花序列 的英文怎麼說
中文拼音 [huāxùliè]
花序列
英文
anthotaxis-
Floral aberrance of cbf1 transgenic tobacco and analysis of its flanking sequences
1基因煙草植株的花器官變異及其插入區側翼序列的分析By means of discontinuous tris - hcl buffer system and poly aery 1 amide gel electrophoresis ( page ), zymogram of 23 species of 11 genera in 4 subfamilies mirinae, orthotylinae, phylinae and deraeocorinae are gained. by specific primer pcr and sequencing, 57 cyt b gene 433bp sequences are obtained from 34 species respectively belonging to 17 genera in 5 subfamilies mirinae, orthotylinae, phylinae, deraeocorinae, bryocorinae from 64 species of 23 genera which involved in this research, and 2 outgroup species of family anthocoridae as well. 1
首次通過特異引物擴增和基因測序的研究方法從被試的5亞科23個屬的64種盲蝽中獲得了盲蝽亞科、合墊盲蝽亞科、葉盲蝽亞科、赤爪盲蝽亞科和蕨盲蝽亞科bryocorinae5個亞科17個屬的34種盲蝽以及外群花蝽科anthocoridae2種花蝽的cytb基因序列57條。Spadix rachis flat, margin with bract - like appendages ; flowers small, monoecious, in 2 series on rachis, apetalous
肉穗花序軸扁平,邊緣有苞片狀附屬物;花小,單性,雌雄同株,呈2列排列于花序軸上,無花被。Cymes 1 - 2 in axil of leaves, rather short ; flowers pale green, 7 mm in diam., 5 - merous ; sepals imbricate, inner two larger ; petals suborbicular, 3 mm long ; stamens without filaments ; pistil without style, stigma appressed, minutely 5 - lobed
聚傘花序1 - 2腋生,短小;花淡綠色,直徑約7毫米; 5數;萼片覆瓦狀排列,內方2片較大,邊緣常有深色細淺齒;花瓣近圓形,長約3毫米;雄蕊無花絲;雌蕊無花柱,柱頭平貼,微5裂。Dsmv is proved as the predominating virus - pathogen on aroid plants from zhejiang province and other regions in china. cdna of dsmv rna 3 " end partial sequence and subgenomic rna promoter region of cucumber mosaic virus ( cmv ) rna3 were used as probes for detection of dsmv and cmv respectively. total rna extracted from field samples were used for rna dot - hybridization
用侵染馬蹄蓮的dsmv3末端序列和黃瓜花葉病毒( cmv )的亞基因組啟動子區互補dna序列為標記探針,對自然感病的天南星科植物進行rna斑點雜交,並結合雙鏈rna分析、病毒提純和形態學觀察,對杭州等地16屬天南星科植物的81個樣品進行了病毒鑒定。For functional genomics, huge est databases from multiple tissues of a number of tree species have been rapidly accumulated, and molecular analyses on secondary growth and wood formation, flowering, and cold hardiness have given some insights into the metabolic pathways of those tree - specific development processes
功能基因組學方面,已分析了主要造林樹種多種組織的轉錄組est序列,對林木次生生長與木材形成、開花和抗寒性的形成等過程開展了功能基因組學研究。In the end, the results in this article were compared to the its sequences of other species in cruciferae and their phylogenetic relations were discussed
本文還將所得的結果與已發表的部分十字花科其它屬植物的its序列進行比較,探討了該科植物系統發育情況。Based on the survey of viruses infecting araceae plants from in zhejiang province, hunan province, hainan province and other regions in china, pathogenic viruses of this family were detected and identified. sequence similarity was compared between dasheen mosaic virus ( dsmv ) isolates of different origin. virus - free seedlings were obtained for two important taros cultivar, colocasia esculenta cv
