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別名: LY 080400, NSC 83244 中文名稱:芹菜素,芹黃素,芹菜苷元
Apigenin是一種有效的CYP2C9抑制劑,Ki為2 μM.。
Apigenin Chemical Structure
CAS: 520-36-5


| 細胞系 | 實驗類型 | 給藥濃度 | 孵育時間 | 活性描述 | 文獻信息(PMID) |
|---|---|---|---|---|---|
| human THP1 cells | Function assay | 20 uM | 1 h | Inhibition of NOX2 in human THP1 cells assessed as downregulation of TPA-induced CD36 mRNA expression at 20 uM incubated for 1 hr prior to TPA challenge measured after 24 hrs by RT-PCR analysis | |
| MDA-MB-231 cells | Function assay | 5 uM | Inhibition of PMA-stimulated NF-kappaB signaling (unknown origin) expressed in MDA-MB-231 cells at 5 uM incubated for 16 hrs by luciferase reporter gene assay | ||
| human MV4-11 cells | Cytotoxicity assay | 72 h | Cytotoxicity against human MV4-11 cells harboring FLT3 mutation after 72 hrs by tetrazolium based Ez CyTox cell viability assay, GI50=2.81 μM | ||
| mouse RAW264.7 cells | Function assay | 24 h | Antiinflammatory activity against mouse RAW264.7 cells assessed as inhibition of LPS-induced nitrite accumulation after 24 hrs by Griess reagent method, IC50=6.7 μM | ||
| human H9 cells | Function assay | 3 days | Antiviral activity against HIV1 3B infected in human H9 cells assessed as inhibition of viral replication after 3 days by p24 antigen capture assay, EC50=9 μM | ||
| HEK293 cells | Function assay | 24 h | Agonist activity at mouse PPARgamma expressed in HEK293 cells co-expressing with Gal4 reporter vector after 24 hrs by dual-luciferase reporter assay, EC50=24.9 μM | ||
| mouse 26-L5 cells | Proliferation assay | 72 h | Antiproliferative activity against mouse 26-L5 cells after 72 hrs by MTT assay, EC50=25 μM | ||
| human RS4:11 cells | Cytotoxicity assay | 72 h | Cytotoxicity against human RS4:11 cells harboring wild type FLT3 after 72 hrs by tetrazolium based Ez CyTox cell viability assay, GI50=27.9 μM | ||
| mouse B16-BL6 cells | Proliferation assay | 72 h | Antiproliferative activity against mouse B16-BL6 cells after 72 hrs by MTT assay, EC50=31.6 μM | ||
| human H9 cells | Cytotoxicity assay | 3 days | Cytotoxicity against human H9 cells after 3 days, IC50=35 μM | ||
| human HT1080 cells | Proliferation assay | 72 h | Antiproliferative activity against human HT1080 cells after 72 hrs by MTT assay, IC | ||
| mouse L929 cells | Function assay | 15 mins | Potentiation of recombinant human TNF-alpha-induced cytotoxicity of mouse L929 cells assessed as survivality preincubated for 15 mins before TNFalpha addition measured after 24 hrs by crystal violet staining | ||
| mouse RAW264.7 cells | Function assay | Inhibition of COX2 protein expression in mouse RAW264.7 cells, IC50=0.5 μM | |||
| human H295R cells | Function assay | Inhibition of aromatase expressed in human H295R cells, IC50=1 μM | |||
| HEK293 FS cells | Function assay | Inhibition of NOX4 expressed in HEK293 FS cells assessed as H2O2 production by H2O2/Tyr/LPO assay, IC50=1.13 μM | |||
| human HeLa cells | Function assay | Inhibition of MRP1 transfected in human HeLa cells assessed as inhibition of [3H]LTC4 transport by rapid filtration assay, Ki=2.4 μM | |||
