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      異惡唑醋酸_42228-92-2_產品詳情
      42228-92-2
      • names:

        Acivicin

      • CAS號:

        42228-92-2

        MDL Number: MFCD00866432
      • MF(分子式): C5H7ClN2O3 MW(分子量): 178.57
      • EINECS: Reaxys Number:42228-92-2
      • Pubchem ID:294641 Brand:BIOFOUNT
      異惡唑醋酸
      異惡唑醋酸(Acivicin,42228-92-2)Acivicin is a modified amino acid and structural analog of glutamine. Acivicin inhibits glutamine amidotransferases in the purine and pyrimidine biosynthetic pathways, thereby inhibiting tumor growth in cell lines dependent on glutamine metabolism. 
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      中文別名 異惡唑醋酸(Acivicin,42228-92-2);阿西維辛,阿西維奇(復合)
      英文別名 Acivicin(異惡唑醋酸,42228-92-2)
      CAS號 42228-92-2
      Inchi InChI = 1S / C5H7ClN2O3 / c6-3-1-2(11-8-3)4(7)5(9)10 / h2,4H,1,7H2,(H,9,10)/ t2-4,4 -/ m0 / s1
      InchiKey QAWIHIJWNYOLBE-OKKQSCSOSA-N
      分子式 Formula C5H7ClN2O3
      分子量 Molecular Weight 178.57
      溶解度Solubility
      性狀 固體粉末,Power
      儲藏條件 Storage conditions -20°C 3 years年 / In solvent溶液中:-80°C 6 months月 -20°C 1 month月
      異惡唑醋酸(Acivicin,42228-92-2)實驗注意事項:
      1.實驗前需戴好防護眼鏡,穿戴防護服和口罩,佩戴手套,避免與皮膚接觸。
      2.實驗過程中如遇到有毒或者刺激性物質及有害物質產生,必要時實驗操作需要手套箱內完成以免對實驗人員造成傷害
      3.實驗后產生的廢棄物需分類存儲,并交于專業生物廢氣物處理公司處理,以免造成環境污染Experimental considerations:
      1. Wear protective glasses, protective clothing and masks, gloves, and avoid contact with the skin during the experiment.
      2. The waste generated after the experiment needs to be stored separately, and handed over to a professional biological waste gas treatment company to avoid environmental pollution.
      Tag:異惡唑醋酸MSDS,異惡唑醋酸蒸汽壓,異惡唑醋酸合成,異惡唑醋酸標準,異惡唑醋酸應用,異惡唑醋酸合成,異惡唑醋酸沸點,異惡唑醋酸閃點,異惡唑醋酸用途,異惡唑醋酸溶解度,異惡唑醋酸價格,異惡唑醋酸作用,異惡唑醋酸結構式,異惡唑醋酸用處,異惡唑醋酸毒理性質,異惡唑醋酸物理性質
      產品說明 異惡唑醋酸(Acivicin,42228-92-2)(AT-125) 是一種有效的由豬鏈霉菌產生的天然產物,異惡唑醋酸是 γ-谷氨酰轉肽酶 (GGT) 的抑制劑3
      IntroductionAcivicin(異惡唑醋酸,42228-92-2)(AT-125) is a natural product produced byStreptomyces sviceusis aγglutamyl transpeptidase (GGT)inhibitor.
      Application1異惡唑醋酸具有抗代謝藥,代謝產物,抗腫瘤藥,EC 2.3.2.2(γ-谷氨酰轉移酶)抑制劑,抗微生物劑,抗衰老劑和谷氨酰胺拮抗劑的作用。
      Application2Acivicin inhibits glutamine amidotransferases in the purine and pyrimidine biosynthetic pathways, thereby inhibiting tumor growth
      Application3
      Structure-based identification of OATP1B1/3 inhibitors Molecular pharmacology/PMID: 23571415
      An in vivo large-scale chemical screening platform using Drosophila for anti-cancer drug discovery Disease models & mechanisms/PMID: 22996645
      Exploration of natural compounds as sources of new bifunctional scaffolds targeting cholinesterases and beta amyloid aggregation: the case of chelerythrine Bioorganic & medicinal chemis/PMID: 23062825
      Luminal transport of thiol S-conjugates of methylmercury in isolated perfused rabbit renal proximal tubules Toxicology letters/PMID: 22800651
      Glutathione and Bcl-2 targeting facilitates elimination by chemoradiotherapy of human A375 melanoma xenografts overexpressing bcl-xl, bcl-2, and mcl-1/Journal of translational medicine/PMID: 22233801

      Structure-based identification of OATP1B1/3 inhibitors

      Abstract

      Several recent studies show that inhibition of the hepatic transport proteins organic anion-transporting polypeptide 1B1 (OATP1B1) and 1B3 (OATP1B3) can result in clinically relevant drug-drug interactions (DDI). To avoid late-stage development drug failures due to OATP1B-mediated DDI, predictive in vitro and in silico methods should be implemented at an early stage of the drug candidate evaluation process. In the present study, we first developed a high-throughput in vitro transporter inhibition assay for the OATP1B subfamily. A total of 2000 compounds were tested as potential modulators of the uptake of the OATP1B substrate sodium fluorescein, in OATP1B1- or 1B3-transfected Chinese hamster ovary cells. At an equimolar substrate-inhibitor concentration of 10 µM, 212 and 139 molecules were identified as OATP1B1 and OATP1B3 inhibitors, respectively (minimum 50% inhibition). For 69 compounds, previously not identified as OATP1B inhibitors, concentration-dependent inhibition was also determined, yielding Ki values ranging from 0.06 to 6.5 µM. Based on these in vitro data, we subsequently developed a proteochemometrics-based in silico model, which predicted OATP1B inhibitors in the test group (20% of the dataset) with high specificity (86%) and sensitivity (78%). Moreover, several physicochemical compound properties and substructures related to OATP1B1/1B3 inhibition or inactivity were identified. Finally, model performance was prospectively verified with a set of 54 compounds not included in the original dataset. This validation indicated that 80 and 74% of the compounds were correctly classified for OATP1B1 and OATP1B3 inhibition, respectively.

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