体外人全血药物诱导mRNA的定量分析

IF 3 Q2 Medicine
M. Mitsuhashi, K. Endo, Kazuhiko Obara, H. Izutsu, T. Ishida, Norio Chikatsu, A. Shinagawa
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引用次数: 8

摘要

采用放射、博来霉素和依托泊苷三种不同的方法诱导肝素化人全血细胞凋亡,并采用我们报道的方法定量测定各种mRNA (Clin。化学2006;52:634 - 642)。我们发现细胞周期蛋白依赖性激酶抑制剂1A (p21)和p53细胞凋亡上调调节剂(PUMA)是白细胞中最敏感和最普遍的细胞凋亡mRNA标志物。为了确定阳性和阴性反应,将合成RNA加入裂解缓冲液中,并计算倍增率。837/880(95.1%)个数据点在0.75 ~ 1.5倍之间,874/880(99.3%)个数据点在0.5 ~ 2.0倍之间。用22种不同的药物刺激40例健康成人的血液样本,超过75%的样本对博来霉素(1 μM)、阿达红霉素(2 μM)、长春新碱(1 μM)、柔红霉素(2 μM)、阿糖胞苷(10 μM)有诱导p21和/或PUMA mRNA的反应,约25%的样本没有诱导作用。p21和PUMA mRNA应答之间、柔红霉素与阿糖胞苷、依达红霉素和长春新碱对p21和PUMA的应答之间存在显著相关性。全血中药物诱导mRNA的定量将被认为是离体的,是生物标志物筛选的合适平台,也是未来药物敏感性试验的模型系统。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Quantification of Drug-Induced mRNA in Human Whole Blood ex vivo
Apoptosis was induced in heparinized human whole blood by 3 different ways (radiation, bleomycin, or etoposide), and various mRNA were quantified using the method we reported (Clin. Chem. 2006; 52:634-642). We found that cyclin-dependent kinase inhibitor 1A (p21) and p53 upregulated modulator of apoptosis (PUMA) were the most sensitive and universal mRNA markers of apoptosis in leukocytes. In order to define positive and negative responses, a synthetic RNA was spiked into the lysis buffer and the fold increase was calculated. As a result, 837/880 (95.1%) of data points stayed between 0.75 and 1.5 fold increase, and 874/880 (99.3%) were within 0.5-2.0 fold increase. When blood samples from 40 healthy adults were stimulated with 22 different drugs, more than 75% of the samples responded to bleomycin (1 μM), idarubicin (2 μM), vincristine (1 μM), daunorubicin (2 μM), cytarabine (10 μM), to induce p21 and/or PUMA mRNA, and approximately 25% showed no induction. Significant correlation was found between p21 and PUMA mRNA responses, and between daunorubicin and cytarabine, idarubicin, and vincristine for both p21 and PUMA. The quantification of drug-induced mRNA in whole blood will be considered as ex vivo, and is a suitable platform for biomarker screening as well as a model system for drug sensitivity tests in future.
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来源期刊
CiteScore
3.70
自引率
0.00%
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审稿时长
8 weeks
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