gene probe 中文意思是什麼
gene probe
解釋
基因探針-
Screening target ' gene of artemisinin antimalarials using drug - western from cdna expressing library : 12 b - deoxoartemisinyl - ( 4 ' - oxyacetic acid ) phenyl ether was linked to bsa by using of edc cross ! inker and the product acted as drug - probe
對重組pmd一18一t克隆載體及pqe一30表達載體雙酶切,提取tctp基因和pqe一30空載體並使二者重組,然後轉化m15 ,挑取陽 -
The data above showed that algae phycobiliprotein fluorescent probes not only facilitate the study to pea actins but also provide a doable method to label other plant proteins. it has a good foreground for algae fluorescence probe to be used in the immunity fluorescent detection of plant cells. the gene clon
對豌豆肌動蛋白藻熒光探針的初步研究,不僅為豌豆肌動蛋白的免疫熒光檢測提供了便利條件,而且通過改變抗體,則可以將藻熒光探針用於其他植物蛋白的標記,藻熒光探針優越的熒光特性使其在植物材料的免疫熒光檢測中具有廣闊的應用前景。 -
In this study, the meaningful results have been achieved, which is the important basic work to research the pili subunit vaccine of avian e. coli, and detect pila gene by nucleric acid probe. moreover, it is significant to research molecular epidemiology, to diagnose, to prevent and treat avian colibacillosis
本研究為雞源致病性大腸桿菌菌毛基因工程疫苗的研究,制備核酸探針檢測pila基因提供了重要材料,對雞大腸桿菌病的分子流行病學研究、診斷和防治研究具有重要意義。 -
We designed a suitable probe in the experiment and used ribonuclease protection assay technology to detect the expression of pdipl gene in mouse liver at different time points after partial hepatectomy. we found that the expression of pdipl gene was increased. it reached the highest level after 12 hours and then decreased
我們設計合適的探針,採用核酸酶保護反應等技術測定了pdip1 -基因在肝臟部分切除后不同時間在小鼠肝臟中的表達,發現pdip1 -基因在肝臟部分切除后表達增強, 12小時表達最強,以後表達減弱。 -
The loop sequence of mb1 and mb2 were the anti sense and sense sequence ofing1, respectively the sequence of mb3 was a piece of ssrna sequence in tobacco mosaic virus, which had no analogical to human gene. mbl was the most suitable probe because mbl had the highest fluorescence enhancemen after hybridizing wtth rna extrated froin normal cell
第三章,根據一種常見的病毒煙草花葉病毒( tmv )的核酸序列設計了分子信標熒光探針,由於tmv的遺傳物質是rna ,分子信標又具有很高的特異性和靈敏度,因此感染了病毒粒子的植物葉片在經過簡單處理后,可用分子信標檢測葉片上。 -
To dress the question if other virulence gene were present in this kind of strains, 152 of 436 irp2 - hybridized strains were re - confirmed and selected for this study. the virulence genes or putative virulence genes detected by pcr or hybridization include heat stable toxin ( st ) & heat labile toxin ( lt ) for enterotoxigenic e. coli ( etec ), invasive plasmid antigen b ( ipab ) for enteroinvasive e. coli ( eiec ), epec adherence factor ( eaf ), epec secretion protein c ( espc ) for enteropathogenic e. coli ( epec ), hemolysin ( hlya ) and shiga toxins ( sltl and slt2 ) for enterohaemorrhagic e. coli ( ehec ) and eaggec probe for entero - aggregative e. coli ( eaggec ). the prra and yc73 genes of pathogenicity associated island ( pai ) of urepathogenic e. coli ( upec ) and " o " island 28 ( rtx 615 ) gene was also detected, the later was a newly discovered putative pathogenicity island in e. coli o157 : h7
為探討攜帶小腸結腸炎耶爾森氏菌的hpi毒力島的大腸桿菌是否具有其他已知的毒力基因,選取82株由原位雜交和pcr方法初篩irp2陽性的大腸桿菌菌株,進行在致瀉性大腸桿菌的25個毒力基因的檢測,包括腸產毒性大腸桿菌的熱穩定毒素st和熱不穩定毒素lt ,腸侵襲性大腸桿菌的侵襲蛋白b基因ipab ,腸致病性大腸桿菌的eaf 、 espc基因,腸出血性大腸桿菌的溶血素hly 、志賀毒素1 ( slt1 ) 、志賀毒素2 ( slt2 )基因,腸集聚性大腸桿菌的eaggec探針,以及在泌尿道致病性大腸桿菌和o157 : h7大腸桿菌中新發現的毒力島基因。 -
