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化合物 U0126-EtOH,U0126-EtOH

化合物 U0126-EtOH|T6223|TargetMol

價格 167 383 617
包裝 1mg 5mg 10mg
最小起訂量 1mg
發(fā)貨地 上海
更新日期 2024-12-12
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產(chǎn)品詳情

中文名稱:化合物 U0126-EtOH英文名稱:U0126-EtOH
CAS:1173097-76-1品牌: TargetMol
產(chǎn)地: 美國保存條件: Powder: -20°C for 3 years | In solvent: -80°C for 1 year | Shipping with blue ice.
純度規(guī)格: 99.82%產(chǎn)品類別: 抑制劑
貨號: T6223
2024-12-12 化合物 U0126-EtOH U0126-EtOH 1mg/167RMB;5mg/383RMB;10mg/617RMB 167 TargetMol 美國 Powder: -20°C for 3 years | In solvent: -80°C for 1 year | Shipping with blue ice. 99.82% 抑制劑

Product Introduction

Bioactivity

名稱U0126-EtOH
描述U0126-EtOH (U0126 Ethanol) is a non-ATP competitive specific inhibitor of MEK1/2 (IC50: 0.07/0.06 μM).
細胞實驗HEK293 cells were maintained in Dulbecco's modification of Eagle's medium (low glucose) plus 10% foetal bovine serum. HeLa cells stably expressing wild type or kinase-dead LKB1 have been described. AMPK activity was determined by immunoprecipitate kinase assays using anti-AMPK-a1 and -a2 antibodies. Antibodies recognising AMPK phosphorylated on Thr-172 (anti-pT172), AMPK-α1 and -α2 and acetyl-CoA carboxylase-1 (ACC1) phosphorylated on Ser-80 [16] were described previously. Quantification of ratios of signals from phosphorylated and total protein using these antibodies was performed by dual labelling using the LI-COR Odyssey IR imager as described. Contents of ATP and ADP were determined for cells in 6 cm culture dishes by quickly pouring off the medium, adding 350 μl of ice-cold 5% perchloric acid, scraping the cells off with a plastic scraper, and centrifuging (14 000 · g; 3 min, 4 °C) to remove insoluble material. The perchloric acid was then extracted from the supernatant and nucleotides analysed by capillary electrophoresis of perchloric acid extracts as described previously. All incubations of cells were performed in triplicate and results are expressed as means ± S.E.M [3].
激酶實驗The amount of immunoprecipitated wild type MEK used in these assays was adjusted to give a similar amount of activity units as obtained with 10 nM recombinant MEK. All other assays were performed with a recombinant, constitutively activated mutant MEK-1 (ΔN3-S218E/S222D) or constitutively active MEK-2(S222E/S226D). Reaction velocities were measured using a 96-well nitrocellulose filter apparatus as described below. Unless otherwise noted, reactions were carried out at an enzyme concentration of 10 nM, in 20 mM Hepes, 10 mM MgCl2, 5 mM β-mercaptoethanol, 0.1 mg/ml BSA, pH 7.4, at room temperature. Reactions were initiated by the addition of [γ-33P]ATP into the premixed MEK/ERK/inhibitor reaction mixture, and an aliquot of 100 μl was taken every 6 min and transferred to the 96-well nitrocellulose membrane plate which had 50 mM EDTA to stop the reaction. The membrane plate was drawn and washed 4 times with buffer under vacuum. Wells were then filled with 30 μl of Microscint-20 scintillation fluid, and the radioactivity of33P-phosphorylated ERK was counted with a Top Count scintillation counter. Velocities were obtained from the slopes of radioactivity versus time plots. Concentrations of ERK and ATP were 400 nM and 40 μM, respectively, unless otherwise indicated [2].
動物實驗Prior to injection, FI cells were labeled with a stable fluorescent dye molecule, DiA at 10 μg/ml for 5 h at 37 1C. After washing to remove free DiA, cells were trypsinized for inoculation (U0126 experiments) or transfection (RNAi experiments). Biliary epithelial cells were injected subcutaneously, at the indicated times, into the tibia of nude mice. In the chemical experiments, 3h after inoculation, mice were treated with U0126 (10.5 mg/kg) daily by intraperitoneal injection. The length and width of each tumor were measured every day by using a caliper. The following formula was used to calculate tumor volumes ? width2 length/2. Mice were killed at the end of experiment. Tumors were immediately frozen in liquid nitrogen [5].
體外活性U0126通過非競爭性抑制具有雙特異性的激酶MEK的活性,從而抵抗AP-1轉(zhuǎn)錄活性,其IC50分別對MEK 1為0.07 microM,對MEK 2為0.06 microM [1]。在用TPA/血清處理的成纖維細胞中,U0126可以降低c-Fos和c-Jun蛋白的上調(diào)50-80%。使用10 μM U0126處理不會影響SP-1、JunD及Fra-1等本質(zhì)上表達的轉(zhuǎn)錄因子的蛋白水平[2]。在HEK293細胞中,U0126導致AMPK的磷酸化和激活,并增加了其下游靶標乙酰-CoA羧化酶的磷酸化,這一效應(yīng)僅在表達上游激酶LKB1的細胞中發(fā)生[3]。
體內(nèi)活性將小鼠通過氣霧劑途徑處理U0126,導致了以下結(jié)果:(i) 抑制了肺部MEK激活 (ii) 相比未經(jīng)處理的對照組,減少了后代IAV滴度 (iii) 保護了IAV感染的小鼠,對抗100倍致死性病毒挑戰(zhàn)[4]。在所有U0126 (10.5 mg/kg) 實驗中,移植和早期腫瘤生長顯著減少。此外,在注射后第9天及以后,用U0126處理的腫瘤體積減少了60-70%。U0126處理的小鼠中Cdk1表達也大幅降低[5]。
存儲條件Powder: -20°C for 3 years | In solvent: -80°C for 1 year | Shipping with blue ice.
溶解度10% DMSO+40% PEG300+5% Tween 80+45% Saline : 7.9 mg/mL (18.52 mM), Please add co-solvents sequentially, clarifying the solution as much as possible before adding the next one. Dissolve by heating and/or sonication if necessary. Working solution is recommended to be prepared and used immediately.
Ethanol : < 1 mg/mL (insoluble or slightly soluble)
DMSO : 55 mg/mL (128.93 mM)
關(guān)鍵字Influenza Virus | Mitogen-activated protein kinase kinase | MAP2K | U-0126-EtOH | MEK | inhibit | competitive | virus | Mitophagy | Autophagy | U0126EtOH | MAPKK | Mitochondrial Autophagy | U 0126 | Inhibitor | progeny | non-ATP | U0126-EtOH | U0126 EtOH | U-0126
相關(guān)產(chǎn)品Guanidine hydrochloride | Naringin | Valproic Acid | Taurine | Gefitinib | Aceglutamide | Hydroxychloroquine | Curcumin | Stavudine | Acetylcysteine | Paeonol | Sodium 4-phenylbutyrate
相關(guān)庫抑制劑庫 | 經(jīng)典已知活性庫 | 已知活性化合物庫 | 激酶抑制劑庫 | 高選擇性抑制劑庫 | 抗衰老化合物庫 | 抗病毒庫 | 酪氨酸激酶分子庫 | 疼痛相關(guān)化合物庫 | 鐵死亡化合物庫
關(guān)鍵字: U0126 Ethanol|||U0126|TargetMol

公司簡介

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