本研究論文對我國浙江省、湖南省和海南省等地的天南星科植物上的主要病毒進行了檢測和分子鑒定,比較了該科主要病原病毒芋花葉病毒( dsmv )不同分離物的序列同源性並分析其種內分化關系;同時,我們對2種重要的芋屬栽培作物? ?奉化芋艿頭、烏梗芋( colocasiaesculenta )和我國特有的天南星科藥用植物? ?掌葉半夏( pinelliacordata )進行了脫毒培養和快速繁殖研究。However, only a few host factors with clear in vivo function have been identified. by using pcr and 5 " and 3 " race, we were able to clone a homologue ( named ttom1 ) of arabdopsis thaliania host factor gene, tom1, which supports the replication of tobacco mosaic virus
根據從擬南芥中已經克隆的支持煙草花葉病毒復制的基因tom1序列設計一對特異性引物,用rt - pcr的方法獲得番茄同源基因的部分序列,然後利用5 』 race與3 』 race方法從番茄中克隆出全長ttom1基因。Genetic diversity and phylogeny of 55 slow - growing rhizobia isolated from peanut ( arachis hypogaea ) in china were determined by analysis of host - plant range, phynotype, 16s rrna rflp, 16s rrna sequence, 16s - 23s igs rflp, rapd, rep - pcr, dna - dna hybridization homology. at the same time, the competitive nodulation capacity of rhizobia, effect of host plants and soil ph on the rhizobia were determined for screening and improvement of high effective rhizobium inoculant
本研究採用宿主范圍試驗、表型性狀測定、 16srrna - rflp 、 16srrna序列分析、 16s - 23srdnaigsrflp分析、 rapd分析、 rep - pcr分析和dna - dna同源性分析等技術系統研究了從我國不同地域分離的55株花生根瘤菌的遺傳多樣性及其在根瘤菌系統發育中的地位和相互關系。Their differences are based on many aspects which include characteristics of morphology, anatomy and epidermis of leaf, types of tapetum in anther walls, patterns of endothecial thickenings, and ways of development of endosperms, presence or absence of perisperm, components of photochemistry, and sequences of rbcl
菖蒲屬與天南星科其它屬在葉的形態、結構、表面特徵,花藥絨氈層類型,藥室內壁增厚的特點,胚乳的發育方式,外胚乳的有無,植物化學成分, rbcl基因序列等多方面存在著顯著的差異。Homology analysis blast analysis showed that the amino acid sequence of the asf gene cloned from cotton was significantly homologous with adp - ribosylation factor ( asf ) of mammalian, plant and yeast, etc. the amino acid sequence of the gene shows 99 % ( 179 / 180 ), 98 % ( 177 / 180 ), 96 % ( 174 / 180 ) and 92 % ( 168 / 180 ) identity to arabidopsisthalianaarfl, triticum aestivum, solatium tuberosum and bos taurus, respectively
棉花arf基因的同源性分析應用ncbi進行dna序列的相似性分析,結果表明:棉花arf基因與其它植物、動物和酵母的arf基因具有較高的同源性。棉花arf基因編碼的氨基酸序列與擬南芥,小麥、馬鈴薯、牛的同源性分別達到99 ( 179 / 180 ) 、 98 ( 177 180 ) 。 96 ( 174 180 )楊花腸p核符吞fi曰手谷回伽皿的夭險和92 ( 168ill ) 。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。It was suggested that the gene t13m11. 8 could be the ast candidate gene. this gene was 1432bp long with 6 exons and 5 introns. the putative protein of t13m11. 8 gene was highly homologous to dihydroflavonol 4 - reductase ( dfr ), which was an important enzyme in the anthocyanin biosynthesis pathway
該基因的dna序列長1432bp ,含有6個外顯子和5個內含子,編碼的蛋白與花青苷生物合成途徑中的二氫黃酮醇4 -還原酶有較高的同源性。Based upon the comparison of cyto b gene sequences in 15 deer species downloaded from genbank, a universal primer set l15774 / hsf21 was used as positive control of the template quality, at the meantime, two species specific primer sets df / dr and cf / cr were desgined to identify red deer ( cervus elaphus ), sika deer ( cervus nippori ) and roe deer ( capreolus capreolus ) from other species. a musk deer ( moschus ) specific primer set wf / mr was designed, siberian musk deer ( afoschus moschiferns ) and forest musk desr ( moschus berezovskii ) could be discriminated when restriction endonuclease rsa i was used to cut the pcr products
