整列插入 的英文怎麼說
中文拼音 [zhěnglièchārù]
整列插入
英文
insert entire column- 整 : Ⅰ形容詞1 (全部在內; 完整) whole; all; complete 2 (整齊) neat; tidy; orderly Ⅱ動詞1 (整理; 整...
- 列 : Ⅰ動1 (排列) arrange; form a line; line up 2 (安排到某類事物之中) list; enter in a list Ⅱ名詞1...
- 插 : 動詞1. (把細長或薄的東西放進、擠入、刺進或穿入; 插上; 插進) stick in; insert 2. (中間加進去; 加進中間去) interpose; insert
- 入 : Ⅰ動詞1 (進來或進去) enter 2 (參加) join; be admitted into; become a member of 3 (合乎) conf...
- 插入 : insert; infix; run in; break in; patch; insertion; plug in; intercalate; intercalation; intromiss...
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In our experiment, the specific fragment was amplified from transgenic bobwhite genome dna at annealing temperature 61 by using high - fidelity pfu dna polymerase and cloned into clone vector pgem - 7fz ( + ), then sequenced. the cloned sequence was completely identical to the sequence which was issued in genbank
本實驗採用了高保真pfudna聚合酶,在退火溫度61條件下從轉基因bobwhite品種基因組dna中擴增出特異性片段,將此片段插入克隆載體pgem - 7fz ( + ) ,經測序和序列分析表明,所擴增得到的片段含有bar基因完整的讀碼框,並且序列與genbank中發表的序列完全一致。According to above consideration, experiments was carried out as below : first, targeted gene - human serum albumin ( hsa ) gene was obtained via pcr technology. secondly, the hsa gene was liganded with a plasmidprla22 whose two arms carry dna sequences necessary for crossing with the human a - lactalbumin yac to form an integration vector prla - hsa, then the integration vector plasmid was co - transformated into the right yac - bearing yeast with another plasmid plrh33 which carrys a selective gene
因此,本試驗首先擴增出整合在酵母基因組里的人血清白蛋白( hsa )基因作為目的基因,並將人血清白蛋白基因插入到一個含有人-乳白蛋白yac同源序列的重組型質粒載體,以構建整合型載體,再與另一個帶篩選基因的質粒共轉化入含人-乳白蛋白yac的酵母細胞體內。Compared with a reported cmv - cp gene sequence, the homology of nucleotide sequences were 100 %. the sequencing result also demonstrated the recombinant vector pet - 22b - cp has a proper orf encoding 218 amino acids. the recombinant vector was transformed into bl21 ( de3 ) cells. transformants were grown and induced by the addition of isothiopropylgalactoside ( iptg ) to a concentration of imm with continued shaking at 37 ?
酶切鑒定及序列測定表明,重組表達質粒pet - 22b - cp連接區域符合設計要求,具有正確的開放閱讀框架,插入片段含有218個氨基酸的完整編碼區,其核苷酸序列與報道的cmv - cp基因的同源性為100 。However, by the time we started collecting index statistics, for example, for the primary key defined on the integer column, there were 10, 000 additional records inserted, hence, the number of rows in the table is 1, 110, 000, and hence the primary index firstkeycard would be 1, 110, 000
但是,在我們開始收集索引統計數據時,例如,對于整型列上所定義的主鍵,就插入了10 , 000條附加記錄,因此,該表中的行數是1 , 110 , 000 ,而主索引firstkeycard將是1 , 110 , 000 。By cheeking the transformed bacterial colonies, we had filtrated the masculine clone successfully. the sequencing result showed that the inserting fragment contained intact coding sequences of dh. pban ( pheromone biosynthesis activating neuropeptide ) and three sgnps ( suboesophageal ganglion neuropeptide ) and the leading frame of it was correct
測序結果表明,重組載體的插入片段中含有dh 、性信息素生物合成激活肽( pheromonebiosynthesisactivatingneuropeptide , pban )及三個食道下神經節肽( suboesophagealganglionneuropeptide , sgnp )的完整的編碼序列,且其閱讀框架( readingframe )完全正確。The insert dna fragments are 7kb and llkb, respectively. two subclones that were designated pgr3h1 and pgr7h1 and can increase glyphosate resistance of e. coli jm109 up to 150mm glyphosate were constructed by subcloning the 2. 4kb and 3. 2 kb hind ? / psti fragments of pgr3 and pgr7 into the corresponding sites of pgem - 3zf and pbluescript. sequence analysis of these two subclones revealed a completely identical 1323bp open reading frame that encodes an epsp synthase
以pgem - 3zf和pbluescript為載體,利用限制性內切酶hind和pst構建這兩個克隆的亞克隆,從中分別得到兩個草甘膦耐受亞克隆pgr3h1和pgr7h1 ,插入片段各為2 . 4kb和3 . 2kb ,對這兩個亞克隆進行序列分析,發現二者均含有一個核苷酸序列完全相同的完整的epsp合成酶基因? ? aroa ,其核苷酸序列長為1323bp ,推導的epsp合成酶由441個氨基酸組成,兩個亞克隆的草甘膦耐受濃度最大可達150mm 。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。分享友人