Fludarabine

製品コードS1491 バッチS149110

印刷

化学情報

 Chemical Structure Synonyms FaraA, Fludarabinum, NSC 118218 Storage
(From the date of receipt)
3 years -20°C powder
1 years -80°C in solvent
化学式

C10H12FN5O4

分子量 285.23 CAS No. 21679-14-1
Solubility (25°C)* 体外 DMSO 57 mg/mL (199.83 mM)
Water Insoluble
Ethanol Insoluble
体内 (毎回新しく調製した物を用意してください)
Homogeneous suspension
CMC-NA
≥5mg/ml Taking the 1 mL working solution as an example, add 5 mg of this product to 1 ml of CMC-Na solution, mix evenly to obtain a homogeneous suspension with a final concentration of 5 mg/ml.
* <1 mg/ml means slightly soluble or insoluble.
* Please note that Selleck tests the solubility of all compounds in-house, and the actual solubility may differ slightly from published values. This is normal and is due to slight batch-to-batch variations.

溶剤液(一定の濃度)を調合する

生物活性

製品説明 Fludarabine is a STAT1 activation inhibitor which causes a specific depletion of STAT1 protein (and mRNA) but not of other STATs. Also a DNA synthesis inhibitor in vascular smooth muscle cells. Fludarabine induces apoptosis.
in vitro

Fludarabine efficiently inhibits the proliferation of RPMI 8226 cells with IC50 of 1.54 μg/mL. The IC50 of this compound against MM.1S and MM.1R cells is 13.48 μg/mL and 33.79 μg/mL, respectively. In contrast, U266 cells are resistant to this chemical with IC50 of 222.2 μg/mL. This compound treatment results in increased number of cells in the G1 phase of cell cycle, accompanied with a concomitant reduction of cells at the S phase of cell cycle in a time-dependent manner. It induces a cell cycle block and triggers apoptosis in MM cells. It triggers time-dependent cleavage of caspase-8, -9, and -3, -7, followed by PARP cleavage. It increases expression of Bax in a time-dependent fashion, while the expression of Bak doesn't change. After exposure to this chemical for 12 hours, RPMI 8226 cells shows a loss of membrane potential with 61.05% of the cells expressing low fluorescence of rhodamine 123 compared with 8.62% of cells in untreated control. [1] To enhance solubility, it is formulated as the monophosphate (F-ara-AMP, fudarabine), which is instantaneously and quantitatively dephosphorylated to the parent nucleoside upon intravenous infusion. Inside the cells rephosphorylation occurs which leads to fuoroadenine arabinoside triphosphate (F-ara-ATP), the major cytotoxic metabolite of F-ara-A. [2] It can also induce pro-inflammatory stimulation of monocytic cells, as evaluated by increased expression of ICAM-1 and IL-8 release. [3] This compound does not affect the growth of ovarian cancer cell lines, whereas it induces marked and dose-dependent inhibition of proliferation in melanoma cell lines. [4] It is an inhibitor of STAT1 that specifically reduces STAT1 without affecting other STAT family members[5]. In addition to cytoplasmic accumulation, repeated low-dose cisplatin (RLDC) induces HMGB1 expression, which is marked suppressed by STAT1 knockdown. Consistently, this chemical suppresses HMGB1 expression during RLDC treatment dose-dependently in RLDC-treat renal tubular cells[5].

in vivo

Tumors treated with PBS grow rapidly to approximately 10-fold their initial volume in 25 day, whereas, the tumors in the Fludarabine at 40 mg/kg increase less than 5-fold. A significant antitumor effect of 40 mg/kg of this compound on RPMI8226 tumor growth is demonstrated. RPMI8226 tumors treated with 40 mg/kg of this chemical at day 10 increase apoptotic nuclei. This compound is effective in suppressing RPMI8226 myeloma xenografts in SCID mice. [1]

プロトコル(参考用のみ)

細胞アッセイ 細胞株 Dexamethasone-sensitive (MM.1S) and -resistant (MM.1R) human MM cell lines, RPMI8226 and U266 cell lines
濃度 2 μg/mL
反応時間 24 hours
実験の流れ

After treated with Fludarabine or control, dexamethasone-sensitive (MM.1S) and -resistant (MM.1R) human MM cell lines, RPMI8226 and U266 cell lines (5 × 105 cells) are washed twice in phosphate-buffered saline (PBS) and fixed with 70% ice-cold ethanol, then centrifuged and suspended in PBS containing 100 μg/mL RNase A. After incubated for 30 minutes at 37 ºC, samples are resuspended in 25 μg/mL propidium iodide. Flow cytometry is performed on a FACSCalibur automated system. Apoptosis is determined by Annexin V-FITC apoptosis detection kit, according to the manufacturer's instructions. For TUNEL (terminal deoxynucleotidyl transferase-mediated deoxyuridine triphosphate nick end labeling) assay, cells are analyzed by flow cytometry using the in situ cell death detection kit.

動物実験 動物モデル Severe combined immunodeficient (SCID) mice bearing RPMI 8226 cells
投薬量 40 mg/kg
投与方法 Administered via i.p.

参考

  • https://pubmed.ncbi.nlm.nih.gov/17976186/
  • https://pubmed.ncbi.nlm.nih.gov/10428391/
  • https://pubmed.ncbi.nlm.nih.gov/16546701/
  • https://pubmed.ncbi.nlm.nih.gov/8983288/
  • https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10240827/

カスタマーフィードバック

Data from [Data independently produced by Mol Cell Biol, 2014, 34(24), 4368-78.]

Data from [Data independently produced by , , Br J Cancer, 2018, 118(4):509-521]

Data from [Data independently produced by , , Brain Behav Immun, 2017, 60:161-173]

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人間や獣医の診断であるか治療的な使用のためにでない。

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