Wientzek M, Kay C M, Oikawa K, Ryan R O
Lipid and Lipoprotein Research Group, University of Alberta, Edmonton, Canada.
J Biol Chem. 1994 Feb 11;269(6):4605-12.
Apolipophorin-III (apoLp-III), a hemolymph protein of Manduca sexta, can reversibly associate with the surface of lipoprotein particles. In order to examine the lipid-associated form of apoLp-III, the present studies investigate the structure and properties of apoLp-III complexes with dimyristoylphosphatidylcholine (DMPC). Association of apoLp-III with DMPC vesicles results in the formation of uniform discs with an average diameter and width of 18.5 +/- 2.0 nm and 4.8 +/- 0.8 nm, respectively, as determined by electron microscopy. ApoLp-III.DMPC complexes analyzed by pore-limiting native gradient PAGE demonstrated that a single major species of complex was formed within a wide range of lipid to protein molar ratios (DMPC:apoLp-III; 13:1 to 360:1). Flotation equilibrium experiments, conducted in an analytical ultracentrifuge, confirmed that only one species of apoLp-III.DMPC complex was formed at an initial lipid to protein molar ratio of 67:1, with an apparent molecular mass of 642,000. Complexes cross-linked with dimethyl suberimidate indicate that there are a maximum of 6 apoLp-III molecules per disc. Circular dichroism experiments revealed that apoLp-III becomes essentially completely alpha-helical on formation of apoLp-III.DMPC complexes. Compared to apoLp-III in the lipid-free state, apoLp-III.DMPC complexes were relatively resistant to denaturation by guanidine HCl, displaying denaturation transitions with midpoints at 2.2 and 3.7 M guanidine HCl, respectively. The fluorescence excitation and emission spectra of apoLp-III.DMPC complexes demonstrate a large enhancement of tyrosine fluorescence as compared to the lipid-free state, suggesting that a conformational change occurs when apoLp-III associates with a lipid surface. Denaturation of apoLp-III in the complex by guanidine HCl resulted in a tyrosine fluorescence level similar to that of lipid-free apoLp-III in the presence of guanidine HCl. The tyrosine-induced fluorescence of the complex was quenched with both Cs+ (Kq = 0.573 M-1) and KI (Kq = 0.376 M-1). The results presented in this study indicate that the conformation of apoLp-III is stabilized when complexed with phospholipids and suggest that tyrosine fluorescence provides a sensitive method to detect M. sexta apoLp-III interaction with lipid surfaces.(ABSTRACT TRUNCATED AT 400 WORDS)
载脂蛋白-III(apoLp-III)是烟草天蛾血淋巴中的一种蛋白质,能与脂蛋白颗粒表面可逆结合。为了研究与脂质结合的apoLp-III形式,本研究探讨了apoLp-III与二肉豆蔻酰磷脂酰胆碱(DMPC)形成的复合物的结构和性质。通过电子显微镜测定,apoLp-III与DMPC囊泡结合形成了平均直径和宽度分别为18.5±2.0纳米和4.8±0.8纳米的均匀圆盘。通过孔径限制的天然梯度聚丙烯酰胺凝胶电泳分析apoLp-III.DMPC复合物表明,在较宽的脂质与蛋白质摩尔比范围内(DMPC:apoLp-III;13:1至360:1)形成了单一的主要复合物种类。在分析超速离心机中进行的浮选平衡实验证实,在初始脂质与蛋白质摩尔比为67:1时,仅形成一种apoLp-III.DMPC复合物,其表观分子量为642,000。用辛二酸二甲酯交联的复合物表明,每个圆盘最多有6个apoLp-III分子。圆二色性实验表明,apoLp-III在形成apoLp-III.DMPC复合物时基本上完全变成α-螺旋结构。与无脂质状态下的apoLp-III相比,apoLp-III.DMPC复合物对盐酸胍变性相对具有抗性,分别在2.2和3.7 M盐酸胍处显示变性转变中点。apoLp-III.DMPC复合物的荧光激发和发射光谱表明,与无脂质状态相比,酪氨酸荧光大幅增强,这表明apoLp-III与脂质表面结合时发生了构象变化。复合物中的apoLp-III被盐酸胍变性后,酪氨酸荧光水平与存在盐酸胍时无脂质的apoLp-III相似。复合物的酪氨酸诱导荧光被Cs+(猝灭常数Kq = 0.573 M-1)和KI(猝灭常数Kq = 0.376 M-1)猝灭。本研究结果表明,apoLp-III与磷脂复合时构象稳定,提示酪氨酸荧光为检测烟草天蛾apoLp-III与脂质表面相互作用提供了一种灵敏方法。(摘要截断于400字)
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