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通过引入甘氨酸-脯氨酸序列实现溶菌酶的稳定化。

Stabilization of lysozyme by the introduction of Gly-Pro sequence.

作者信息

Ueda T, Tamura T, Maeda Y, Hashimoto Y, Miki T, Yamada H, Imoto T

机构信息

Faculty of Pharmaceutical Sciences of Kyushu University, Fukuoka, Japan.

出版信息

Protein Eng. 1993 Feb;6(2):183-7. doi: 10.1093/protein/6.2.183.

Abstract

Three mutant lysozymes where the Asp101-Gly102 sequence of lysozyme was converted to Asp101-Pro102, Gly101-Pro102 and Pro101-Gly102 were prepared to investigate the effect of proline residues on the stabilization of proteins. The free energy changes of lysozymes for the unfolding in aqueous solution at pH 5.5 and 35 degrees C were 10.0, 10.1, 11.0 and 7.7 kcal/mol for wild type, Asp101Pro102, Gly101Pro102 and Pro101Gly102 lysozyme respectively. When the energy level in the unfolded state of wild type lysozyme was fixed at a standard level, the energy levels in the folded state of Asp101Pro102 and Pro101Gly102 lysozymes were found to be higher than that of wild type lysozyme on the basis of delta GD(H2O) and entropy losses of their polypeptide chains in the unfolded state. The presence of some strain in the folded state of these lysozymes was supported by both the calculation of conformational energy for a trans-L-prolyl residue [Schimmel, P.R. and Flory, P.J. (1968) J. Mol. Biol., 34, 105-120] and the analysis of structures of energy-minimized mutant lysozymes. Therefore, it is concluded that the formation of the Gly-Pro sequence is effective in avoiding possible strain in the folded state of a protein caused by the introduction of proline residue(s).

摘要

制备了三种突变溶菌酶,其中溶菌酶的天冬氨酸101-甘氨酸102序列被转换为天冬氨酸101-脯氨酸102、甘氨酸101-脯氨酸102和脯氨酸101-甘氨酸102,以研究脯氨酸残基对蛋白质稳定性的影响。在pH 5.5和35℃的水溶液中,野生型、天冬氨酸101脯氨酸102、甘氨酸101脯氨酸102和脯氨酸101甘氨酸102溶菌酶展开的自由能变化分别为10.0、10.1、11.0和7.7千卡/摩尔。当野生型溶菌酶未折叠状态的能量水平固定在标准水平时,根据其未折叠状态下多肽链的ΔGD(H2O)和熵损失,发现天冬氨酸101脯氨酸102和脯氨酸101甘氨酸102溶菌酶折叠状态的能量水平高于野生型溶菌酶。这些溶菌酶折叠状态中存在一些应变,这一点得到了反式-L-脯氨酰残基构象能量计算[Schimmel, P.R.和Flory, P.J. (1968) J. Mol. Biol., 34, 105-120]以及能量最小化突变溶菌酶结构分析的支持。因此,可以得出结论,甘氨酸-脯氨酸序列的形成对于避免因引入脯氨酸残基而在蛋白质折叠状态中可能产生的应变是有效的。

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