增序列

The gene regulating sequence of human collagen type Ⅰ is located at 5'end and first intron. The carriers of reporting gene was made, and the function of promoter, enhancer and inhibiter was examined in this study. On the basis of above work, MBP ectopic expression carriers were further built. The result laid a foundation for investigating the feasibility, and validity to specially express MBP gene of human nervous system, in tendon fibroblast.

人Ⅰ型胶原基因调节序列位于5'端和第一内含子，本研究构建了带报告基因的载体并检测了其启动子，增强子和减弱子的功能，以此为基础，进一步构建了MBP异位表达载体，为探索在神经系统少突胶质细胞特异表达的人脑髓鞘碱性蛋白MBP基因转至肌腱成纤维细胞表达的可行性和有效性奠定了基础。

Methods:The expressive plasmids of AML1b and AML1-ETO were transfected into CV-1 and 293 cells.The expression level of endogenous pig7 gene was detected by Realtime-PCR.The luciferase reporter plasmids containing pig7 enhancer/corresponding mutant sequences were constructed and co-transfected into CV-1 cells with expressive plasmids of AML1b and AML1-ETO.The transactivity of pig7 enhancer was assayed by luminometer.

研究方法：AML1b和AML7-ETO表达质粒分别转染及共转染CV-1和293细胞，用Realtime-PCR方法检测上述基因对两种细胞内源性pig7基因mRNA表达水平的影响；构建含AML1b结合位点的pig7基因增强子序列以及相对应的突变位点的荧光素酶报告基因质粒；将表达载体/突变载体与AML1b或AML1-ETO基因瞬时共转染CV-1细胞，分析AML1b、AML1-ETO对报告基因的转录调节作用。

A discrete weighted Hardy inequality is studied, and by proving a refinement lemma, the characterization of the weight sequence ｛ω_｝_(n≥1) in order that the weighted l~-Hardy inequality holds for all nonnegative and nonincreasing sequence c_ is given.

本文研究离散的加权Hardy不等式，通过建立权序列的加细引理，给出了对任何非负非增数列 lp-加权Hardy不等式成立时权序列{ωn}n≥1的特征刻划。

We consider Theorem 1 to be highly significant and apply it to obtaining the rank of a certain augmentation quotient group by proposing Theorem 3 and giving its complete proof.

应用具有Np-序列有限p-群的特殊性质和重量函数，基本序列等概念以及已有的一些结果，分别研究了类为1的pk(k 2)阶A bel基本p-群和类为2的p4阶基本p-群之增广商群Qn的结构，得到了当n足够大时Qn作为A bel基本p-群的秩。

Firstly, it is found that there are many obvious differences between Acorus and Araceae. Their differences are based on many aspects which include characteristics of morphology, anatomy and epidermis of leaf, types of tapetum in anther walls , patterns of endothecial thickenings, and ways of development of endosperms, presence or absence of perisperm, components of photochemistry, and sequences of rbcL.

研究表明：1。菖蒲属与天南星科其它属在叶的形态、结构、表面特征，花药绒毡层类型，药室内壁增厚的特点，胚乳的发育方式，外胚乳的有无，植物化学成分，rbcL基因序列等多方面存在着显著的差异。

According to the classical signal transduction pathway of estrogen, we use Luciferase reporter gene to screen phytoestrogen form Selaginella tamariscina, Pinus massoniana Lamb, Corallodiscus flabellate, Dryopteris sublaeta Ching et Hsu and Leonurus heterophyllus. In this study,the pβgal-Control vector, the pERE-TAL-luc vector, the pCNX2-hERα/pCNX2-hERβvector were transfected into HEK293 cell line. If the components in the herbs combine with the ER, then it could induce the expression of reporter gene controlled by ERE.

根据体内的雌激素信号转导途径，我们选用了以luc为报告基因、ERE为调控序列的重组报告基因载体pERE-TAL-luc，并将其与重组人ERα(humanERα，hERα)表达载体pCXN2-hERα和重组人ERβ(humanERβ，hERβ)表达载体pCXN2-hERβ共转染ER阴性细胞系，建立了靶向ERα或ERβ的细胞水平药物筛选模型，结合小鼠子宫增重实验，对卷柏、松针、益母草、石胆草及贯众等5种中药的植物雌激素作用进行了研究，以期为临床防治更年期综合症等提供准确、科学的实验基础。

In the last part of thesis, primary study of enhancer binding protein was done using yeast one-hybrid system.

在本文的最后一部分，首次应用酵母单杂交系统对痘苗病毒增强子序列在大肠杆菌中的DNA结合蛋白作了初步研究。

It should be pointed out that designing an efficient solution method for a nondifferentiable optimization problem is not an easy task.

