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正常皮肤和银屑病皮肤角质形成细胞的质膜流动性:一项使用三甲基铵二苯基己三烯(TMA-DPH)荧光各向异性的研究。

Plasma membrane fluidity of keratinocytes of normal and psoriatic skin: a study using fluorescence anisotropy of trimethylammoniumdiphenylhexatriene (TMA-DPH).

作者信息

Simonetti O, Ferretti G, Offidani A M, Gervasi P, Curatola G, Bossi G

机构信息

Clinica Dermatologica, Ospedale Umberto I, Piazza Cappelli, Ancona, Italy.

出版信息

Arch Dermatol Res. 1996;288(1):51-4. doi: 10.1007/BF02505043.

Abstract

The aim of this study was to investigate plasma membrane fluidity in human keratinocytes using fluorescence anisotropy of 1,6-diphenyl-1,3,5-hexatriene (DPH) and its cationic derivative 1-[4-(trimethylamino)-phenyl]-6-phenyl-1,3,5-hexatriene (TMA-DPH). Keratinocytes from normal or psoriatic skin were isolated using trypsin-EDTA or dispase. In keratinocytes isolated from normal skin, TMA-DPH anisotropy values were higher than those observed using DPH; the difference must be related to the different localization of the two probes. In fact, DPH in whole cells localizes in plasma as well as intracellular membranes, yielding an average value of fluidity, while the cationic derivative TMA-DPH resides in the plasma membrane of the whole cells for a sufficient time for anisotropy measurements. Moreover, it has to be considered that plasma membrane is more ordered than intracellular membranes. The kinetics of incorporation of TMA-DPH was similar in keratinocytes isolated using trypsin-EDTA and those isolated using; dispase, however, the fluorescence anisotropy values were lower in keratinocytes isolated with dispase (0.260 +/- 0.01 vs 0.270 +/- 0.01, p = 0.029). This difference is probably related to modifications of lipid-protein interactions after trypsin treatment. Since no damage to plasma membrane after incubation with dispase seems to have been reported, we decided to use this separation procedure to study plasma membrane fluidity in psoriasis, a human pathological condition characterized by excessive cell proliferation and incomplete differentiation. Lower anisotropy values (0.260 +/- 0.01 vs 0.270 +/- 0.01, p = 0.001), indicating an increase in fluidity, were observed in keratinocytes isolated from skin of psoriatic patients than in epidermal cells isolated from normal human skin. We suggest that the measurement of fluorescence anisotropy in living cells is a convenient and useful tool to study membrane fluidity in human keratinocytes isolated from normal and diseased skin. Its application represents a technical advance because plasma membrane fluidity can be measured using very limited amounts of tissue, as obtained from biopsies.

摘要

本研究的目的是利用1,6 - 二苯基 - 1,3,5 - 己三烯(DPH)及其阳离子衍生物1 - [4 - (三甲氨基) - 苯基] - 6 - 苯基 - 1,3,5 - 己三烯(TMA - DPH)的荧光各向异性来研究人角质形成细胞的质膜流动性。使用胰蛋白酶 - EDTA或中性蛋白酶分离正常或银屑病皮肤的角质形成细胞。在从正常皮肤分离的角质形成细胞中,TMA - DPH各向异性值高于使用DPH时观察到的值;这种差异必定与两种探针的不同定位有关。实际上,全细胞中的DPH定位于质膜以及细胞内膜,产生流动性的平均值,而阳离子衍生物TMA - DPH在全细胞质膜中停留足够长的时间以进行各向异性测量。此外,必须考虑到质膜比细胞内膜更有序。使用胰蛋白酶 - EDTA分离的角质形成细胞与使用中性蛋白酶分离的角质形成细胞中TMA - DPH的掺入动力学相似,然而,用中性蛋白酶分离的角质形成细胞中的荧光各向异性值较低(0.260±0.01对0.270±0.01,p = 0.029)。这种差异可能与胰蛋白酶处理后脂 - 蛋白相互作用的改变有关。由于未报道用中性蛋白酶孵育后对质膜有损伤,我们决定使用这种分离方法来研究银屑病中的质膜流动性,银屑病是一种以细胞过度增殖和不完全分化为特征的人类病理状况。在从银屑病患者皮肤分离的角质形成细胞中观察到比从正常人皮肤分离的表皮细胞更低的各向异性值(0.260±0.01对0.270±0.01,p = 0.001),表明流动性增加。我们认为,测量活细胞中的荧光各向异性是研究从正常和患病皮肤分离的人角质形成细胞质膜流动性的一种方便且有用的工具。它的应用代表了一项技术进步,因为可以使用从活检获得的非常少量的组织来测量质膜流动性。

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