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依赖ATP的蓖麻毒素跨纯化内体膜的转运

ATP-dependent translocation of ricin across the membrane of purified endosomes.

作者信息

Beaumelle B, Alami M, Hopkins C R

机构信息

Department of Biochemistry, Imperial College of Science, Technology and Medicine, London, United Kingdom.

出版信息

J Biol Chem. 1993 Nov 5;268(31):23661-9.

PMID:7901210
Abstract

Ricin translocation was demonstrated (using both fluorescence- and radiolabel-based assays) across the membrane of endosomes purified from mouse lymphocytes. Selectivity of the process was shown by the absence of translocation activity of transferrin and horseradish peroxidase used as membrane-bound and fluid-phase endosome labels, respectively. Endocytosed 125I-ricin translocation was found to be strictly ATP- (Km approximately 4 mM) and temperature-dependent, with up to 30% endosomal 125I-ricin appearing in the external medium after 2 h at 37 degrees C. No treatments neutralizing the acidic endosome pH (ammonium chloride, nigericin, chloroquine) significantly impaired ricin translocation, and the pH gradient across the endosome membrane is not required for this process. Chase experiments showed that the ability of 125I-ricin to translocate increases with its depth in the endocytic system (i.e. plasma membrane << early endosomes < late endosomes). Both A and B ricin chains displayed translocation ability as demonstrated by the results of our assay on ricin, ricin B, transferrin-ricin A, and transferrin-ricin B conjugates. Biological activity of both ricin chains is preserved after translocation as shown by the inhibitory effect of the A chain on cell-free protein synthesis and the binding of the B chain to lactose-agarose.

摘要

利用基于荧光和放射性标记的检测方法,在从小鼠淋巴细胞中纯化得到的内体膜上证实了蓖麻毒素的转位。分别用作膜结合和液相内体标记的转铁蛋白和辣根过氧化物酶缺乏转位活性,这表明了该过程的选择性。发现内吞的125I-蓖麻毒素转位严格依赖ATP(Km约为4 mM)和温度,在37℃下2小时后,高达30%的内体125I-蓖麻毒素出现在细胞外培养基中。中和酸性内体pH值的处理(氯化铵、尼日利亚菌素、氯喹)均未显著损害蓖麻毒素的转位,并且该过程不需要内体膜上的pH梯度。追踪实验表明,125I-蓖麻毒素的转位能力随其在内吞系统中的深度增加而增强(即质膜<<早期内体<晚期内体)。我们对蓖麻毒素、蓖麻毒素B、转铁蛋白-蓖麻毒素A和转铁蛋白-蓖麻毒素B偶联物的检测结果表明,A链和B链均具有转位能力。转位后,蓖麻毒素两条链的生物学活性均得以保留,如A链对无细胞蛋白质合成的抑制作用以及B链与乳糖-琼脂糖的结合所示。

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