酶單位 的英文怎麼說
中文拼音 [dānwèi]
酶單位
英文
enzyme unit-
In trpsin tolerance assay. this virus could resist to 1 % trpsis at 37 in an hour. in acid tolerance assay, this virus was resistant to ph3. 0 and ph5. 0 at 37 in 2 hours, and the average infection litre of the virus decreased little. in heat assay, at 50, the virus was processed from 5 minutes to 150 minutes and at each condition the viral virulence reduced to some certain degree. among these conditions, when at 50 in 30 minutes. the average infection litre of this virus decreased over 2 tilre. and when al 50 in an hour, cpe of ihis virus disappeared. when time was set for an hour. but with processed in different temperature as 50 60 70, 80, the virus losl the multiplication capacity complelely. in biological assay, we selected different cell lines to cultivate this virus by laking advantage of possesional cells at that time in our laboratory. then we found that fcwf cell line was the most sensitive to dxmv and mdck was the second. with f81 cell line, after passaged for 12 times continuously with low concentration of fcs. the virus could produce cpe. however, with vero cell line. the virus could not procuce any cpe after many passages. the hemagglutination and lumadsorption reaction test proved that this virus had no any reaction to erythrocyte of pig, fowl and cavy. by neutrolizaion assay, dxmv could be identified as a kind of ccv
理化學研究表明,該病毒為rna病毒,對氯仿、乙醚敏感;胰酶試驗中,經37 、 1小時處理的病毒,仍然能夠在貓源細胞fcwf細胞上生長,並且毒力基本保持不變;耐酸性試驗中,病毒分別在ph5 . 0和ph3 . 0經37作用2小時,毒力僅下降一個滴度;耐熱性試驗中,該病毒在恆定溫度50 ,設定不同時間,從5分鐘到150分鐘,毒力均有不同程度下降,其中, 50作用30分鐘,病毒平均滴度下降2個單位; 50 , 60分鐘, cpe消失;恆定時間1小時,設定不同溫度( 50 - 60 - 70 - 80 ) ,病毒在細胞上完全喪失增殖能力, cpe消失。生物學試驗,利用實驗室現有條件,選擇不同的細胞系對該病毒進行培養,發現該病毒對貓源細胞fcwf最敏感; mdck細胞次之; f81細胞經多次傳代,亦可出現cpe ;而vero細胞則不敏感。血凝試驗表明,該病毒對豬、雞、人及豚鼠的紅細胞均無血凝性。As indicated above, several m1gs that cleaved hcmv ul54 mrna segments in vitro were successfully designed and constructed. our studies demonstrates the utility of this ribozyme m1gs for antiviral application
我們的研究成功地利用引導序列,將核酶rnasep催化亞單位m1rna構建為序列識別的核酶m1gs ,證實了核酶在抗病毒方面的應用價值。Effects of arsenic trioxide on htert expression and tolemerase activity of human colonic carcinoma xenograft in nude mice
三氧化二砷對人結腸癌裸鼠移植瘤端粒酶活性及其催化亞單位表達的影響The sod activity in s. maltophilia 276 increased rapidly during the bacteria growth at early log phase, and reached highest with 570 units / ml of cell extract ( from 10 ml of cell culture ) at the end log phase of bacterial growth. the sod activity decreased when the bacteria entered growth of stationary phase. it was clear that the production of sod by s. maltophilia276 was consistent with the growth of bacteria
Maltophilia276菌株對數生長前期, sod的活性迅速增強;到對數生長後期,其活性達到最大,此時每毫升該細菌培養液的sod含量達到570iu (酶活力單位) ;在細菌進入生長穩定期后, sod的活性開始下降,這就說明276菌株所產生的sod活性同該菌的生長量是一致的。In our study we have cloned the osd gene from s. typhimurium by pcr, characterized the gene product and used this gene to construct asd + expression cloning vectors ptrc99a - asd
再將hpylori尿素酶b亞單位基因與尿素酶b和熱休克蛋白a融合基因分別克隆入ptrc99a一asd質粒的多克隆位點之內。Advance on catalytic subunit of telomerase in tumor
端粒酶催化亞單位在惡性腫瘤中的研究進展An array of regulatory proteins have been found, which inhibit the formation of central enzymes involved in early stages of the complement activation pathway. these include membrane cofactor protein ( mcp cd46 ), decay - accelerating factor protein ( daf cd5 5 ), complement receptor 1 ( cr1, cd35 ), as well as cd59, which inhibits formation of the membrane attack complex during later stages. these regulatory factors are widely expressed and abundant on many cells, and in fluids of reproductive system
目前發現,機體多種細胞以及生殖系統的體液中表達和分泌豐富的補體調控蛋白,包括作用於補體活化早期階段的cd55 、 cd46 、 cd35和作用於補體活化終末階段的cd59 ,它們分別通過抑制補體活化過程中關鍵的c3 、 c5轉化酶和抑制形成膜攻擊單位,抵抗補體對自身組織細胞的攻擊。The enzyme reacted with the calf thymus dna at different temperature, then its activity unit was detected
將該酶在不同溫度下與小牛胸腺dna反應后測定酶的活力單位。The targeting enzyme reacted with the calf thymus dna at different ph, then its activity unit was detected
將該酶在不同ph條件下與小牛胸腺dna反應后測定酶的活力單位。The purified dnaase reacted with the calf thymus dna at different naci concentration at ph5. 4, at 41, then its activity unit was detected
在不同的naci濃度下41 、 phs 4下準確反應15分鐘后測定酶的活力單位。The different bivalent cations with the same final concentration were put into the dnaase reacting system for 15 minute at ph5. 4, at 41, then dnaase ' s activity unit was detected
