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首页> 外文期刊>Biochimica et biophysica acta. Biomembranes >A comparison of the fluorescence properties of TMA-DPH as a probe for plasma membrane and for endocytic membrane
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A comparison of the fluorescence properties of TMA-DPH as a probe for plasma membrane and for endocytic membrane

机译:TMA-DPH用作质膜和内吞膜探针的荧光性质比较

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摘要

In earlier studies, the fluorescence probe 1-(4-(trimethylamino)phenyl)-6-phenylhexa-1,3,5-triene (TMA-DPH) was shown to interact with living cells by instantaneous incorporation into the plasma membrane, according to a water (probe not fluorescent)/membrane (probe highly fluorescent) partition equilibrium. This made it interesting both as a fluorescence anisotropy probe for plasma membrane fluidity determinations and as a quantitative tracer for endocytosis and intracellular membrane traffic. In order to ascertain the limiting concentrations for its use in these applications, we performed a systematic study of its fluorescence properties (intensity, lifetime, anisotropy) in the plasma membrane and in endocytic membranes of intact L929 mouse fibroblasts. Some of the experiments were repeated on mouse-bone-marrow-derived macrophages and on phospholipidic LUV to confirm the results. Rather unexpectedly, it was observed that: (i) the incorporation of TMA-DPH into the membranes, monitored by UV absorption measurements, remained proportional to the probe concentration over the wide range explored (5 · 10?7 M–2.5 · 10?5 M); (ii) however, concerning fluorescence, quenching effects occurred in the membranes above certain critical concentrations. These effects were shown to result from F?rster-type resonance auto-transfer; (iii) strikingly, the critical concentrations were considerably higher in early-endocytic-vesicle membranes than in the bulk plasma membrane. It was established that membrane fluidity was involved and this was confirmed by the parallel study on phospholipidic vesicles. Potential applications of these properties as a novel approach for evaluating membrane fluidity are suggested.
机译:在较早的研究中,荧光探针1-(4-(三甲基氨基)苯基)-6-苯基六-1,3,5-三烯(TMA-DPH)被证明通过瞬时掺入质膜与活细胞相互作用。达到水(探针不发荧光)/膜(探针强发荧光)的分配平衡。这既使荧光各向异性探针可用于质膜流动性测定,又可作为定量示踪剂用于内吞作用和细胞内膜运输,因此非常有趣。为了确定其在这些应用中使用的极限浓度,我们对完整的L929小鼠成纤维细胞的质膜和内吞膜中的荧光性质(强度,寿命,各向异性)进行了系统的研究。在源自小鼠骨髓的巨噬细胞和磷脂LUV上重复了一些实验,以证实结果。出乎意料的是,观察到:(i)在紫外吸收测量的监测下,TMA-DPH掺入膜中的比例在探索的大范围内仍与探针浓度成正比(5·10?7 M–2.5·10? 5 M); (ii)但是,关于荧光,超过某些临界浓度的膜发生了猝灭作用。这些作用表明是由弗斯特型共振自动转移引起的。 (iii)惊人的是,早期内吞囊泡膜中的临界浓度比体质膜中的临界浓度高得多。已经确定涉及膜的流动性,并且这通过对磷脂囊泡的平行研究得到证实。建议将这些性质作为评估膜流动性的新方法的潜在应用。

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