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Static light scattering study of complex formation between protein and neutral water-soluble polymer

机译:蛋白质与中性水溶性聚合物形成复合物的静态光散射研究

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Complex formation of poly(N-isopropylacrylamide) (PNIPA) having a weight-average molecular weight of 1,720,000 g/mol with human serum albumin (HSA), ovalbumin (OVA) and lysozyme (LYZ) was studied in an aqueous medium containing 0.01 M NaCl and adjusted to pH 3. The polymer–protein mixtures at different molar ratios (rm) were examined by static light scattering (SLS). The analysis of SLS data using our own approach [Kokufuta et al., Langmuir 15 (1999) 940; Biomacromolecules 4 (2003) 728] showed that the molecular weight of each resulting complex is smaller than that of the interpolymer complex composed of two polymer chains plus one protein. This indicates the formation of an intrapolymer complex in all the polymer–protein systems studied. Thus, at each rm we calculated the number of bound proteins per polymer, the value of which was OVA > HSA > LYZ in order. These results were compared with the hydropathy profiles of each protein which are a good tool for obtaining an information about distribution of hydrophobic and hydrophilic segments in a protein. It has become apparent that the hydrophobic interaction between polymer and protein plays an important role in the intrapolymer complex formation.
机译:在含有0.01 M的水性介质中研究了重均分子量为1,720,000 g / mol的聚(N-异丙基丙烯酰胺)(PNIPA)与人血清白蛋白(HSA),卵清蛋白(OVA)和溶菌酶(LYZ)的复合形成用NaCl调节至pH3。通过静态光散射(SLS)检查不同摩尔比(rm)的聚合物-蛋白质混合物。使用我们自己的方法对SLS数据进行分析[Kokufuta等,Langmuir 15(1999)940; Biomacromolecules 4(2003)728]显示,每种所得配合物的分子量均小于由两条聚合物链加一种蛋白质组成的互聚物配合物的分子量。这表明在所有研究的聚合物-蛋白质系统中均形成了聚合物内复合物。因此,在每个均方根下,我们计算每个聚合物结合蛋白的数量,其值依次为OVA> HSA> LYZ。将这些结果与每种蛋白的亲水性谱进行了比较,这是获得有关蛋白中疏水性和亲水性片段分布信息的良好工具。显而易见的是,聚合物和蛋白质之间的疏水相互作用在聚合物内复合物的形成中起重要作用。

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