tobacco (l) 中文意思是什麼
tobacco (l)
解釋
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This paper describes a strategy that has developed to transfer the cdna of tobacco mnsod gene into the commercially important breeding line - baoding alfalfa via agrobacterium infection. transgenic alfalfa plants have been generated that overproduce a nicotiana plumbaginifolia l. manganese superoxide dismutase ( mnsod ). the results domenstrated that baoding alfalfa is an important breeding line which easily amenable to genetic transformation
本研究採用我國農藝性狀優良的豐產苜蓿品種保定苜蓿,通過農桿菌介導的轉基因方法,使用特定的質粒載體pchlsod將煙草mnsod基因的cdna序列導入保定苜蓿中,說明保定苜蓿是一種易於遺傳轉化的優良苜蓿育種品系。 -
The regeneration system of tobacco was established. the adventitious shoots were induced from leaf explants of tobacco based on ms basal medium supple - - mented with 2. 0mg / l 6 - ba and 0. 3mg / l naa. then the regenerated plants were rooted on ms medium containing 0. 3mg / l naa
植株再生體系的建立採用無菌苗煙草葉片為外植體,以ms為基本培養基,篩選出ms + 6 - ba2 . 0mg l + naa0 . 3mg l以誘導不定芽的分化,並於ms + naa0 . 3mg l的pa碩士學位論文v沉了砂「工隊nk 」主根培養基上生根,獲得完整再生植株。 -
Leaves of tobacco ( nicotiana tabacum ) were wounded, infected by agrobacterium tumefaciens strain lba4404 and gv3101 : pmp90 harboring expression vector pbgsb and pbglsb and co - cultured for 3 days in darkness on the culture medium ( ms + 0. 5mg / l 6 - ba + 0. 7 % agor ph 5. 7 )
4以煙草(品種sr )無菌苗葉片為外植體,採用農桿菌浸染的葉盤轉化法,用構建好的植物表達載體對煙草進行遺傳轉化。外植體置於無抗生素的誘芽培養基( ms 0 -
The critical concentration of mannitol stress is 0. 8 - 0. 9mol - l - 1. the maximal level of aba accumulation is attached after 5 hours " treat with 0. 9mol - l - 1 mannitol solution. cell wall plays important roles in tobacco cells perception to osmotic stress
滲透脅迫誘導aba積累的水平與脅迫處理的濃度和時間相關,脅迫處理的有臨界濃度為0 . 8 ? 0 . 9mol ? l ~ ( - 1 ) , aba積累水平在脅迫處理5小時后達到最大。 -
3. through the ladder experiment of selecting transformer concentration by hyg, the proper selecting transformer concentration is 20mg / l hyg to tomato cotyledons and 35mg / l hyg to tobacco discs
經潮黴素梯度篩選試驗,最終確定番茄的適宜篩選濃度為20mg l ,煙草的適宜篩選濃度為35mg l ; 4 -
Volatile components in citrus medica l. leaves and its application in tobacco flavoring
香櫞葉揮發性化學成分及其在卷煙加香中的應用研究 -
When the seeds from to transgenic plants were cultured on medium supplemented with 50mg / l hygromycin, the ratio of germinated to non - germinated seeds is 3 : 1, which is consisted with mendel ' s first law. southern blotting demonstrated that the svde gene had been integrated into the genome of tobacco plants
轉基因植株的l代種了在潮黴素培養基上的萌發數與未萌發數的比值為3 : l ,符合單基因的盂德爾分離規律。 -
Three binary expression vectors were constructed, which harbored the cl - i - 2kl, r - 2kl, and d - l - 2kl - r - 2kl respectively, driven by the camv 35s promoter. then, agrofeac / erium - mediated transformation of iobacco ( nicotiana tabacum, w38 ) was carried out. transformed tobacco lines were obtained through tissue culture and confirmed by pcr and southern blotting analysis
通過分子克隆技術,將c1 - i - 2k1 、 r - 2k1和二者的連接( c1 - i - 2k1 ? r - 2k1 )分別構建到雙元表達載體上,並使它們分別置於35s啟動子的驅動之下,然後通過農桿菌介導的技術分別對煙草( nicotianatabacum , w38 )進行了轉化,利用組織培養技術再生植株。 -
Based on the plant expression vector of pcambia1300 - hbmp - 3m and pcambial 301 - hbmp - 3 constructed, we set up the system of high frequency regeneration and transformation of tomato cotyledons. the hbmp - 3m gene and hbmp - 3 gene were respectively transformed into tomato and tobacco by transfection of agrobacterium tumefaciens. and the transgentic plants were detected. the main results are as follows : l. the plasmid pcambial300 - hbmp - 3m carried hbmp - 3m gene and pcambia - 1301 - hbmp - 3 carried hbmp - 3 gene were respectively transferred into agrobacterium tumefaciens by electroporation
本試驗是在已經構建好的植物表達載體pcambia1300 - hbmp - 3m和pcambia1301 - hbmp - 3載體的基礎上,建立番茄子葉的高頻率再生體系和番茄子葉的高頻遺傳轉化系統,利用根癌農桿菌介導的方法,將人骨形成蛋白- 3成熟肽( hbmp - 3m )基因和人骨形成蛋白- 3 ( hbmp - 3 )全長基因分別導入番茄和煙草,並對轉基因植株進行了檢測。
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