉及的关键问题-基于本体的农业领域知识库的建立和问题解答过程中问题状态的控制机制进行了深入的讨论.     

陆地棉转录因子GhNAC78基因的特征及功能分析

本实验室从陆地棉中克隆得到GhNAC78,分析了其基因特征及功能。该基因cDNA全长为937 bp,开放阅读框为876bp,编码291个氨基酸,隶属于NAM转录因子亚家族。体外转录激活实验表明,GhNAC78具有转录激活活性。上游启动子区1537 bp序列的生物信息学分析可知其包含多种激素、胁迫和光响应元件,表明GhNAC78广泛地参与植物生长发育和胁迫响应的调控。荧光定量结果显示,GhNAC78在棉花叶片衰老过程中高调表达,推测其参与叶片衰老的调控。     

玉米Gln1-3 gDNA序列分离、基因结构、保守功能域与等位变异分析

谷氨酰胺合成酶家族是高等植物体内氨态氮同化酶, 是植物体内氮利用与循环的核心构件。玉米Gln1-3基因编码叶肉细胞中的细胞质同工酶, 与全株氮向籽粒蛋白质同化与氮利用效率及产量紧密相关。本研究以玉米自交系辽白371为材料, 采用PCR与接头步移(walking)方法分离得到Gln1-3基因区域基因组DNA(gDNA)全长4 571 bp, 起始密码子至终止密码子序列长3 062 bp。将该基因在GenBank注册, 登录号为EU338535, 并进行了详细注释。该基因由10个外显子、9个内含子组成, 剪接方式主要为5′供位保守的GU与3′受位AG模式。编码的GS1蛋白由356个氨基酸组成, 分子量39.2 kD, 等电点 (pI) 为5.202。保守功能域分析表明, 氨基末端外显子2到外显子6为氨离子结合结构域, 羧基末端外显子8与外显子9构成ATP酶结构域, 在胞内行使催化功能。对50个玉米自交系Gln1-3基因重要分析区域进行了等位变异分析, 鉴定出364个等位变异, 其中313个为SNP变异, 占86%。