真核 的英文怎麼說
中文拼音 [zhēnhé]
真核
英文
eucaryon-
It was suggested that eric - pcr could substitute for rapd in research related to the genetic identification and genetic diversity in auricularia and other edible and medicinal fungi : 2 to a certain extent, genetic differences among auricularia strains tested in this study did not have necessary relativity with their geographical origins respectively ; 3 in this study, genetic diversity in a. polytricha was higher than that in a. auricula : 4 in this study, a. fuscosuccinea had a higher homology to a. auricula than to a. polytricha ; 5 morphological characteristics validated the results from eric - pcr and provided a potential explanation for the higher similarity coefficient between a. auricular and a. fuscosuccinea ; 6 southern hybridization was employed by choosing a strain from a. auricula as a probe which hybridized with a. auricula and a. fuscosuccinea except a. polytricha, further confirming the veracity of the results from eric - pcr ; 7 in this study, isozyme analysis could not cluster the 7 strains from three auricularia species to different groups efficiently ; 8 2 strains from two auricularia species revealed high conservative degree and the restriction fragment patterns by 4 kinds of restricted enzymes showed no diversity
本研究中,木耳屬2個種的2個菌株在its區域表現出較高的保守性, 4種限制型內切酶的酶切圖譜沒有顯示出多態性;增加內切酶種類及供試菌株數量,有可能獲得具有多態性的限制性內切酶酶切圖譜; 9本實驗中, its區域的真菌特異性引物與真核生物通用引物對于擴增效果無較大差異,擴增片段長度均為650bp左右; 10根據形態學實驗、 eric - pcr實驗以及southern雜交實驗的結果分析,紫木木耳屬種質資源的遺傳鑒定和遺傳多樣性評價耳極有可能是毛木耳種的一個變種; n .本研究中所用的gutc法是一種適用於木耳屬菌株基因組洲a快速提取的方法; 12 .傳統的形態學分類法和現代的分子生物學分類法,兩者的關系是相輔相成,互為驗證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。Protective immunity to schistosoma japonicum elicited by co - immunization of cathepsin b dna vaccine with eukaryotic plasmid encoding il
4真核表達質粒聯合免疫誘導小鼠保護性的研究The chromosomes of eukaryotes are nucleoproteins.
真核細胞的染色體是核蛋白。Ciliate, a unicellular protozoa and low eukaryotes in evolution, has perfect vesicular trafficking system among organelles
纖毛蟲是單細胞的原生動物,在進化上屬于低等的真核生物,但其各細胞器之間囊泡運輸系統極為完善。Endoplasmic reticulum ( er ) a system of membranes forming tubular channels and flattened sacs ( cisternae ), running through the cytoplasm of all eukaryotic cells and continuous with the nuclear envelope
內質網:是真核細胞細胞質內的一種管道或扁平囊狀的膜系統,與核膜相連。Homologues of era have been identified in prokaryotes and eukaryotes. there are two domains in era : the n - terminal gtp - binding domain and c - terminal rna binding kh domain. era plays an important role in cell cycle progression at a specific point in the cycle, after chromosome partitioning but before cytokinesis
Era是在原核和真核生物以及植物中普遍存在的g蛋白,是一個結構上既具有gtp結合結構域又有rna結合結構域、不同於ras的獨特的新的g蛋白亞家族。That cell hybridization can be used to dissect regulatory mechanisms controlling gene expression in eukaryotic cells.
雜交細胞能被應用於剖析真核細胞中控制基因表現的調節機理。Compared to the prokaryotic gene expressing systems and mammalian gene expressing systems, insect gene expressing systems possess the stronger ability of the transcription and post - translation processing, which also has high production. we can anticipate it will be a kind of potent effective ectogenesis eukaryotic gene expressing system
與原核表達系統和哺乳動物細胞表達系統比較,昆蟲細胞表達系統既有較強轉錄和翻譯后加工修飾能力,又有高表達量等特點,可望成為基因產業中一種比較理想的外源真核基因表達系統。Cloning and sequecing analyzing of the hemagglutinin gene from influenza a h3n
基因真核表達載體的構建及序列分析In this study five recombinant plasmids containing hn ( hemagglutinin - neuraminidase ) genes of ndv ( newcastle disease virus ) were constructed, hn genes were amplified by reverse transcriptase - polymerase chain reaction ( rt - pcr ) and were inserted directly into eukaryotic expression plasmid pcdna3
應用反轉錄-聚合酶鏈反應( rt - pcr )獲得兩株新城疫病毒( ndv )血凝素-神經氨酸酶( hn )基因cdna ,然後定向插入真核表達質粒pcdna3中,構建了含hn基因的重組質粒。We generated a recombinant eukaryotic gene expressing vector harboring a full - length hgh gene, 2. 4 kb genomic dna with four introns and the signal peptide sequence cloned to the eukaryotic gene expressing vector pcdna3. 0
我們直接將含有4個內含子和自身信號肽的2 . 4kb全長人生長激素基因直接克隆至真核表達載體pcdna3 . 0 ,然後利用脂質體轉染家蠶bmn細胞,瞬時表達hgh 。In eukaryotic cells, dna is located in nucleolus in the form of chromatin by combining with histone proteins
在真核生物中, dna分子纏繞在組蛋白上形成染色質保存在細胞的細胞核中。The cellular homologue of v - src is c - src, and its protein product c - src is located in the cytoplasm with 60kd
隨后在真核細胞中也找到了同源性的c - src蛋白,分子量為60kd ,位於細胞的胞質中。Conclusions : prokaryotic and eukaryocytic expression plasmids of the shortened hepatitis b surface antigen were successfully constracted, and the target proteins expressed by iptg induced in escherichia coli. as well as in eukaryocyte ( hepg2 and cos - 7 ), then their antigenity were detected
結論:截短的乙型肝炎表面抗原分子的原核和真核表達』重組質粒成功被構建及分別在人腸桿菌efl得到誘導表達和存貞核細胞ifj表達,並檢測劍其表達產物的抗原特性。Construction of eukaryotic expression vector of human telomerase reverse transcriptase in immortalized hepatocytes
構建永生化人肝細胞系人端粒酶反轉錄酶真核表達質粒Mitochondria are present in all eukaryotic cells.
一切真核的細胞都有線粒體。It is inferred that its active transcription occurs in the same region, not the nucleoplasm. the result will help us to further comprehend the mechanism of rna polymerase transcription, the way of its transcripts processing and transport, and the structural and functional relationship among the three rna polymeraes
這一結果不僅直觀地向人們表明了rna聚合酶在真核細胞核中的轉錄位點,而且對於人們進一步認識和理解rna聚合酶的轉錄機制、其轉錄產物的加工運輸途徑、以及真核細胞當中不同的rna聚合酶間的組織和調控關系都將有著重要的理論意義。From these results, it is inferred that the active transcription of pol iii occurs in the nucleoli and its periphery region, but not the nucleoplasm. the result will help us to further comprehend the mechanism of rna polymerase iii transcription, the way of its transcripts processing and transport, and the structural and functional relationship among the three rnapolymeraes
本實驗為rna聚合酶在真核生物細胞核中的轉錄位點提供了較為直接的證據,這對人們進一步了解rna聚合酶的轉錄機制、加工和運輸過程及三種rna聚合酶之間的結構與功能關系具有重要的意義。Like eukaryotes, but unlike bacteria, they have introns in their transfer rna, but like bacteria they have polycistronic operons ( gene regulators )
像真核生物而不像細菌,轉運rna中含有內含子,還有細菌不具備的多順反子的操縱子(基因的調控子) 。分享友人