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KGF and KGFR are expressed in Hela cells. Hela細胞中有KGF和KGFR的表達;
Hela cells were also injected to normal BALB/c and Kunming mice. 同時(shí)用Hela細胞作為陽(yáng)性腫瘤細胞對照，并接種于免疫功能正常的BALB/c小鼠和昆明種小鼠。
HPV16 E7 was expressed efficiently in HEK-293 and HeLa cells. 熒光顯微鏡下,轉染后HEK-293細胞和HeLa細胞表達綠色熒光蛋白。
Either the cell growth inhibitory rate or the colony inhibitory rate of the HeLa cells was 100%(P<0.01) after being exposed to 12 Gy irradiation, meanwhile, the value of 2,3-DPG was nearly unchanged(P>0.05). 12 Gy的輻射劑量能夠完全抑制腫瘤細胞的增生(細胞生長(cháng)抑制率及克隆形成抑制率均為100%25;P<0.;01);且不影響紅細胞的攜氧功能(不輻射與輻射后的2;3 DPG值無(wú)顯著(zhù)性差異;P>0
Methods: (1)To detect toxic effect of PAP to Hela cell by MTT assay. 方法:(1)用MTT法檢測PAP對Hela細胞的毒性作用;
RT-PCR showed that E1A gene had a stable transfection in Hela cells and obviously down-regulated Her-2 expression. RT-PCR結果顯示:E1A基因在Hela細胞中能穩定表達,E1A基因的轉染明顯降低了Her-2基因在Hela細胞中的表達水平;
Objective: To study the fate of LAK cell and rescuing effect of Astragalus polysaccharide (APS) during and following assault on Hela cells. 目的：進(jìn)一步探討LAK細胞攻擊Hela細胞后的歸宿及黃芪多糖（APS）的影響。
Low dose cisplatin can enhance the sensitivity of radiotherapy through change cell cycle of Hela cell lines. 小劑量順鉑可通過(guò)改變培養的人Hela細胞周期 ,誘導細胞G2 /M期延遲從而提高放療敏感性 ,可能與其內在的 p5 3基因表達改變有關(guān)。
At 12 h, the H_2O_2 level in HeLa cells and AsPC-1 cells were similar to that of the control group. 結論:As2O3誘導HeLa細胞和AsPC-1細胞凋亡與細胞內的H2O2水平改變有關(guān),而與HPV的感染無(wú)明顯相關(guān)性。
The s-lap/GFP fusion protein can express in Hela cells and locate in entire cells, but express highly in the nucleus. s- lap/ GFP融合蛋白可在人 Hela細胞中表達 ,并主要定位于細胞核。
Flow cytometry (FCM) was used to examine the effects of 4-HPR with or without DDP on cell cycle and apoptosis of HeLa cells. 采用流式細胞儀測定4-HPR、DDP、4-HPR+DDP對HeLa腫瘤細胞系細胞增殖周期和細胞凋亡的變化。
The CPE inhibition assay was used to test the antiviral activity of GD4 on RSV in Hela cells. 采用細胞病變抑制實(shí)驗,觀(guān)察GD4在Hela細胞中對RSV的抑制作用。
G418-resistant clones of Hela cells were obtained and confirmed as positive by RT-PCR. 重組質(zhì)粒轉染Hela細胞后,經(jīng)G418篩選成功獲得陽(yáng)性克隆。
Aim To evaluate the manner and molecular mechanism of HeLa cell death induced by Coxsackie virus B3(CVB3). 目的評價(jià)柯薩奇病毒B3CVB3致HeLa細胞死亡的方式及分子機制。
Gpd-Tp92 fusion gene constructed in pcDNA3.1 (+) vector could express a fusion protein in Hela cells. pcDNA3.;1(+)/Gpd-Tp92在HeLa細胞中能有效表達。
Both genes were cloned into GFP expression vector pIRES2 EGFP and transfected into HeLa cells. 將上述基因克隆入綠色熒光蛋白(GFP)表達載體pIRES2-EGFP中,轉染人HeLa細胞,在熒光顯微鏡和電鏡下觀(guān)察轉染細胞的形態(tài)和結構。
The KGF and KGFR genes were expressed in the Hela cells. The KGF and KGFR proteins were expressed in the Hela cells. 從基因水平和蛋白水平證實(shí)KGF及KGFR在Hela細胞中有表達。
The augment of G 1 ratio in the proliferation cycle of Hela cells presents a concentration-dependent manner. 細胞周期分析顯示槲皮素組 G 1 期細胞比例明顯增多，呈量-效關(guān)系。
Role of Mitochondria in HeLa Cell Apoptosis Induced by Hematoporphyrin monomethyl ether- PDT[J]. 引用該論文丁新民;劉凡光;顧瑛;曾晶;戴維德;李曉松.
Stably transfected and control Hela cell lines were injected subcutaneously into female Balb/c/nu mice. 穩定轉染Ang-2的細胞注射Balb/c裸鼠皮下。

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