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Secretion of Bacillus subtilis levansucrase. Fe(III) could act as a cofactor in an efficient coupling of the folding and translocation processes.

机译:枯草芽孢杆菌分泌的蔗糖酶。 Fe(III)可以在折叠和转运过程的有效耦合中充当辅助因子。

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摘要

The refolding of levansucrase denatured by urea was studied as a possible model for the second step of the secretion pathway of this protein. The folding-unfolding transition was monitored by measuring intrinsic fluorescence and resistance to proteolysis. Both methods provided the same estimation for the unfolding free energy of levansucrase, delta GD, which was 30.1 +/- 1.7 kJ.mol-1 (7.2 +/- 0.4 kcal.mol-1) at pH 7 in 0.1 M-potassium phosphate buffer. The rate of refolding was greatly enhanced by Fe3+, whereas the Fe3+ chelator EDTA prevented correct refolding. Fe3+ allowed the protein to reach its folded form in medium in which the dielectric constant had been lowered by ethanol. The efficiency in vivo of the export of levansucrase bearing an amino acid modification which blocks the second step of the translocation pathway was greatly increased by high concentrations of Fe3+ in the culture medium. Assuming that the protein folding governs the second step of the secretion process of levansucrase, we discuss from an irreversible thermodynamic point of view the possible role of Fe3+ in the efficient coupling of the two events.
机译:研究了尿素变性的左蔗糖酶的重折叠,作为该蛋白分泌途径第二步的可能模型。通过测量内在的荧光和对蛋白水解的抗性来监测折叠-展开转变。两种方法对左旋蔗糖酶的展开自由能提供了相同的估计值,δGD在0.1 M磷酸钾中于pH 7时为30.1 +/- 1.7 kJ.mol-1(7.2 +/- 0.4 kcal.mol-1)。缓冲。 Fe3 +大大提高了重折叠的速度,而Fe3 +螯合剂EDTA阻止了正确的重折叠。 Fe3 +使蛋白质在介电常数已被乙醇降低的介质中达到其折叠形式。培养基中高浓度的Fe3 +极大地提高了带有氨基酸修饰的甘露聚糖酶在体内的输出效率,该氨基酸修饰阻止了易位途径的第二步。假定蛋白质折叠决定了葡糖蔗糖酶分泌过程的第二步,我们从不可逆的热力学观点讨论了Fe3 +在两个事件的有效偶联中的可能作用。

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