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首页> 外文期刊>The Journal of Nuclear Medicine >A beta-camera integrated with a microfluidic chip for radioassays based on real-time imaging of glycolysis in small cell populations.
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A beta-camera integrated with a microfluidic chip for radioassays based on real-time imaging of glycolysis in small cell populations.

机译:基于微细胞群体中糖酵解实时成像的β-相机与微流控芯片集成,可进行放射分析。

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An integrated beta-camera and microfluidic chip was developed that is capable of quantitative imaging of glycolysis radioassays using (18)F-FDG in small cell populations down to a single cell. This paper demonstrates that the integrated system enables digital control and quantitative measurements of glycolysis in B-Raf(V600E)-mutated melanoma cell lines in response to specific B-Raf inhibition. METHODS: The beta-camera uses a position-sensitive avalanche photodiode to detect charged particle-emitting probes within a microfluidic chip. The integrated beta-camera and microfluidic chip system was calibrated, and the linearity was measured using 4 different melanoma cell lines (M257, M202, M233, and M229). Microfluidic radioassays were performed with cell populations ranging from hundreds of cells down to a single cell. The M229 cell line has a homozygous B-Raf(V600E) mutation and is highly sensitive to a B-Raf inhibitor, PLX4032. A microfluidic radioassay was performed over the course of 3 days to assess the cytotoxicity of PLX4032 on cellular (18)F-FDG uptake. RESULTS: The beta-camera is capable of imaging radioactive uptake of (18)F-FDG in microfluidic chips. (18)F-FDG uptake for a single cell was measured using a radioactivity concentration of 37 MBq/mL during the radiotracer incubation period. For in vitro cytotoxicity monitoring, the beta-camera showed that exposure to 1 muM PLX4032 for 3 days decreased the (18)F-FDG uptake per cell in highly sensitive M229 cells, compared with vehicle controls. CONCLUSION: The integrated beta-camera and microfluidic chip can provide digital control of live cell cultures and allow in vitro quantitative radioassays for multiple samples simultaneously.
机译:开发了一种集成的β相机和微流控芯片,该芯片能够使用(18)F-FDG在小细胞群体(直至单个细胞)中对糖酵解放射分析进行定量成像。本文证明了该集成系统能够对B-Raf(V600E)突变的黑色素瘤细胞系中的糖酵解进行数字控制和定量测量,以响应特定的B-Raf抑制作用。方法:β相机使用位置敏感的雪崩光电二极管来检测微流控芯片中带电粒子发射探针。校准了集成的β相机和微流控芯片系统,并使用4种不同的黑色素瘤细胞系(M257,M202,M233和M229)测量了线性。微流体放射分析的细胞群范围从数百个细胞到单个细胞。 M229细胞系具有纯合的B-Raf(V600E)突变,并且对B-Raf抑制剂PLX4032高度敏感。在3天的过程中进行了微流体放射分析,以评估PLX4032对细胞(18)F-FDG摄取的细胞毒性。结果:β照相机能够成像微流控芯片中(18)F-FDG的放射性摄取。 (18)在放射性示踪剂孵育期间,使用37 MBq / mL的放射性浓度测量单个细胞的F-FDG摄取。对于体外细胞毒性监测,β相机显示,与媒介物对照相比,在高度敏感的M229细胞中暴露于1μMPLX4032 3天可降低每细胞的(18)F-FDG摄取。结论:集成的β相机和微流控芯片可以提供活细胞培养的数字控制,并允许同时对多个样品进行体外定量放射测定。

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