blotting membrane 中文意思是什麼
blotting membrane
解釋
印跡膜-
In addition, the well retained stability and integrity of cell membrane of boea leaves might also be an important mechanism which make them resurrect well. by using mrna differential display, 5 desiccation sensitive cdnas, 52 desiccation - induced cdnas, 21 up - regulated cdnas, 14 down - regulated cdnas and 16 phosphate induced cdnas were obtained. the cloning, sequencing, homological blasting and northern blotting results of 5 desiccation - induced cdnas and 3 phosphate induced cdnas implied that signal transduction induced by desiccation, regulatory gene cascades and functional genes such as g protein, protein kinase, vp3 - and mad3 - like genes might be involved in dehydration in the resurrection plant boea hygrometrica
對其中5個脫水特異誘導表達牛耳草光合作廠j的脫水保護和復甦機理的cdna (包括可能與復甦能力有關的cdna )和3個磷酸鹽處理誘導表達的cdna進行克險測序、同源性探測和northern雜交檢測表明,牛耳草脫水過程中誘導表達的基因可能涉及到脫水脅迫的信號轉導「蛋白、蛋白激酶等) 、調節基因的級聯作用( vp3 , mad3樣基因等) 、結構基因產物調節細胞結構(包括細胞質膜)在脫水脅迫中的穩定性等。 -
After stimulation of insulin > epinephrine in 10 ~ 6m to the differentiated 3t3 - l1 cells for 48h, or incubated with 16. 8mm glucose for 48h, the crude membrane proteins were extracted, then investigated the effects of various factors on aqpap protein expression by western blotting. the subjects were divided into three groups according to body mass index : the normal, the overweight, the obese. the expression of adipose aqpap were detected with rt - pcr and western blotting
2 、利用半定量rt - pcr及westernblotting技術,從基因及蛋白質表達水平研究激素(胰島素、腎上腺素、地塞米松、 igf - 1 ) 、營養物質(葡萄糖、甘油) 、調脂藥(非諾貝特、洛伐他汀)對3t3 ? l1脂肪細胞aqpap表達的影響,並觀察不同體重研究對象脂肪組織aqpap表達量的變化。 -
The recombinant pcr technic was used to introduce a linking peptide klgggg to the site between scfv single chain form of the monoclonal antibody sz - 51 specific for the glycoprotein gmp140 on activated platelet membrane and uk32 low molecular weight form of pro - urokinase, to make the scfv - linker - uk32 chimeric gene. this gene was cloned into the transfer vector pbacpak9, and cotransfected with bacpak6 bsu36i digest into sf 9 cells. the fusion protein was secreted into the medium. in the fifth day after the cotransfection, the supernatant of the medium showed 107 iu ml fibrinolytic activity, higher than 25 iu ml fibrinolytic activity of scfv - uk32. elisa showed that the supernatant had the binding activity to activated platelet. wastern blotting also indicated that the supernatant could bind to the monoclonal antibody of urokinase b chain
為了提高重組導向溶栓分子scfv - uk32的溶纖活性,通過重組pcr方法在編碼scfv與uk32的堿基之間引入編碼klgggg連接肽的堿基序列,並克隆到轉移載體pbacpak9上,通過與線性病毒dna bacpak6 bsu36i digest共轉染到昆蟲細胞sf 9內,進行表達。表達產物分泌到上清中,共轉染后第5d天用纖維平板法測得sf 9細胞上清溶纖活性達到107 iu ml ,比未引入連接肽的scfv - uk32的表達活性25 iu ml高。
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