The c - phycocyanin ( cpc ) operon of blue - green alga ( or cyanobacteria ) arthrospira platensis fachb341 was cloned, sequenced and characterized by using chromoseme walking method. the sequence includes cpcb gene ( 519 bp ), cpca gene ( 489 bp ), cpch gene ( 357 bp ), and upstream sequence of cpcb ( 427 bp ) and upstream sequence of cpch genes ( 184 bp ), 111 bp of phycocyanin intergenetic spacer ( pc - igs ). upstream sequence of cpcb gene was ligated into promoter - probe vector pegfp - 1 and transformed into three systems : e. coli, synechocystis pcc 6803 and a. platensis fachb341 by supersonic and electrophoresis methods
根據genbank中報道的節旋藻藻藍蛋白基因序列設計引物,首先克隆了鈍頂節旋藻( arthrospiraplatensisfachb341 )藻藍蛋白操縱子中亞基基因、亞基基因部分序列及二者之間的間隔區序列( pc - igs )並進行序列測定,然後根據此測序結果設計引物,通過染色體步移法克隆得到藻藍蛋白操縱子長度為2086bp的基因片段,其中包括藻藍蛋白亞基基因( cpcb , 519bp ) ,亞基基因( cpca , 489bp ) ,連接蛋白h基因( cpch , 357bp ) ,亞基基因上游啟動子序列( 427bp )以及各基因之間的間隔區( pc - igs , 111bp ; cpch與cpca間隔區, 184bp ) 。 -
Lastly by using the technique of dot blot hybridization, the genome dna of chlamydia was detected with the probe of momp gene labeled with dig - 11 - dutp by using the way of random primer. the results showed the degree of sensitivity of the probe was 10 pg and other pathogens could not be detected by this probe. by comparing the diagnostic ways of nucleotide probe and fc, the technique of nucleotide probe were proved to have high sensitivity and speci fi city
最後,用地高辛隨機引物法標記成momp基因核酸探針,斑點雜交檢測衣原體基因組dna ,靈敏度可達10pg ,且不能檢出其它病原體的核酸。將核酸探針法與補體結合反應法對衣原體感染的診斷進行比較,初步證明該探針具有較高的敏感性與較強的特異性。 -
Hybridization bands were detected by southern blot analysis using lea3 gene probe labeled by digoxigenin the result showed that foreign lea3 gene integrated into strawberry genome
2 。對點雜交為陽性的植株進行southernblot分析,轉化植株檢測到了雜交帶,除預期的1 -
One was cloning, sequence analysis and expression of the fragment containing the b and c antigenic sites locating at the 5 " terminus in spike gene of tgev in prokaryotic expression system ( fused with gst ), the other was preparation of non - radioactive probe labeled by digoxigenin for detecting the rna extracted from tgev by assay of dot - blot
為了鑒別診斷tgev與prcv及對tgev進行流行病學調查,本研究採用原核表達系統( gst融合表達系統)表達tgev纖突蛋白( s蛋白)中含有b和c抗原位點的多肽,並且制備了非放射性地高辛標記的核酸探針,通過斑點雜交( dot - blot )檢測tgev核酸rna 。 -
We found that sit variant gene ( slt2vha ) was identified in strains e. coli o157 : h7 isolated from patients and dung beetles 2000 in xuzhou city, jiangsu province. the primers used for stx2 variant analysis are shown in tablel. genomic dna restriction fragments digested by pstiwere sonthern - blotted and hybridized with an stx2 - specific dna probe. the probe was prepared fromed a 285 - bp pcr productof the strain 882364 stx2 gene obtained by using the specific primer pair ( tablel )
2000年在江蘇省徐州市銅山縣腹瀉病患者的糞便標本分離的10株產生志賀毒素的菌株以及從蜣螂腸道分離到的4株產生志賀毒素的大腸桿菌o157 : h7 ,屬于另兩個pfge型,和1986 、 1987 、 1988年在徐州市腹瀉病患者的糞便標本分離的菌株pfge圖譜不同。 -
Typing of vibrio cholerae with 16srrna gene probe and ctx a gene probe
基因探針用於霍亂弧菌分型 -
Rapid detection of l. monocytogenes in foodstuffs by gene probe methods
基因探針快速檢測食品中單增李斯特氏菌 -
Lea3 gene probe and marker probe were labeled by dig - chem - link
Okblea3片段,並用地高辛標記法進行了lea3基因探針的制備。 -
Was multiplied and the tk gene was cloned. the cloned tk gene was retrieved by proper restrictive hemodynamics. the retrieved tk gene was labeled by digoxin according to the kit of labeling and detection of digoxin. then, the specificity and sensitivity of tk gene probe were detected with dot blot hybridization. the sequence of tk gene of nm98a strain was analysed. the result of the analysis of tk gene ' s sequence confirmed that autoploidy between tk gene of nm - 98a strain and issued strain was 99. 7 %
