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采用 LC-MS/MS 监测 3'-脱氧-3'-氟胸苷(FLT)及其单磷酸代谢物(FLT-MP)在细胞内的积累,作为体外细胞增殖的衡量指标。

Monitoring cellular accumulation of 3'-deoxy-3'-fluorothymidine (FLT) and its monophosphate metabolite (FLT-MP) by LC-MS/MS as a measure of cell proliferation in vitro.

机构信息

Department of Pharmacokinetics, Dynamics, & Metabolism, Pfizer Worldwide Research and Development, San Diego, CA 92121, USA.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2011 Oct 15;879(28):2963-70. doi: 10.1016/j.jchromb.2011.08.024. Epub 2011 Aug 31.

DOI:10.1016/j.jchromb.2011.08.024
PMID:21925976
Abstract

Accurate measurement of in vitro cell growth is critical for oncology drug development, but cell counting and the most accurate indirect proliferation assays are impractical. Here, we describe a robust alternative method that monitors proliferating cell thymidine kinase 1 (TK1) activity via LC-MS/MS quantification of 3'-deoxy-3'-fluorothymidine (FLT) and its monophosphate metabolite FLT-MP. LNCaP prostate cancer cells were cultured at four densities (20,000; 10,000; 5000; and 500 cells/well) and incubated with 2000 ng/mL FLT in multi-well plates. Internal standards were FLT-d3 for FLT and d4-thymidine for FLT-MP. In culture medium, peak area ratios of FLT to FLT-d3 and FLT-MP to d4-thymidine were linear over the range 0.25-100 ng/mL (r(2)≥0.998). Accuracy for quality controls was between -7.3% and 6.3% for FLT, and from -3.3% to 1.7% for FLT-MP. Quality control precision was from 2.4% to 5.7% for FLT and 3.2% to 7.5% for FLT-MP. The limit of quantification was 0.25 ng/mL, with good control results (precision of 9.6% for FLT and 14.8% for FLT-MP). FLT-MP formation was linearly proportional to cell number from 500 to 20,000 cells/well 1 h after FLT addition. FLT-MP and ATP generation were comparable in LNCaP cells exposed to cell cycle inhibitor drugs (Spearman r=0.925, p<0.0001), demonstrating assay suitability for drug screening. This fit for purpose method is amenable to analysis of tumor tissue extracts, and should enable direct assessment of in vitro-in vivo relationships in animal models of cancer.

摘要

准确测量体外细胞生长对肿瘤药物开发至关重要,但细胞计数和最准确的间接增殖测定法不切实际。在这里,我们描述了一种可靠的替代方法,通过 LC-MS/MS 定量 3'-脱氧-3'-氟胸苷 (FLT) 及其单磷酸代谢物 FLT-MP 来监测增殖细胞胸苷激酶 1 (TK1) 活性。LNCaP 前列腺癌细胞在四种密度(20,000;10,000;5000 和 500 个细胞/孔)下培养,并在多孔板中用 2000ng/mL FLT 孵育。内标物为 FLT-d3 用于 FLT 和 d4-胸苷用于 FLT-MP。在培养基中,FLT 与 FLT-d3 和 FLT-MP 与 d4-胸苷的峰面积比在 0.25-100ng/mL 范围内呈线性(r(2)≥0.998)。FLT 的质控准确度在-7.3%至 6.3%之间,FLT-MP 的准确度在-3.3%至 1.7%之间。FLT 的质控精密度为 2.4%至 5.7%,FLT-MP 的精密度为 3.2%至 7.5%。定量限为 0.25ng/mL,控制效果良好(FLT 的精密度为 9.6%,FLT-MP 的精密度为 14.8%)。FLT 添加 1 小时后,FLT-MP 的形成与细胞数量呈线性比例,范围为 500 至 20,000 个细胞/孔。暴露于细胞周期抑制剂药物的 LNCaP 细胞中,FLT-MP 和 ATP 的产生相当(Spearman r=0.925,p<0.0001),表明该测定法适用于药物筛选。这种适合目的的方法适用于肿瘤组织提取物的分析,并且应该能够直接评估癌症动物模型中的体外-体内关系。

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引用本文的文献

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Monitoring metabolic responses to chemotherapy in single cells and tumors using nanostructure-initiator mass spectrometry (NIMS) imaging.利用纳米结构引发质谱(NIMS)成像技术监测单细胞和肿瘤对化疗的代谢反应。
Cancer Metab. 2013 Jan 23;1(1):4. doi: 10.1186/2049-3002-1-4.
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Limits of [18F]-FLT PET as a biomarker of proliferation in oncology.
[18F]-FLT PET 作为肿瘤增殖生物标志物的局限性。
PLoS One. 2013;8(3):e58938. doi: 10.1371/journal.pone.0058938. Epub 2013 Mar 15.