液體培養基 的英文怎麼說
中文拼音 [yètǐpéiyǎngjī]
液體培養基
英文
broth-
Mycelial growth and exo - biopolymer production by submerged culture of various edible mushrooms under different media
中譯:數種可食用真菌于含不同媒介之液態培養基中的菌絲體生長與外生物大分子的產生。The cultural conditions such as temperature, fermentation period and the compound of medium are studied. the result of test show that suitable factors for both bacterium to grow and active substance to produce are 28, 200rpm and 72 hours. the bacterium is gotten through centrifuge with 8000rpm for 20min. then the bacteria is diluted and colophony named s - 8 is put into and used to absorbed active substance for 4 hours
對該菌株發酵條件的研究表明:該菌株用馬鈴薯葡萄糖液體培養基發酵培養, 28 , 200rpm搖瓶中振蕩培養72h可獲得高活性的發酵產物,用蘇雲金芽孢桿菌hd - 1做指示菌,將發酵液稀釋40倍生測仍可形成明顯的抑菌圈。Hydroponics ( water culture ) the growth of plants in liquid culture solutions rather than soil
水培:是在液體培養基中栽培植物而不是在土壤中。All the hairy roots of a. ficoidea cv. " ruliginosa " could have a rapid autonomous growth on phytohormone - free liquid or solid ms medium
紅龍草毛狀根能在無激素的固體或液體培養基上快速自主生長。At the anaphase of cultured, the bacteria exsist as a cycloidal dormancy body - sporocyst, and the decomposing rate of filter - paper began to decrease. we know the sporocyst is a form that sporocytophaga genus appear in a ill circumstance, so we think the sporocyst did n ' t have the cellulose decomposing activity. after cultered 96 hours, we can found many sporocysts and filter - paper slices in the fermentable liquid
並且這一時期的濾紙降解率開始降低,證明小孢囊並不與纖維素的旺盛降解有關。培養96小時后,濾紙纖維素被降解成碎屑,液體培養基中有大量孢囊存在;培養6 ? 7天後該菌可以將濾紙纖維素完全降解。The most common means of agitation of liquid media is by placing the culture vessels on a drum (for test tubes).
液體培養基最普通的搖動方式,要把培養器皿放置於圍繞一根近水平的軸緩慢旋轉的圓筒(用於試管)。The four psb strains, wst22 sc21 sc42 sx51, grow rapidly and can be conserved for a long time. 2. the resistant function to pathogenic e. coli and salmonella enteritidis of four psb strains was test that they had different function by oxford cup test
Wst22 、 sc21 、 sc42 、 sx514株光合細菌生長較快,在培養基中光照培養3天活菌數即可達到10 ~ 9個/ ml ;存活期長,在液體培養基中保存3個月後將其轉入新的培養基中仍然能夠保持很高的繁殖能力。Degradability of the isolates on acetic ester compounds was proved according to the increase of biomass and the decrease of substrates in liquid cultures
該菌對醋酸酯類化合物的降解性是通過在液體培養基內菌體的增加及底物的減少來證實的。After co - cultivation, all the explants were washed in liquid mso medium containing 500mg / l cef and 500mg / l carb for 2 hours. washed with sterile water for 5 times and patted dry on the filter paper again
共培養后,以附加有500mg / l的cef和500mg / l的carb的ms0液體培養基震蕩脫菌培養2小時,無菌水沖洗5次,無菌濾紙吸干水分。The results showed that the growth of root tips in liquid medium was better than that in agar - solidified medium and solid - liquid two phase medium, for that increasing agar concentrations in medium will reduce the root growth ; darkness was beneficial for fraxinus mandshurica root tip culture in vitro ; as the carbon sources, sucrose was better than glucose and maltose as the carbon sources, and 3 % sucrose was best for the root tip growth of fraxinus mandshurica
結果表明,不添加瓊脂的液體培養基對根尖的生長較添加瓊脂的固體培養基和固液培養基好,原因是增加瓊脂的量會抑制根的生長;暗培養比光培養更有利於水曲柳離體根尖的培養;蔗糖作為碳源的效果較果糖和麥芽糖好,其中以3 %的蔗糖對離體根尖的生長效果最好。The most common means of agitation of liquid media is by placing the culture vessels on a drum ( for test tubes )
