核表法 的英文怎麼說
中文拼音 [hébiǎofǎ]
核表法
英文
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The problem of calculating the core attributes of a dicision table is studied, a new discernibility matrix and the computation of core is put forward in this paper, and correctness of this method is proved. this method is the same with consistent and antipathic dicision tables
論文對目前求核方法存在的問題進行了分析,提出了一種新的可區分矩陣與求核方法,並證明了方法的正確性,該方法適用於任何決策表(相容的或不相容的) 。In the experiment, the full code sequence of bar gene was cloned by pcr from transgenic herbicide resistant bobwhite wheat and checked. it was expressed in e. coli and its protein was determined. after having been properly modified, the bar gene which correctly codes pat was cloned into binary vector pbi121 and then transferred into lba4404 by triparantal crossing, which is the prerequisite work for genetic transformation
本實驗從抗除草劑轉基因bobwhite小麥中,利用pcr克隆的方法擴增出bar基因全長,並在原核表達系統中表達,鑒定表達蛋白的活性,將能夠正確編碼ppt乙酰轉移酶的bar基因片段,經過適當的修飾構建入真核表達載體。On the other hand, - 6 fatty acid desaturase injection assay will be performed to check whether a metabolic pathway is established. methords of research three plasmids vector with expression elements are used to establish a eucaryotic expression vector by restriction enzyme cutting and ligation. this vector is used to pronucleus microinjection
本實驗以pegfp - n1質粒為骨架載體,用酶切連接的方法構建一個順序含有- actin啟動子、 fad2cdna 、 sv40polya加尾信號的真核表達載體,雙切線性化后回收,使用回收的表達載體經原核顯微注射生產轉基因小鼠。The purpose of this study was to clone the major structural protein vp3 gene of gpv hl isolate after pcr, and express by protokaryotic and eukaryotic expressing system, then develop molecuiar diagnostic reagent of goose piaque and construct recombillat fowlpox vina life vector vaccine
利用pcr方法擴增和克隆gpvh1分離株主要免疫原性蛋白基因vp3 ,並對其進行原核和真核表達,是建立小鵝瘟分子診斷方法、構建vp3基因重組禽痘病毒活載體疫苗的基礎,具有極為重要理論和實踐意義。We successfully construct the eukaryotic expression vector of gfp - eif - 5a and its mutational vector using genetic engineering techniques. we found that eef - 5 a localized in nucleus as well as in cytoplasm just for a short time after its transient expression, then distributed only in cytoplasm
Eif - 5a的hypusine修飾是其活性和功能發揮所必需的,我們通過pcr方法實現了hypusine位點的定點突變,並進一步構建了含gfp標簽的eif - 5a及其hypusine位點突變的真核表達載體。Various concentrations of rrta and rrta - yqrl were added into the wells and incubated for 6 h to allow internalization of toxins by fluid - phase endocytosis. the cells were then incubated in rpmi - 1640 medium containing 10 % fetal calf serum for another 24 h
結論本實驗用基因工程方法原核表達了rl 』 a蛋白和rl 』 a一yqrl蛋白,利用rta蛋白和f3ga的結合特性,溫和、簡單、有效地洗脫了目的蛋白。In this paper, phylogenetic relationship of 13 species involved in 6 genera of cruciferae wer e carried out through both the clones of homologous sequences with the primers designed on the basis of conserved regions of cyp86mf gene in cytochrome p450 gene superfamily and the differential analyses of them. meanwhile, complete sequences of some genes in cytochrome p450 gene superfamily were isolated and identified by smart pcr - race strategy, and expressed in e. colt. the results were as follows : ( 1 ) isolated by pcr from 11 species of cruciferae, eleven homologous gene segments that deduced amino acids were identities of over 80 % at nucleotide sequence level and similarities of over 70 % at amino acid sequence level
本論文以已知的細胞色素p450基因超家族成員cyp86mf基因的保守區設計引物對十字花科重要蔬菜作物的6個屬13個物種進行了同源序列的分離克隆,通過核酸序列的差異比較分析,研究了該基因在不同物種中的進化關系;同時,通過保守引物的pcr擴增和race相結合的方法對十字花科植物不同物種的細胞色素p450基因家族成員基因全長進行了分離克隆、鑒定和原核表達的研究,獲得如下研究結果: ( 1 )通過pcr從十字花科植物不同物種中擴增到11個可以推導出完整氨基酸序列的同源片段。Thus, immunologists have sought smaller molecules with the antigen - recognition capability of antibodies. the variable domains of the heavy ( h ) and light ( l ) chains are sufficient for antigen recognition but the non - covalent complex of the two variable domains ( fv ) is unstable. it is possible to genetically engineer a single - chain fv ( scfv ) with the h chain v region connected to the l chain v region via a 15 amino acid linker composed of serine and glycine amino acid residues
