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Calibrators for Clinical Measurements of Phosphorylated H2AX in Patient Cells by Flow Cytometry

机译:通过流式细胞术临床测量患者细胞中磷酸化H2AX的校准物

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Agents that induce DNA double-strand breaks (DSBs), such as ionizing radiation, are frequently used in cancer therapy. H2AX is rapidly phosphorylated in response to DSBs and serves as a way to measure the extent of DSBs induced in patient cells. We have previously reported a flow cytometry-based method for measuring H2AX phosphorylation in pa-tient cells undergoing radiotherapy. To be able to implement measurement of H2AX phosphorylation in clinical practice, we have characterized calibrators for the flow cytometry analysis based on phosphopeptide-coated beads and fixed cells. The calibrator beads and fixed cells lost less than 11% of the signal after storage for 40 days under optimal conditions and were able to correct for day-to-day variation in method performance.
机译:诱导DNA双链断裂(DSB)的试剂,例如电离辐射,经常用于癌症治疗。 H2AX响应于DSB迅速被磷酸化,并用作测量患者细胞中诱导的DSB程度的一种方式。我们先前已经报道了一种基于流式细胞术的方法,用于测量正在接受放射治疗的患者细胞中H2AX磷酸化。为了能够在临床实践中实现H2AX磷酸化的测量,我们对基于磷酸肽包被的珠子和固定细胞的流式细胞仪分析进行了表征。在最佳条件下储存40天后,校准珠和固定细胞损失的信号少于11%,并且能够校正方法性能的日常变化。

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