本研究中首次對iltv - nm98a株的tk基因進行了克隆和序列分析,結果表明: iltv - nm98a株tk基因的核苷酸序列與已發表的iltvtk基因的核苷酸序列具有高度的同源性,兩者之間僅相差4個核苷酸,同源性高達99 . 7 ,從而證實了iltvtk基因是高度保守的,為iltvtk基因核酸探針的制備提供了有力的依據。 -
Part 1 : identification of a novel gene, tsarg2, and its sequence character cloning new apoptosis - related novel gene is a key to further understanding of apoptosis mechanism and the biological process of germ cell, and it is of momentous significance on clarifying physiology and pathology process of spermatogenesis. to rapidly attain human novel gene full - length cdna sequence, the gene - specific primers and the vector - specific primers have been designed for successful performing nested pcr and draft human genome searching to rapidly identify the tsarg2 ( genebank accession number ay040204 ) 5 " end from a human testis cdna library by using a cdna fragment ( genebank accession number be644542 ) as a electronic probe, which was significantly changed in cryptorchidism and represents a novel gene. furthermore, a mouse homologue of this gene was identified ( genebank accession number af395083 ) by lab on - line
本研究分為三個部分,其主要實驗方法及實驗結果如下:第一章tsarg2基因的克隆與序列分析從已獲得的在隱睪和正常睪丸對照中表達量有明顯差異的est片段( be644542 )入手,設計了基因特異性引物和載體特異性引物進行巢式pcr擴增,結合人類基因組草圖搜索法,從睪丸cdna文庫中快速分離出人類睪丸凋亡相關基因的5末端而獲得全長cdna , genbank登錄號為ay040204 ,同時應用生物信息學的方法克隆了該基因在小鼠中的同源基因, genbank登錄號為af395083 。 -
Determine the relationship between the measured variability of gene expression in one or more data sets and the variation of the melting temperature within a probe set
確定在一個或多個資料組的基因表達變化和探針裝置內部溶解溫度變化之間的關系。 -
In order to study the expression of 3 - defensins in liver as acute phase response proteins, a murine systemic acute phase responsive model was established by intraperitoneal injection o f lipopolysaccharide ( lps ) in our study. the mbd3 cdna sequence ( 145 - 169 bp ) was labled with [ - 32p ] atp as a probe to detect mbd3 mrna in different tissues by northern blot and analyze the time - and dose - dependant expression caused by lps. the 5 " flanking sequence ( - 167 - 179 bp ) of the mbd3 gene was designed as the probe and labled with [ - 32p ] dctp to investigate the binding of transcriptional factors to this region by electrophoretic mobility shift assay ( emsa ) and south - western blot
以小鼠mbd3基因145 ? 169bpcdna序列合成探針,經[ - ~ ( 32 ) p ] atp標記后通過northernblot方法檢測mbd3在肝臟中的表達,同時分析了mbd3基因誘導表達的組織特異性,劑效和時效關系;結合mbd3基因啟動子區序列分析,以- 164 ? - 179bp雙鏈dna序列合成探針,經[ - ~ ( 32 ) p ] dctp標記后通過電泳遷移率改變實驗( emsa )和south ? westernblot方法對參與mbd3在肝臟中誘導表達調節的轉錄因子進行分析。 -
The key stage of fabricating gene chip is pretreatment of glass surface including the processes of nh3h2o treatment, aminosilane treatment and aldehyde treatment. the pretreatment can grow active group that can bind probe effectively on the surface of glass slide. as a result, the actively treated glass slide can suit for fabricating in - situ synthesis high density gene chips
基因晶元制備技術的關鍵步驟是玻片表面預處理,即對玻片表面進行羥基化、氨基化和醛基化處理,使表面生長的活性基團能有效固定寡核苷酸探針,以滿足原位合成高密度基因晶元對玻片的要求。 -
A pair of primer, dig labeled probe and a taqman probe based on the conserved nucleotide sequence of cp gene of different pnrsv strains were designed and synthesized
本文根據病毒各株系外殼蛋白基因的保守序列,設計了雜交誘捕探針、 dig標記雜交探針以及確定了最佳誘捕參數和雜交檢測參數,建立雜交誘捕rt - pcr ? elisa 。
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