在dna酶的酶促反應體系中加入終濃度相同的二價金屬陽離子41下、 phs 4準確反應15分鐘后測定酶的活力單位。Reverse malignant phenotypes of colonic carcinoma cells transfected with antisense gene to htrt
反義人端粒酶催化亞單位基因轉染對人結腸癌細胞惡性表型的逆轉作用The findings of this phase ii dose - finding study also suggest that an effective dose is 25, 000 units of lipase, 25, 000 units of protease, and 3750 units of amylase
這項ii期藥物劑量摸索研究的結果還表明,有效劑量是25 , 000單位脂酶, 25 , 000單位蛋白酶和3750單位澱粉酶。Expression of telomerase subunits in normal liver tissue and hepatocellular carcinoma tissue
肝細胞癌組織和正常肝組織中端粒酶亞單位的表達In this study the definition is under the conditions of 55, ph4. 6, from 0. 1 % phytic acid sodium salt, release 1 nmol free phosphorus in one mintiue is one enzyme activity unit and the acetone method is the suitable measure way of the research was also decided
確定本實驗用的植酸酶酶活定義為: 55 , ph4 . 6的條件下,每分鐘從0 . 1的植酸鈉溶液中釋放1nmol的無機磷為一個酶活單位( u ) 。Methods : in cultured lung explants without serum, the lipid component synthesis of pulmonary surfactant was evaluated in [ 3h ] - choline incorporation ; mrna content of phosphocholine cytidylyltransferase ( cct ) in lung explants was investigated in rt - pcr ; the changes of the ultrastructure of the at ii cells were observed with electron microscope ; the expression of nmdar1 subtype was observed in immunohistochemistry staining ; nitric oxide synthase ( nos ) activity, nitric oxide ( no ) content, superoxide dismutase ( sod ) level, malondialdehyde ( mda ) content and lactae dehydroase ( ldh ) level were determined by biochemistry methods. results : 1. influence of glutamate on synthesis of the lipid component of pulmonary surfactant ? with l - arginine, glu inhibited [ 3h ] - choline incorporation with good dose - dependence and time - dependence ; ( 2 ) mrna content of cct of the glu treatment groups was decreased ; ( 3 ) glu increases the release of ldh in cultured lung explants ; ( dwith electron microscope histochemistry, glu induced the changes of the ultrastruture of at ii iv cells
方法:採用成年大鼠肺組織無血清培養,運用[ ~ 3h ] -膽堿摻入法測定ps主要脂質磷脂酰膽堿( pc )合成量; rt - pcr擴增檢測肺組織中pc合成限速酶磷酸膽堿二胞苷酰基轉移酶( cct ) mrna含量;透射電子顯微鏡法觀察肺泡型上皮細胞和ps系統超微結構的變化;免疫組織化學染色檢測glu的受體nmdar1亞單位的表達;生化測定肺組織乳酸脫氫酶( ldh )釋放量和肺組織勻漿中一氧化氮合酶( nos )活性、一氧化氮( no )生成量、超氧化物歧化酶( sod )水平以及丙二醛( mda )含量。Mpf ( m phase promoting factor ) which is made up of cdc2 as the active subunit and cyclin b as the regular subunit is a key factor in cell division. cdc2 is the active part of the mpf, which can active multiple ser / thr
Mpf ( mphasepromotingfactor )是細胞分裂的中心調控因子,由催化亞基cdc2和調節亞基周期素b ( cyclinb )組成,其中cdc2是mpf的活性單位,具有絲蘇氨酸蛋白激酶活性。It has made the strong basis for further studying mechanism of replication, virulence and determinant, attenuation, pathogenesis, functions of genetic products, specific diagnosis, cell and host tropism, development of dna vaccine and marker vaccine of csfv, and provided an excellent tool for molecular virology. main research contents include : based on published nucleotide sequences of csfv and by the help of computer analysis software, high conservative regions and single restriction enzyme sites of genome were selected. utilizing rt - pcr and nested - pcr techniques, 7 overlapping cdna fragments covering the full genome of csfv c - strain were successfully amplified
中國豬瘟兔化毒(脾淋毒)基因組cdna文庫的構建、序列分析:根據已發表的豬瘟病毒( csfv )核苷酸序列,藉助計算機軟體分析,選擇高保守區段和基因組中的單一限制性酶切位點,利用rt - pcr及nested - pcr和helf - nestedpcr技術,成功地擴增出了覆蓋c -株全基因組的7個cdna重疊片段f1 f7 ,分別克隆到pmd - 18t或pgem - teasy載體進行測序后,拼接出了其核苷酸序列。On the base of construction of pbi121vp7, we constructed the fusion gene expression vector pbi121ctbvp7 by the same sigle cloning site ( ndei and xbai ) of vector puc19ctb and pbi121vp7
設計具有ndei和saci單限制性酶切位點的vp7基因引物,通過pcr擴增出vp7基因並經測序驗證。As a result of adapting shaded environment, large variations took place in photosynthetic unit size, electron transmission, pigment content, endogenous hormones and enzyme activities, morphological and anatomical structure, nutrient absorption and distribution to ensure fully utilizing light energy at shading conditions, and to maintain its energy equilibrium and normal life activities
草本植物為適應蔭的環境,導致在光合作用單位、電子傳遞、光合色素含量、內源激素及酶活性、植株形態解剖結構、營養物質的吸收及分配等方面產生變化,以保證在遮蔭下仍能充分利用光能,維持生長所需的能量平衡,進行正常的生命活動。分享友人