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乳光腔肠蚓溶细胞素A-III对细胞膜的损伤。单价和二价阳离子对A-III溶血活性的影响。

Membrane damage by Cerebratulus lacteus cytolysin A-III. Effects of monovalent and divalent cations on A-III hemolytic activity.

作者信息

Liu J W, Blumenthal K M

机构信息

Department of Biochemistry and Molecular Biology, University of Cincinnati, College of Medicine, OH 45267.

出版信息

Biochim Biophys Acta. 1988 Jan 13;937(1):153-60. doi: 10.1016/0005-2736(88)90237-4.

Abstract

The effects of monovalent and divalent cations on the hemolytic activity of Cerebratulus lacteus toxin A-III were studied. The activity of cytolysin A-III is remarkably increased in isotonic, low ionic strength buffer, the HC50 (the toxin concentration yielding 50% lysis of a 1% suspension of erythrocytes after 45 min at 37 degrees C) being shifted from 2 micrograms per ml in Tris or phosphate-buffered saline to 20-30 ng per ml in sucrose or mannitol buffered with Hepes, corresponding to a 50-100-fold increase in potency. On the contrary, hemolytic activity decreases progressively as the monovalent cation concentration in the medium increases for Na+, K+, or choline salts. The divalent cations Ca2+ and Zn2+ likewise inhibit the cytolysin A-III activity, but more strongly than do the monovalent cations specified above. Zn2+ at a concentration of 0.3 mM totally abolishes both toxin A-III-dependent hemolysis of human erythrocytes and toxin-induced leakage from liposomes. The observation of similar effects in both natural membranes and artificial bilayers suggests an effect of Zn2+ on the toxin A-III-induced membrane lesion, especially since Zn2+ does not alter binding of the cytolysin. The dose-response curve for toxin A-III exhibits positive cooperativity, with a Hill coefficient of 2 to 3. However, analysis of toxin molecular weight by analytical ultracentrifugation reveals no tendency to aggregate at protein concentrations up to 2 mg per ml. These data are consistent with a post-binding aggregational step which may be affected by the ionic strength of the medium.

摘要

研究了单价和二价阳离子对乳脑纽虫毒素A-III溶血活性的影响。在等渗、低离子强度缓冲液中,溶细胞素A-III的活性显著增加,HC50(在37℃下45分钟后使1%红细胞悬液发生50%溶血的毒素浓度)从Tris或磷酸盐缓冲盐水中的每毫升2微克转变为用Hepes缓冲的蔗糖或甘露醇中的每毫升20 - 30纳克,效力相应增加了50 - 100倍。相反,随着培养基中单价阳离子(Na⁺、K⁺或胆碱盐)浓度的增加,溶血活性逐渐降低。二价阳离子Ca²⁺和Zn²⁺同样抑制溶细胞素A-III的活性,但比上述单价阳离子的抑制作用更强。浓度为0.3 mM的Zn²⁺完全消除了毒素A-III依赖的人红细胞溶血以及毒素诱导的脂质体渗漏。在天然膜和人工双层膜中观察到类似的效应,这表明Zn²⁺对毒素A-III诱导的膜损伤有影响,特别是因为Zn²⁺不会改变溶细胞素的结合。毒素A-III的剂量反应曲线表现出正协同性,希尔系数为2至3。然而,通过分析超速离心对毒素分子量的分析表明,在蛋白质浓度高达每毫升2毫克时没有聚集倾向。这些数据与结合后可能受培养基离子强度影响的聚集步骤一致。

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