作为统一的算法方面的研究，我们可以看到增广的拉格朗日方法可以用来解上述的第一类问题，而基于灵敏度的分析的序列二次规划方法完全有能力解上述的第二类问题。

Erve growth factor combined with its receptor, activated Ras - MAP kinase , mitogen - activated protein kinase kinase is the important regulating factor that make IkB kinase, IKK, phosphated, IkB kinase make the IκBα:(the subunit of NF -κB ) phosphated, the phosphated IkBα degraded, and p65 - p50 heterodimer can be formed, then the heterodimer translocated to nucleus and combined with the promoter domain or other consensus sequence.

GF与其受体相结合，最后可以激活Ras-有丝分裂激活的蛋白激酶途径，有丝分裂激活的蛋白酶激酶(MEKK1)是IγB激酶发生磷酸化的重要调节因子，IKK使NF-κB的亚单位IKBα发生磷酸化，磷酸化的IKBα发生降解，而最后留下p65-p50二聚体，该二聚体然后转位到细胞核内与κB基因的增强子区域或与他的顺式作用序列结合。

A series PCR amplification for differential control strains and DNA samples diluted gradient (1:10) have been used to evaluate the specificity and sensitivity of PCR assay established.Results 1. Detection of GAS by PCR assay: The 345bp specific fragment of speB gene were amplified in all the tested GAS strains including three strains of scarlet fever, whereas it was detected in none of the differential control strains. The lowest limit of detection was 6.5pg genome DNA of GAS strain. 2. Detection of corynebacterium diphtheria by PCR assay: The318bp specific fragment of toxB gene were amplified in all the tested toxigenic corynebacterium diphtheria strains, whereas it was detected in none of the differential control strains. The lowest limit of detection is 850fg/μl genome DNA of corynebacterium diphtheria strain. 3. Detection of Lp by PCR assay: The 340bp specific fragments of mip gene were amplified in all the tested Lp strains, whereas it was detected in none of the differential control strains including three strains of non-pneumophila.

结果：1、用PCR方法检测A组链球菌：以A组链球菌致热性外毒素基因speB为靶序列，设计的扩增引物对全部对照菌株的扩增结果为阴性，而全部A组链球菌参考株均能扩增出特异的345bp片段，其中包括三株猩红热链球菌，检测敏感性为6.5pg／μl DNA.2、用PCR方法检测白喉杆菌：以白喉外毒素基因toxB为靶序列，设计的扩增引物对全部白喉杆菌参考株均能扩增出特异的318bp片段，而全部对照株的扩增结果为阴性，检测敏感性为850fg／μl DNA.3、用PCR方法检测嗜肺军团菌：以嗜肺军团菌巨噬细胞感染增强子基因mip为靶基因，设计的引物对嗜肺军团菌14个血清型参考株均扩增出特异的340bp片段，而鉴别对照株包括三株非嗜肺军团菌均未扩增出任何片段。

increasing progression：递增级数

increasing function 增函数 | increasing progression 递增级数 | increasing sequence 增序列

increasing sequence：增序列

increasing progression 递增级数 | increasing sequence 增序列 | increasing series 递增级数

slowly increasing sequence：缓增序列

slope of a curve 曲线的斜率 | slowly increasing sequence 缓增序列 | small circle 小圆

increasing series：递增级数

increasing sequence 增序列 | increasing series 递增级数 | increasing transfinite sequence 递增超限序列

insulator：绝缘子

绝缘子(insulator)长约几百个核苷酸对,是通常位于启动子同正调控元件(增强子)或负调控因子(为异染色质)之间的一种调控序列. 绝缘子本身对基因的表达既没有正效应,也没有负效应,其作用只是不让其他调控元件对基因的活化效应或失活效应发生作用.

repressor：阻遏蛋白

2 操纵序列 --阻遏蛋白(repressor)的结合位点激活蛋白(activator)可结合启动序列邻近的DNA序列,促进RNA聚合酶与启动序列的结合,增强RNA聚合酶活性. (一)乳糖操纵子(lac operon)的结构TATA盒 GC盒 CAAT盒 2. 增强子(enhancer)

slope of a curve：曲线的斜率

slope line 倾斜线 | slope of a curve 曲线的斜率 | slowly increasing sequence 缓增序列

small circle：小圆

slowly increasing sequence 缓增序列 | small circle 小圆 | small inductive dimension 小归纳维数

XII ARIMA：子菜单项 增倍和加性季节因子分析

......ARIMA子菜单项 综合自回归移动平均分析 | ......XII ARIMA子菜单项 增倍和加性季节因子分析 | ......Seasonal Decomposition子菜单项对时间序列增倍和加性季节因子分析

enhancer：增強子 增强子

2.增强子 增强子(enhancer)是另一种与基因表达有关的调控序列. 它可使启动子发动转录的能力大大增强,从而显著地提高基因的转录效率. 增强子多为重复序列,一般长约50bp,不同基因中的增强子序列差别较大,但含有一个基本的核心序列,