二、日本血吸蟲單克隆杭獨特型抗體np30的單鏈狐( scf )的構建、表達及對balbic小鼠誘導保護性作用研究l 、日本血吸蟲單克隆杭獨特型抗體np0的單鏈抗體歸cfv )的構建、表達通過pcr方法體外擴增並經測序驗證的重鏈、輕鏈可變區( vh 、 vl )基因先後重組入原核表達質粒ptha90相應的位點上,中間通過一連接肽( gly在er ) 。Dla advised that having considered the comments of the review committee and to avoid possible perception of conflict of interest, the department would avoid as far as possible instructing counsel who had represented the legal aid appellant at appeal hearings to represent lad at review committee hearings
經考慮覆核委員會的意見,和為避免產生利益沖突的嫌疑,法援署署長表明法援署會盡量避免委派曾在上訴聆訊代表法律援助上訴人的大律師在覆核委員會聆訊時代表法援署。Salmonella typhimuriwn, one of the invasive bacterial species, can be attenuated without loss of invasiveness and thus used for delivery of eukaryotic expression vectors into host cells in vivo. the recombinant plasmid containing the target gene is released inside the host cells and gain entry into the nucleus, resulting in expression of encoded antigens and subsequent induction of humoral and cellular immune responses
沙門氏菌( salmonellatyphimurium )是一種較為常見的侵襲性胞內菌,通過基因工程方法減毒后對宿主致病性顯著降低,但仍保留良好的侵襲力,可直接將真核表達質粒攜帶進入動物細胞內表達相應的蛋白而誘導特異性的免疫應答反應。After the analysis, we raise several questions and go for an in - depth discussion. then we put forward our suggestion that standards of pe shall be made according to various positions and objectives and the employees who will be evaluated shall also have a voice in making the standards to improve its acceptability. the new pe system is objective oriented by mixed standards system and compellent distributed system etc. through careful analysis, the author hope to show us the function of pe system should not only limited to a summary of past work, but also a control beforehand as well as improve employees " performance and reinforce pe management
論文從績效考核的基本理論、方法出發,通過對改制后的xt公司培訓體系的全面分析,以及對培訓組織的原有考核標準、方法等的剖析,提出了原有的考核存在的幾個問題,並就這幾個問題深入展開討論,對績效考核指標的確定提出了新的要求,即根據績效期內的工作目標確定考核指標以及被考核者參與制定考核標準與權重,以達到高接受性的目的;應用目標管理法、混合標準量表法等方法制定出以目標為導向的績效考核方案。The modified sequence was cloned into binary vector pbi121. the constructed expression vector was named pbi121 - bar, then transferred into agrobacterium tumefaciens lba4404 by triparental crossing. thus the project bacterium has been successfully constructed
改造后的目的基因克隆于真核表達載體pbi121 ,構建表達載體pbi121 - bar ,通過三親雜交法將真核表達載體pbi121 - bar轉入農桿菌lba4404 ,成功構建出工程菌。Considering different microstructures and properties of metal of hardened layer and the core of back - up roller, the distributions of shear stress below surface and the contact stress between work roller and back - up roller of a four - high - mill were simulated with nonlinear fem
摘要考慮軋輥表面淬硬層與其心部金屬材料組織性能的差別,採用非線性有限元方法對四輥軋機的工作輥與支撐輥間接觸應力及輥內剪應力分佈進行模擬,並將模擬結果與傳統強度校核方法進行了對比分析,研究了軋輥淬硬層厚度對輥間接觸應力的影響規律。Purpose 1 construction of prokaryotic high expression vector of human platelet factor 4 ( h pf4 ) 2 expression and purification of r h pf4 3 bioassay of r h pf4 methods according to the modulation character of eukaryotic protein expression in prokaryotic cells, we design a pair of particular primers, and construct a prokaryotic expression vector pbv220 - r hpf4 by dna polymerase chain reaction ( pcr ) and dna recombinant technic. the expression plasmid was identified with pcr and dna sequencing. pbv220 - r hpf4 was transformed into e. coli dh5a, bl21 ( de3 ) and induced by increasing the temperature to 42. we identified the expression protein by sds - page and western - blotting
