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The binding of calcium to a salivary phosphoprotein, protein C, and comparison with calcium binding to protein A, a related salivary phosphoprotein

机译:钙与唾液磷蛋白,蛋白C的结合以及与钙与蛋白质A,相关唾液磷蛋白的结合的比较

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pThe binding of Ca2+ to a salivary phosphoprotein, protein C, was studied by equilibrium dialysis. In 5mM-Tris/HCl buffer, pH 7.5, protein C bound 190 nmol of Ca2+/mg of protein. The apparent dissociation constant, K, was determined to be 1.9 x 10(-4)M and the binding of Ca2+ to the protein was non-co-operative. The binding of Ca2+ to protein C apparently depends on groups which ionize above pH 5.0. Ca2+ binding decreased with increased concentration of the dialysis buffer and on addition of SrCL2, MgCl2 and MnCl2 to the dialysis buffer. Digestion of protein C with trypsin or collagenase or heating of the protein to 60 degrees or 100 degrees C had little or no effect on the Ca2+ binding. Digestion of protein C with alkaline phosphatase caused a decrease in the amount of protein-bound Ca2+. This was also found for another salivary phosphoprotein, protein A. In the absence of Ca2+ the S020,w for protein C was 1.29 S and in the presence of Ca2+ it was 1.46S. Ca2+ may cause a conformational change in the protein or an aggregation of the protein molecules. No conformational changes of protein C in the presence of Ca2+ could be detected by circular dichroism or nuclear magnetic resonance./p
机译:通过平衡透析研究了Ca2 +与唾液磷蛋白C的结合。在pH 7.5的5mM-Tris / HCl缓冲液中,蛋白质C结合了190 nmol的Ca2 + / mg蛋白质。确定的表观解离常数K为1.9 x 10(-4)M,Ca2 +与蛋白质的结合是非协同的。 Ca 2+与蛋白C的结合显然取决于在pH 5.0以上离子化的基团。随着透析缓冲液浓度的增加以及向透析缓冲液中添加SrCL2,MgCl2和MnCl2的作用,Ca2 +的结合力降低。用胰蛋白酶或胶原酶消化蛋白C或将蛋白加热到60度或100度对Ca2 +结合几乎没有影响。用碱性磷酸酶消化蛋白质C导致蛋白质结合的Ca2 +量减少。在另一个唾液磷蛋白,蛋白A中也发现了这一点。在不存在Ca2 +的情况下,蛋白C的S020,w为1.29 S,在存在Ca2 +的情况下为1.46S。 Ca2 +可能导致蛋白质构象变化或蛋白质分子聚集。圆二色性或核磁共振检测不到Ca 2+存在时蛋白C的构象变化。

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