| human mast cells | Function assay | Inhibition of SYK in human mast cells assessed as reduction in mast cell degranulation, EC50=3 μM | |||
| MDCK cells | Function assay | Inhibition of BCRP expressed in MDCK cells using Hoechst 33342 staining, IC50=3.1 μM | |||
| human MDA-kb2 cells | Function assay | Antagonist activity at androgen receptor in human MDA-kb2 cells assessed as inhibition of DHT-induced luciferase activity by luciferase reporter gene assay, IC50=5.2 μM | |||
| MCF-7 MX cells | Function assay | Inhibition of BCRP expressed in MCF-7 MX cells using Hoechst 33342 staining, IC50=5.9 μM | |||
| MDCK cells | Cytotoxicity assay | Cytotoxicity against MDCK cells by MTT assay, CC50=39.59 μM | |||
| 點擊查看更多細胞系數(shù)據(jù) | |||||
| 產品描述 | Apigenin是一種有效的CYP2C9抑制劑,Ki為2 μM.。 | ||
|---|---|---|---|
| 特性 | 對CT-L的抑制比 kaempferol和myricetin更有效。 | ||
| 靶點 |
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| 體外研究(In Vitro) | ||||
| 體外研究活性 | Apigenin通過與三磷酸腺苷(ATP)競爭而抑制PKC。Apigenin也降低TPA誘導的細胞蛋白的磷酸化水平,并抑制TPA誘導的c-jun和c-fos表達。Apigenin對轉化的v-H-ras表型的NIH3T3細胞具有反轉作用。在中國倉鼠卵巢細胞中,Apigenin能夠抑制硝基芘誘導的毒性基因引起的突變。在小鼠巨噬細胞中,Apigenin抑制LPS誘導的環(huán)氧合酶-2 和一氧化氮合成酶-2的活性和表達。Apigenin被報道具有抑制蛋白激酶C,分裂素激活的蛋白激酶(MAPK),C3HI小鼠胚胎成纖維細胞的轉化以及v-Ha-ras-轉化的NIH3T3細胞中下游致癌基因的活性。 Apigenin阻斷過氧物酶體增殖調控的激酶(ERK),離體肝細胞中的MAPK。Apigenin可以下調Na+/Ca2+-交換器的表達,該蛋白是大鼠心肌細胞鈣離子外排的一個重要蛋白。在表皮細胞和成纖維細胞中,Apigenin通過抑制p34 (cdc2)激酶活性引起G2/M and G0/G1可逆阻滯,并伴隨p53蛋白質穩(wěn)定性增加。在培養(yǎng)的人類內皮細胞中,Apigenin能夠有效抑制TNFα誘導的細胞粘附分子-1的上調。在人類卵巢癌細胞中,Apigenin通過PI3K/Akt/p70S6K1和HDM2/p53信號通路抑制HIF-1α 和 VEGF表達在人類角質細胞中,Apigenin通過抑制MAPK信號轉導并降低API轉錄因子水平抑制分化。Apigenin也會抑制人類角質細胞的增殖。 | |||
|---|---|---|---|---|
| 實驗圖片 | 檢測方法 | 檢測指標 | 實驗圖片 | PMID |
| Western blot | MHC / MHC2A / MHC2B / MyoD CXCR4 CDK1 / Cyclin B1 / p21 |
|
29108230 | |
| Immunofluorescence | E-caherin / Vimentin Snail |
|
27203387 | |
| Growth inhibition assay | Cell viability |
|
23224239 | |
| 體內研究(In Vivo) | ||
| 體內研究活性 | 在卵清蛋白免疫的BALB/C小鼠中,Apigenin下調IL-4的產生。Apigenin通過抑制腫瘤細胞和內皮細胞的相互作用抑制黑色素瘤的肺轉移。在雌性小鼠中,Apigenin引起子宮重量和整個子宮中雌激素受體(ER)-α濃度顯著增加,通過雌激素受體β1抑制前列腺癌和乳腺癌細胞生長。Apigenin抑制前列腺移植瘤中IGF-I水平,增加在血液循環(huán)中結合IGF-I 蛋白的IGFBP-3含量。 Apigenin (12.5 毫克/千克)增加成年小鼠海馬區(qū)齒狀回區(qū)域細胞的增殖。 | |
|---|---|---|
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| 分子量 | 270.24 | 分子式 | C15H10O5 |
| CAS號 | 520-36-5 | SDF | Download Apigenin SDF |
| 儲存條件(自收到貨起) | |||
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體外溶解度 |
DMSO : 54 mg/mL ( (199.82 mM) ;DMSO吸濕會降低化合物溶解度,請使用新開封DMSO) Water : Insoluble Ethanol : Insoluble |
摩爾濃度計算器 |
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體內溶解配方 現(xiàn)配現(xiàn)用,請按從左到右的順序依次添加,澄清后再加入下一溶劑 |
動物體內配方計算器 | |||||
動物體內配方計算器(澄清溶液)
第一步:請輸入基本實驗信息(考慮到實驗過程中的損耗,建議多配一只動物的藥量)
第二步:請輸入動物體內配方組成(配方適用于不溶于水的藥物;不同批次藥物配方比例不同,請聯(lián)系Selleck為您提供正確的澄清溶液配方)
計算結果:
工作液濃度: mg/ml;
DMSO母液配制方法: mg 藥物溶于μL DMSO溶液(母液濃度mg/mL,注:如該濃度超過該批次藥物DMSO溶解度,請先聯(lián)系Selleck);
體內配方配制方法:取μL DMSO母液,加入μL PEG300,混勻澄清后加入μL Tween 80,混勻澄清后加入μL ddH2O,混勻澄清。
體內配方配制方法:取μL DMSO母液,加入μL Corn oil,混勻澄清。
注意:1. 首先保證母液是澄清的;
2.一定要按照順序依次將溶劑加入,進行下一步操作之前必須保證上一步操作得到的是澄清的溶液,可采用渦旋、超聲或水浴加熱等物理方法助溶。
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