桿菌黴素 的英文怎麼說
中文拼音 [gǎnjūnméisù]
桿菌黴素
英文
bacillomycin-
The total rna was isolated from pokeweed ( phytolacca americana ) leaves using the method of guanidine isothiocyante and used as template to amplify the total length and deleted mutant pokeweed antiviral protein ( pap ) gene by rt - pcr and then the pap gene was cloned into pgem - t vector. the sequencing results showed that pap gene had 99. 9 % identity comparing with the pap gene nucleotide sequence reported by lin et al ( 1991 ). the iptg - inducible expression vector containing the pap gene was constructed and transferred into e. coli bl21 ( de3 ) - plyss
將缺失型pap基因克隆到植物表達載體pbi121中,通過液氮冷凍法將重組質粒轉入農桿菌lba4404細胞中,然後採用葉盤法,在該農桿菌的介導下將pap基因導入普通煙草中,經過卡那黴素抗性篩選,最後獲得了轉pap基因的工程煙草植株,摩擦接種煙草花葉病毒( tmv ) ,與非轉基因煙草相比,能夠推遲癥狀表現達2月之久,說明pap基因能夠在其它植物體內產生有活性的高抗病毒的蛋白質。It is an important that bacteria contaminated vaccine in the biologicals production. we collected 703 samples of cell culture, virus cultivation and harvest which were contaminated by bacteria during poliovaccine production within two years. we checked these samples by bacteriological method and antibiotics sensitivity tests were done. it shows that 1 ) the main contaminated bacteria come from staphylococci, bacilli and streptococci of environment in the poliovaccine production. 2 ) it is effect that antibiotics to contaminated bacteria are doxycycline, albiotic, prescription 2, cefotaxime na salt, gentamycin, neomycin, aureomycin and erythromycin
在疫苗生產實踐中,細菌污染是影響疫苗質量和產量的關鍵性因素,筆者通過了兩年左右的時間,選取正常生產中零星細菌污染的細胞培養瓶、病毒培養瓶及收毒污染樣品等共703份,進行細菌學檢查,並對造成污染的主要細菌種類進行了各種抗菌藥物的耐藥性實驗,結果表明:我所脊灰疫苗生產中主要的污染威脅來自環境中的葡萄球菌,潛在威脅是桿菌和鏈球菌;強力黴素、林可黴素、配方2 、噻孢黴素鈉鹽、慶大黴素、新黴素、金黴素和紅黴素等抗生素對目前引起污染優勢細菌-葡萄球菌有明顯的抑菌效果,可作為疫苗生產后備抗菌手段參考Those pathogens were susceptible to ciprofloxacin and novobiocin, however resistance to penicillin c, streptomycin, bacitracin and polymyxin b was produced
這些致病菌對環丙沙星、新生黴素等藥物有很高的敏感性,而對青霉素、鏈黴素、桿菌膚和多粘菌素已經產生耐藥性。The results also revealed that it was a reasonable choice to use carbenicillin as the antibiotics of inhibiting growth of remnant agrobacterium after co - culture, and when hygromycin was used as the selective agent, continuous selection at low concentrations ( 50 ~ 150mg / l ) produced the highest numbers of transgenic plants without escapes
試驗表明,在農桿菌介導高羊茅遺傳轉化中,抑菌劑宜選用梭節青霉素;以潮黴素作為選擇劑時,採用低濃度( 50一15om留l )連續篩選的方式比較合適,在該方式下,獲得的轉基因植株較多。All of our products is exported likelactobacillus acidophilus, bidifobacterium longum, lactobacillus paracasei, lactobacillus rhamnosus, tagatose, lnulin, nisin, natamycin, - polylysine, nucleotides mix, adenosine monophosphate, cytidine monophosphate, guanosine monophosphate disodium, uridine monophosphate disodium, calcium inosinate, calcium guanylate, calcium 5 - ribonucleotide, damp, dcmp, dgmp, tmp, deoxyadenosine, 2, 6 - diaminopurine nucleoside, 2, 6 - diaminopurine deoxynucleoside, adenine arabinoside, adenosine triphosphate, uridine triphosphate, guanosine triphosphate, cytidine triphosphate, cytidine diphosphate choline ( citicoline ) to all over the world, if you are interested in our products, please do visit our website, hope there will fullfill your requirement