液體培養基最普通的搖動方式,要把培養器皿放置於圍繞一根近水平的軸緩慢旋轉的圓筒(用於試管) 。The optimization of fermentation process for mycelia production of cordyceps militaris
菌絲體液體培養基的優化和發酵條件的研究Development system in some streptomyces spp. is characterized by an unique multiphasic growth kinetics in liquid medium. after spore germination, first logarithmic growth is followed by a transient cessation of cell growth, which potentially serves as a key developmental switch in regulatory system, leading to initiation of second logarithmic growth
某些鏈黴菌在液體培養基中表現獨特的多相生長動力學特徵:第一次對數生長之後,細胞生長過渡性地停止,這個過渡期可能起著一個重要的發育調控開關作用,啟動細胞第二次對數生長。According to morphologic characteristics. when cultured in liquid medium, cadmium with initial concentration below 4. 61mg / l did n ' t inhibited the growth of f2, 163. 8mg / l of cadmium affected it obviously but growth continued to a great extent. cadmium removal from medium by f2 under liquid culture was not so stable with low cadmium concentration below 4. 61mg / l, but removal ratio reached 96 % with initial cadmium concentration of 163. 8mg / l and cadmium content of biomass reached 28 %, which showed high capacity of cadmium accumulation by f2
F2在液體培養時,培養基初始鎘濃度在4 . 61mg l以下時對其生長無抑制作用,鎘濃度為163 . 8mg l時有較大影響,但仍有明顯生長; f2對液體培養基中低濃度鎘( 4 . 61mg l以下)的去除效果不太穩定,但初始鎘濃度為163 . 8mg l時,其去除率為96 ,菌體最大鎘含量可達28 ,顯示了較大的富集容量。Sequence analysis shows that they share 98. 75 % similarity at the dna, and 98. 67 % at the protein level. ns2 gene was cloned into the multiple cloning sites of prokaryotic expression vector pgex - 6p - l. the recombinant plasmid pgex - 6p - ns2 was constructed and transformed to the competent cell bl21 ( de3 ) plyss, positive bacterium strain was induced by iptg
將ns2基因插入到原核表達性質粒pgex - 6p - 1的ecor 、 bamh多克隆位點之間,將重組原核表達質粒pgex - 6p - ns2轉化到bl21 ( de3 ) plyss感受態細胞中,獲得了表達ns2基因的陽性亞克隆重組子,在含amp的lb液體培養基中培養,經iptg誘導表達,用sds - page分析表達產物。These hairy roots grew well on ms agar medium or liquid medium withour growth regulator for over one year. they grew vigorously and produced numerous lateral branches. four hairy root clones, namely tra1, tra2, tra3 and tra4, were established
毛狀根能在不含任何激素的ms固液體培養基中快速生長,且表現出多分支,多根毛,失去向地性生長等典型毛狀根特性;建立了tra1 , tra2 , tra3 , tra4四個毛狀根無性系。Culture a population of microorganisms or dissociated cells of a tissue grown on or within a solid or liquid medium for experimental purposes
培養:以試驗為目的在固體或液體培養基上生長的微生物種群或解離的細胞或組織。When the bacterial strain of s. maltophilia 276 was cultured in the three media of lb, pda and kmb, and the sod activities of cell extracts were detected, it was found that s. maltophilia 276 could produce higher activity of sod when cultured in lb media than that in the other two media
利用lb 、 pda和kmb三種液體培養基培養s maltophilia276菌株,檢測其細胞提取物中sod的活性,結果發現在lb培養基上培養的276菌株中的sod活性比在利用pda或kmb培養基培養的276中的sod活性要高。通過對不同培養時間的細菌含量和sod的活性檢測發現:在sThe trick was to culture the individual cells separately while allowing them to share the same liquid medium
試驗的關鍵在於對每個細胞進行分離培養的同時將它們置於同樣的液體培養基。Culturing them together in this way allowed them to encourage each other ' s growth by chemical signals through the medium
將它們放在同一液體培養基中,可以使這些細胞在液體培養基中傳遞化學信號,從而相互促進彼此的生長。分享友人