寡核苷酸酶 的英文怎麼說
中文拼音 [guǎhésuān]
寡核苷酸酶
英文
oligonucleotidase-
Degenerate oligonucleotides to highly conserved regions of cucumis melo 1 - aminocyclopropane - 1 - carboxylic acid ( acc ) oxidase gene were used to prime the amplification of fragment of 128bp by ploymerase chain reaction ( pcr ) in samples of genomic dna from fruit of cucumis melo l. cv hetao flesh, which was cloned into plasmid vector pmd - 18 - t. the clon of antisense orientation were selected, and it was inserted downstream of camv35s promoter and enhancer " " of tmv into the plant expression vector pbinyxw, antisence expression vector pbinya was constructed. at the base that pollination and fertilization of cucumis melo l. cv hetao was studied, using pollen tube pathway transformate cucumis melo l. cv hetao, 76 fruit had been obtained, moreover, hardness and content of sugar were analysed
本實驗以河套蜜瓜果肉基因組dna為模板,用甜瓜acc氧化酶基因特異寡核苷酸鏈為引物進行pcr擴增,得到128bp的擴增產物。將得到的擴增產物克隆到質粒載體pmd - 18 - t上,篩選反向克隆,然後將其反向構建到植物表達載體pbinyxw的camv35s啟動子和tmv增強子「 」的下游,構建成反義表達載體pbinya 。並在對河套蜜瓜授粉受精生物學研究的基礎上,通過花粉管通道法轉化河套蜜瓜,共獲76顆瓜,並進行了硬度和含糖量的分析。Inhibitory effects of heparinase antisense oligodeoxynucleotides on growth of human malignant melanoma trans planted subcutaneously in nude mice
乙酰肝素酶反義寡核苷酸對人惡性黑素瘤裸鼠皮下移植瘤抑制作用的研究The results showed mn and ni complexes possibly bind to dna by the mode of interaction, whereas zn complex possibly bind to dna by the modes of interaction and electrostatic binding. 5. in addition, we conjugated cleavage system with recognize system and analyzed joint products by hplc, which provide experimental basic for design of dual effects cleavage
此外,本文還選用咖啡酸純品來突破切割體系與識別體系(用氨基臂修飾的寡聚脫氧核苷酸)的連接,並用高效液相色譜法分析其偶聯產物,為今後設計併合成一種具有特異識別和高效切割雙重功能的人工核酸酶提供了實驗基礎。A pair of primers was designed based on the conserved regions of other higher plants " epsp synthase through homology alignments. two dna fragments were first cloned from o. violaceus by performing prc which used o. violaceus genome as the template. one has 798 nucleotides and the other 1157 nucleotides, but they can encode the same amino acid sequence and have same extrons according to the gt - ag rule of characteristic sequence of enkaryoutic intron
根據同源比較其它高等植物中epsp合成酶基因,找出該基因的保守序列並設計一對寡核苷酸引物,以諸葛菜的總dna為模板進行pcr反應,克隆出了兩個epsps基因的片段,其中一條長為797bp ,另一條1157bp ,它們在genbank的登錄號為: af440390 、 af440391 。Rapd ( random amplified polymorphic dna ), which bases on the polymerase chain reaction ( pcr ), is by far one of the most commonly molecular techniques to uncover dna sequence polymorphisms. the basic priciple of this technique is that an arbitrary primer ( usually lobp oligonudetide ) is used to amplify random segments of dna, and a small number of fragments will be amplified when the primer anneals on each strand over a length range. if sequence variation is present at the priming site, then a fragment may not be amplied, so the dna polymorphic can be detected
Rapd (隨機擴增多態性dna )技術是二十世紀90年代發展起來的一項dna分子多態性檢測技術,它建立於聚合酶鏈式反應( pcr )技術基礎之上,利用隨機合成的寡聚核苷酸序列為引物(一般為10個bp ) ,分別與dna的兩條單鏈結合,在dna聚合酶的作用下,對基因組的特定區域進行pcr擴增,其電泳結果為不同大小和數目的dna譜帶即rapd圖譜,可反映基因組相應區域的dna多態性。A reverse - transcriptase polymerase chain reaction ( rt - pcr ) based technique was developed to detect newcastle disease virus ( ndv ) of different poultry species origin. four oligonucleotide primers, based on the differences of nucleotide sequence at the cleavage site of fusion ( f ) protein gene between virulent and non - virulent strains of apmv - 1, were designed to amplify specific dna fragment from different viruses
依據apmv - 1融合蛋白( f )基因裂解位點的核苷酸序列與其毒力的相關規律,分別設計合成了四條寡核苷酸引物,建立了一個可迅速檢測不同禽源apmv - 1並可鑒定強、弱毒株的逆轉錄酶?聚合酶鏈式反應( rt - pcr )技術。And the two pah ' s of pcr primers that bind to the adapter and the sequence of f fragment close by tn5 respectively were also designed. the genomic dna of b8 was isolated, digested with bamh i, and ligated to the adapter. using the two pairs of the primers, two rounds of pcr were performed hi turn and a fragment of 239bp was amplified successfully. lt was proved by cloning and sequencing that 18bp of the fragment is the sequence opposite to f fragment on the left of tn5 insertion site in b8f, the other is part of the 728 bp of f fragment. this result makes it possible to continue to carry out chromosome walking, to clone and sequence the whole genes of b fragment and f fragment, and to reveal the antagonistic molecular mechanism of b8
試驗研究設計併合成了由40和44個堿基的寡聚脫氧核苷酸組成的染色體爬行接頭,在接頭序列和測定的f片段近tn5的序列上,設計了2對染色體爬行用的pcr引物,從b8菌株中提取基因組dna , bamhi酶切,與染色體爬行接頭連接,依次用2對引物進行pcr ,擴增出239bp產物,經克隆、測序,發現其中18bp為擴增的相應于f片段在b8f菌株tn5插入位點對面的序列,其餘則為f片段728bp序列的一部分,為進一步進行染色體爬行,克隆和測定整個b和f基因,揭示陽菌株的拮抗分子機制提供了技術資料貯備。Neuronal nitric oxide synthase antisense oligodeoxynuleotide attenuates morphine withdrawal symptoms in rats
神經元型一氧化氮合酶反義寡脫氧核苷酸抑制大鼠嗎啡戒斷癥狀分享友人