主營產品有益生菌(嗜酸乳桿菌、長雙歧桿菌、乾酪乳桿菌、鼠李糖乳桿菌) 、塔格糖、菊粉(菊糖) 、乳酸鏈球菌素、納他黴素、 -聚賴氨酸、核苷酸,腺苷酸,胞苷酸,鳥苷酸二鈉,尿苷酸二鈉,肌苷酸,鳥苷酸鈣,核糖核苷酸鈣,脫氧腺苷酸,脫氧胞苷酸,胸苷酸二鈉,脫氧鳥苷酸二鈉,脫氧腺苷, 2 -氨基脫氧腺苷, 2 -氨基腺苷,阿糖腺苷,胞二磷膽堿,腺苷三磷酸,三磷酸尿苷,三磷酸胞苷,三磷酸鳥苷等Indication : for the treatment of bacterial enteritis caused by e. coli, salmonella spp., proteus, dysentery bacillus, an d other organisms susceptible to neomycin
用於治療禽畜的大腸桿菌、沙門氏菌、變形桿菌、痢疾桿菌以及其他對新黴素敏感菌感染引起的腸炎。Agobacterium tumefaciens strain a311 carrying the plant tranfer vector pb1121, which contains the neomycin phosphotransferasell gene ( nptll ) and p - glucuronidase reporter gene ( gus ) both under the control of the camv 35s promoter, was used in the establishment of the genetic tranformation of white clover
選用苗齡4 5天的帶柄子葉作為外植體,先將外植體預培2天,再與根癌農桿菌a311共培養3 4天後,轉入附加有40mg l ~ ( - 1 )卡那黴素和400mgThe regeneration system of soybean cytoledon node and agrobacteriunr mediated transformation method is the first selection at present. in the second part of this experiment, the expression vector prok2 containing npt ii and ssnhx1 ( na + / h + antiporter ) gene from suaeda salsa was introduced into soybean cytoledon nodes by gene transformation mediated by agrobacterium tumefaciens, and kanamycin resistant transgenic p lants were obtained by screening in selective condition
本實驗第二部分通過農桿菌介導法將含npt -和鹽地堿蓬na ~ + h ~ +反向轉運蛋白基因( ssnhx1 )的表達載體prok2導入大豆子葉節中,經過含km的篩選培養基連續篩選,獲得了ssnhx1轉基因植株,篩選劑卡那黴素的適宜濃度是50mg . l ~ ( - 1 ) 。Therapeutic efficacy of ranitidine bismuth citrate with clarithromycin for seven days in the eradication of helicobacter pylori
克拉黴素7天根除幽門螺旋桿菌療效觀察The resulting plasmid, named prok - sod2, was mobilized to agrobacterium tumefaciens strain gv3101 used for plant transformation. the yeast sod2 gene was introduced into arabidopsis thaliana ( ecotype landsberg erecta ) by agrobaterium tumefaciens - mediated transformation with floral - dipping method under the control of camv 35s promoter. transformants were selected for their ability to grow on medium containing kanamycin ( 30mg / l ), several homozygous lines that were all tolerant to kanamycin were selected and used for further molecular and physiological determination
本實驗將sod2基因構建到植物表達載體prok中,導入農桿菌后,進行植物遺傳轉化,實現其在擬南芥中過量表達,在含30mg l的卡那黴素的培養基上篩選獲得純合轉基因株系,自交一代獲得足夠的純和轉基因種子后,對其進行了分子生物學的驗證及生理指標的檢驗。Ssmapkk transformations were screened on media with kanamycin ( 30mg / l ). nineteen individual kanamycin resistant plants were obtained. t2 plants were checked for integration of foreign gene by counting ratio of the number of tolerant plants to the number of non - tolerant plants on selection medium with kanamycin ( 30mg / l )
將ssvp和ssmapkk的全長cdna分別克隆入植物表達載體pcambia1300和prok中,導入根瘤農桿菌gv3101后,由花浸泡法進行擬南芥遺傳轉化,轉化ssvp鹽地堿蓬ssop和ssmapkk基因的克隆與功能鑒定的擬南芥在含潮黴素( 25mg )的ms培養基上篩選,獲得t ;代轉基因植株。Based on a 3. 1kb pst i fragment of genomic dna of a wild s. avermitilis, a 1. 5 kb apramycin resistance fragment was inserted into sph i site of avec gene in the 3. 1 kb fragment, then a recombinant plasmid pc05 was obtained by introducing above inactivated avec fragment into mcs region of phjl401. competent cells of et12567 were transformed by recombinant plasmid pid03 and pc05 respectively
