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首页> 外文期刊>Cell structure and function >Investigation of Factors Involved in the Uptake Velocity of Fluorescein Diacetate and Intracellular Fluorescence Polarization Value. I. Physiological Aspects in Lymphoblastoid Cells
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Investigation of Factors Involved in the Uptake Velocity of Fluorescein Diacetate and Intracellular Fluorescence Polarization Value. I. Physiological Aspects in Lymphoblastoid Cells

机译:双乙酸荧光素吸收速度和细胞内荧光偏振值的影响因素研究。 I.淋巴母细胞的生理方面

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摘要

References(25) Cited-By(4) Measurement of cellular fluidity by the fluorescence polarization method with a fluorogenic dye, fluorescein diacetate (FDA), is used widely. But values obtained with this method may be affected greatly by unknown factors. To determine the various factors that affect fluorescence polarization (FP-) measurements and intrinsic cellular fluidity, we investigated the uptake of FDA into cells, cellular esterases, fluorescein-binding protein, microtubules and osmolarity. Our results show that some reagents inhibit FDA-uptake without affecting esterases and that several types of esterases are involved in FDA-hydrolysis.The dye-binding experiment indicated that dye-binding protein is absent from the cells. In addition, to determine whether there is involvement of microtubules in cellular fluidity, we treated cells with Ca2+ antagonists, calmodulin inhibitors and low temperature, and verified that there is little evidence for that hypothesis. In other experiments, cells were brought into a hypertonic condition, which resulted in osmolysis and higher intracellular concentrations, primarily of biopolymers, and higher viscosity. The effect of this viscosity on the FP value was investigated. Results showed a parallel relationship between osmolarity and therefore, intracellular viscosity and FP value.In conclusion, the concentrations of intracellular proteins and other biopolymers appear to be a major factor that determines cellular fluidity, but the role of microtubules which undergo assembly-disassembly appears to be insignificant.
机译:参考文献(25)引用(4)使用荧光染料荧光二乙酸酯(FDA)通过荧光偏振法测量细胞的流动性。但是用这种方法获得的值可能会受到未知因素的很大影响。为了确定影响荧光偏振(FP-)测量和固有细胞流动性的各种因素,我们调查了FDA对细胞,细胞酯酶,荧光素结合蛋白,微管和渗透压的摄取。我们的结果表明,某些试剂在不影响酯酶的情况下抑制FDA摄取,并且FDA水解涉及多种类型的酯酶。染料结合实验表明细胞中不存在染料结合蛋白。另外,为了确定微管是否参与细胞流动性,我们用Ca2 +拮抗剂,钙调蛋白抑制剂和低温处理了细胞,并验证了没有关于该假说的证据。在其他实验中,细胞进入高渗状态,导致渗透作用和细胞内较高的浓度(主要是生物聚合物)和较高的粘度。研究了该粘度对FP值的影响。结果表明,渗透压与细胞内粘度和FP值之间存在平行关系。总而言之,细胞内蛋白质和其他生物聚合物的浓度似乎是决定细胞流动性的主要因素,但经历组装拆卸的微管的作用似乎无关紧要。

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