目的1人血小板因子4 ( hpf4 )原核高效表達克隆的構建2重組hpf4的表達及分離、純化工藝研究3重組hpf4的特性研究方法根據原核細胞表達真核蛋白的基因表達調控特點,設計合成一對特異引物,在pt7 - 7 - rpf4表達質粒的基礎上,應用聚合酶鏈式反應( pcr )對其cdna進行改造,通過dna重組技術構建成重組hpf4原核表達質粒pbv220 - rhpf4 ,用快速pcr檢測法、 dna測序分析,鑒定重組hpf4表達質粒的正確性。Thirdly, by the method of questionnaire and quality control tools, the buying and selling process quality control proposal is given in this article, thereby, the analytical methods of quality control including the acceptance criterion of wheat, the process capacity of supply and customer satisfaction indexes evaluation are discussed in this article. fourthly, based on the methods of statistical process control, this article evaluate the factor that have a impact on the process of the stored grain with qualitative analysis and quantitative analysis, and bring forward the design proposal of controlling temperature for stored grain in warehouse. at last, in order to bring the optimization design for quality management system into effect and advance the enterprise in overall management, the article table a proposal including strengthening the training of quality management, introducing iso9000 standard into quality management, bringing about the grain industrialization, standardizing quality inspection criterion, developing the computer auxiliary control system
首先依照iso9001標準,藉助于設計的專家調查表通過專家調查,對該糧庫的質量管理體系現狀進行詳細分析,確定出質量管理體系文件、資源管理、產品實現過程、質量控制和質量改進五個方面存在的主要問題;其次運用系統方法建立了糧庫質量管理體系完善程序及質量管理體系的三維空間結構模型,並在此基礎上優化設計出了質量管理體系內部審核、不合格控制、糾正和預防措施等質量改進實施方案;再次,運用調查表法和質量管理控制工具對該糧庫的糧食輪換過程的質量控制進行了優化設計,確定出糧食采購標準、供應過程能力分析以及顧客滿意度評價等分析方案;然後,運用統計過程分析方法對糧食倉儲過程的影響因素及其原因進行定性和定量分析評價,確定出倉儲過程質量控制的優化方案;最後,為確保設計方案的有效實施,從糧庫加強質量管理培訓、導入iso9000族標準、糧食產業化開發、規范糧食質量檢驗標準、開發計算機輔助控制系統五個方面提出具體實施建議,以便提高其整體質量管理水平。They cannot naturally produce essential fatty acids - beneficial nutrients found mainly in plant and fish oil, so they must rely on a dietary supply. here we want to establish transgenic mice carry a tissue - specific expression gossypium hirsutum - 6 fatty acid desaturase ( fad2 ) gene which can add a double bond into an monosaturated fatty - acid hydrocarbon chain and convert oleic acid to linoleic
本試驗試圖構建一個肌肉組織特性的- 6脂肪酸去飽和酶(脫氫酶)真核表達載體,通過原核顯微注射法把棉花的- 6脂肪酸去飽和酶導入到小鼠體內,以小鼠為動物模型,建立動物體內的必需脂肪酸合成代謝通路。The paper systematically introduces the evaporation, nucleation, condensation and agglomeration of mineral and trace element in pulverized coal combustion and analyzes the research review of the formation of submicron particles
本文系統的綜述了煤燃燒過程中礦物質和痕量元素的氣化、冷凝成核、表面凝結、團聚的機理、模擬和預測方法以及細粒子形成機理的研究進展。It has not only many advantages of the prokaryotic expression system such as growing quickly, manipulating easily, strong power to express and control foreign protein, but also the ability to make foreign protein modified in post - translation. so pichia pastoris gene expression system is more appropriate to express many eukoryotic proteins than prokaryotic system and has attracted more and more people " s attention on it
它不僅具有原核表達系統生長快速,操作簡單,外源基因表達量大並受到嚴格調控等特點,還具有真核生物特有的蛋白質翻譯后修飾的功能,表達真核生物蛋白質具有原核表達系統無法比擬的優越性。The concrete design method of the votating speed difference frequency fuzzy controller is studied in detail. based on single - chip microcomputer 8031, using table look - up method, votating speed difference frequency fuzzy controller applied to induction motors is implemented. simulation result demonstrates that the control result for the producing plastic flat yarn of votating speed difference frequency fuzzy control to the speed of induction motors is idealer
本文對轉差頻率模糊控制器的具體設計方法進行了討論:以單片機為核心,用查表法實現異步電動機轉差頻率模糊控制;最後,結合工廠塑料平膜拉絲機驅動電機參數對系統進行了模擬,分析了轉差頻率模糊控制對異步電動機轉速的控制效果,結果是比較理想的。These include cell growth characteristics, expression levels, intracellular and extracellular expression, posttranslational modifications, and biological activity of the protein of interest, as well as regulatory issues in the production of therapeutic proteins. in addition, the selection of a particular expression system requires a cost breakdown in terms of process, design, and other economic considerations. section i : construction of pet22b ( + ) / hpk - 5 vector the hpk - 5 gene encoding 82 amino acid residues from c462 to c543 was recombined with the sequence of plasmid pet22b ( + ) for constructed a new expressed vector pet / hpk - 5
方法在對hpk - 5 ( humanplasminogenkringle5 , hpk - 5 )因子的基因序列和蛋白質序列進行分析的基礎上,利用pcr技術分別構建其可溶性原核表達載體和不溶性原核表達載體;用pcr快速檢測法及其基因測序儀測序以鑒定pet22b hpk - 5和pbv220 hpk - 5重組質粒,用不同的感受態大腸桿菌( e分享友人