以含有avec基因的3 . 1kb基因組dnapsti片段為基礎,將1 . 5kb的安普黴素抗性基因片段插入到avec基因中的sphi酶切位點,再將此插入失活的avec基因片段連接到具有接合轉移功能(含有orit基因)的鏈黴菌-大腸桿菌穿梭質粒phjl401的多克隆位點區,由此得到重組質粒pc05 。Kurstaki strain hd73, were inserted into two copy sets of res sites. the res sites have same direction. when - the recombinant plasmid was introduced into crystal negative b. thuringiensis host bmb171, antibiotic resistance genes and other non - 5, thuringiensis dna can be selectively eliminated after the selection by antibiotic resistance marker
將crylac10基因或壯觀黴素基因和蘇雲金芽胞桿菌的質粒復制起始區oril030連接在一起,置於兩個同向的解離區之間,再將基因操作中所必需的大腸桿菌質粒復制起始區和抗生素標記基因等與之相連構成解離載體。The minimum inhibitory concentrations ( mic ) of imipenem, panipenem and meropenem for 225 clinical isolates was determined by agar dilution method, in comparison to 13 other antimicrobial agents
結果,三種碳青黴烯類抗生素對腸桿菌科細菌具高度抗菌活性,對銅綠假單胞菌、不動桿菌屬、糞腸球菌等亦具良好抗菌作用。5 lahaie rg, a randomized trial of the efficacy of three regimens for t he eradication of helicobacter pylori. gastroenterology 1995 ; 108 : a141
6劉文忠,呂寶妹,蕭樹東等.含克拉黴素的短程三聯療法根除幽門螺桿菌.中華內科雜志1996 ; 35 : 803 - 8066. transformation system of mustard a serials of kanamycin concentration was added to optimum medium to test the explants resistance capacity of two kinds of mustard. the transformation procedures described were derived from numerous regeneration and trasformation designed to test factors that might affect shoot regeneration, which including length of co - cultivation. those producing the best result parameters were described as below : after the mustard explants were precultured on regeneration medium for 2 days. they were inoculated with agrobacterium for 20 minutes. inoculated explants were co - cultivated for 4 days and in shadow at first 2 days. then transferred to the same medium plus 30 mg / l kanamycin and 500mg / l garb. all of them were transferred to fresh medium every 2 weeks. the kan - resistant plants were regenerated
芥菜外植體高頻遺傳轉化體系的建立在最適培養基上試驗了兩類芥菜的三種外植體對卡那黴素的敏感性、預培養天數、浸菌時間等因素的影響,建立了芥菜高頻轉基因再生體系:取生長4天的芥菜子葉、下胚軸和25天的葉片在分化培養基上( ms + ba3 . 0mg / l + naa0 . 1mg / l )預培養2 - 3天後,投入農桿菌菌液中浸染20分鐘,在分化培養基上暗培養2天,正常條件下培養2天後,轉入抗性培養基( ms ba3We obtained our transgenic material, the rice suspension cells, by inducing embryonic rice callus. then we constructed the expression vector pca - ced9, and transferred ced - 9 gene into the rice callus and embryogenic suspension cells. the work of using hygromycin selective medium to obtain regenerated plants is still going
構建了用於水稻中表達的載體pca - ced9 ,通過農桿菌eha105轉化導入水稻愈傷組織和水稻懸浮細胞,經潮黴素( hym )篩選,以期望獲得抗性植株,目前該工作仍在進行中。A 1. 5 kb apramycin resistance fragment was inserted into nru i site of aved gene and the inactivated aved gene fragment was then introduced into mcs region of phjl401 - an e. coli / streptomyces shuttle vector with conjugation function ( containing orit gene ). as a result of above procedures, a recombinant plasmid pid03 was obtained
將1 . 5kb的安普黴素抗性基因片段插入到aved基因中的nrui酶切位點,再將此滅活的aved基因片段插入到具有接合轉移功能(含有orit基因)的鏈黴菌?大腸桿菌穿梭質粒phjl401的多克隆位點區,由此得到重組質粒pid03 。To create transgenic mushrooms, researchers attached a gene that confers resistance to hygromycin, an antibiotic, to circular pieces of bacterial dna called plasmids, which hae the ability to multiply within a bacterium known as agrobacterium
為了創造轉基因蘑菇,研究人員需要把一種抵抗潮黴素(一種抗生素)的基因片段插入細菌dna的圓形片段(也叫質粒)中去,它將隨著土壤桿菌復制而大量復制。Study of e. coli resistance to the active components of phellodendron and tylosin by microcalorimetry
微量量熱法研究大腸桿菌對黃柏中活性成分和泰樂黴素的耐藥性分享友人