Department of Biochemistry, Michigan State University, East Lansing, MI 48824.
Proc Natl Acad Sci U S A. 1986 Jan;83(1):95-9. doi: 10.1073/pnas.83.1.95.
Fluorescent lipid and phospholipid probes were incorporated at 4 degrees C into soybean protoplasts prepared from cultured soybean (SB-1) cells. Fluorescence microscopy showed that the plasma membrane as well as the nucleus were labeled. Fluorescence redistribution after photobleaching (FRAP) analysis was performed on these cells at 18 degrees C to monitor the lateral mobility of the incorporated probes. After labeling at low concentrations (40 mug/ml) of phosphatidyl-N-(4-nitrobenzo-2-oxa-1,3-diazolyl)ethanolamine (NBD-PtdEtn), a single mobile component was observed with a diffusion coefficient (D) of approximately 3 x 10(-9) cm(2)/sec. After labeling at higher probe concentrations (>/=100 mug/ml), two diffusing species were observed, with diffusion coefficients of approximately 3 x 10(-9) cm(2)/sec ("fast") and approximately 5 x 10(-10) cm(2)/sec ("slow"). Similar results were observed with fluorescent derivatives of phosphatidylcholine and fatty acids. In contrast to these results, parallel analysis of 3T3 fibroblasts, using the same probes and conditions, yielded only a single diffusion component. These results suggest that the soybean plasma membrane may contain two distinct lipid domains in terms of lipid mobility. Consistent with this idea, experiments with soybean protoplasts yielded a single diffusion component under the following conditions: (i) labeling with NBD-PtdEtn (100 mug/ml), FRAP analysis at 37 degrees C (D = 1.1 x 10(-8) cm(2)/sec); (ii) labeling with NBD-PtdEtn (100 mug/ml), FRAP analysis at 18 degrees C in the presence of 2 mM EGTA (D = 4.2 x 10(-9) cm(2)/sec); (iii) labeling with 5-(N-dodecanoyl)aminofluorescein (a short-chain lipid probe), FRAP analysis at 18 degrees C or 37 degrees C (D = 2.5 x 10(-8) cm(2)/sec). These results suggest that the plasma membrane of soybean cells may contain stable immiscible domains of fluid and gel-like lipids.
荧光脂质和磷脂探针在 4°C 时被掺入到由培养的大豆(SB-1)细胞制备的大豆原生质体中。荧光显微镜显示,质膜和核都被标记了。在 18°C 下对这些细胞进行荧光漂白后荧光再分布(FRAP)分析,以监测掺入探针的横向流动性。在用磷脂酰-N-(4-硝基苯并-2-恶唑-1,3-二氮唑基)乙醇胺(NBD-PtdEtn)的低浓度(40μg/ml)进行标记后,观察到单个可移动的成分,其扩散系数(D)约为 3×10^(-9)cm^(2)/sec。在用更高的探针浓度(≥100μg/ml)进行标记后,观察到两种扩散物种,扩散系数约为 3×10^(-9)cm^(2)/sec(“快”)和约 5×10^(-10)cm^(2)/sec(“慢”)。用荧光衍生的磷脂酰胆碱和脂肪酸进行类似的分析,也得到了类似的结果。与这些结果相反,使用相同的探针和条件平行分析 3T3 成纤维细胞,仅得到一个扩散成分。这些结果表明,大豆质膜在脂质流动性方面可能包含两个不同的脂质域。与这个想法一致,用大豆原生质体进行的实验在以下条件下得到了单个扩散成分:(i)用 NBD-PtdEtn(100μg/ml)标记,在 37°C 进行 FRAP 分析(D=1.1×10^(-8)cm^(2)/sec);(ii)用 NBD-PtdEtn(100μg/ml)标记,在 18°C 且存在 2mM EGTA 时进行 FRAP 分析(D=4.2×10^(-9)cm^(2)/sec);(iii)用 5-(N-十二烷酰基)氨基荧光素(短链脂质探针)标记,在 18°C 或 37°C 进行 FRAP 分析(D=2.5×10^(-8)cm^(2)/sec)。这些结果表明,大豆细胞的质膜可能含有稳定的不相容的流体和凝胶状脂质域。
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