經過對來自genbank中的15種鹿類動物的cytob基因序列的比較,用通用引物l15774和hsf21作為模板的質量控制,設計了特異性引物df dr和cf cr來鑒定馬鹿、梅花鹿、狍;設計了麝類特異性引物mf mr ,用限制性內切酶rsa酶切擴增產物來區分原麝和林麝。Meanwhile, these six coat protein genes were sequenced and compared with other homologous sequences in genbank. the strain designation of the six isolates of tumv was finally determined. the results are as the following : 1. six isolates of turnip mosaic virus named tumv - sd1, tumv - sd2, tumv - sd3, tumv - sd4, tumv - sd5 and tumv - sd6 were respectively acquired from infected chinese cabbages and radishes in 3 cities ( taian, yantai and zaozhuang ) of shandong province
利用rt - pcr方法克隆了tumv山東分離物的外殼蛋白( cp )基因,測定了它們的核苷酸序列、並將其與已報道的序列進行同源性比較和分析,最終確定了其歸屬地位,具體研究結果如下: 1 .從山東省3地市感病的白菜和蘿卜上分離到蕪菁花葉病毒的6個分離物,分別命名為tumv - sd1 、 tumv - sd2 、 tumv - sd3 、 tumv - sd4 、 tumv - sd5和tumv - sd6 。2. an up - dated method was employed to purify tumv in this research. using the protease k method, we acquired the viral genome - rna. a pair of specific primers was designed and synthesized based on the nucleotide sequences of tumv coat protein genes reported before and rt - pcr was used to clone the cp genes of the six tumv isolates
應用改進的蕪菁花葉病毒的提取方法從病葉中提取病毒粒體,應用蛋白酶k法從病毒粒體中提取病毒rna基因組,根據已報道的tumv的cp基因序列,設計併合成了一對特異引物,利用rt - pcr法克隆了6個分離物的外殼蛋白基因,與克隆載體puc19連接后通過熱激法轉化大腸桿菌dh5 。A very complex sequence probably won ' t be re - used in many test scripts, so it might not be worth the labor required to generalize it, document it, and insert the error - checking code into it that you would expect of a competently written library function
因為一個很復雜的命令序列很可能在很多測試腳本中無法重用,所以,就不值得花力氣去生成它,為它寫文檔,並為它加入錯誤檢查代碼以期成為編寫完善的庫函數。Genetic diversity analyses of three wild populations of pinctada martensii dunker. using rapd technique
月季切花衰老相關基因的差異顯示及其序列分析In this paper, phylogenetic relationship of 13 species involved in 6 genera of cruciferae wer e carried out through both the clones of homologous sequences with the primers designed on the basis of conserved regions of cyp86mf gene in cytochrome p450 gene superfamily and the differential analyses of them. meanwhile, complete sequences of some genes in cytochrome p450 gene superfamily were isolated and identified by smart pcr - race strategy, and expressed in e. colt. the results were as follows : ( 1 ) isolated by pcr from 11 species of cruciferae, eleven homologous gene segments that deduced amino acids were identities of over 80 % at nucleotide sequence level and similarities of over 70 % at amino acid sequence level
本論文以已知的細胞色素p450基因超家族成員cyp86mf基因的保守區設計引物對十字花科重要蔬菜作物的6個屬13個物種進行了同源序列的分離克隆,通過核酸序列的差異比較分析,研究了該基因在不同物種中的進化關系;同時,通過保守引物的pcr擴增和race相結合的方法對十字花科植物不同物種的細胞色素p450基因家族成員基因全長進行了分離克隆、鑒定和原核表達的研究,獲得如下研究結果: ( 1 )通過pcr從十字花科植物不同物種中擴增到11個可以推導出完整氨基酸序列的同源片段。分享友人