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迈向蛋白质折叠问题的简化:在T4溶菌酶中设计的稳定聚丙氨酸α-螺旋。

Toward a simplification of the protein folding problem: a stabilizing polyalanine alpha-helix engineered in T4 lysozyme.

作者信息

Zhang X J, Baase W A, Matthews B W

机构信息

Institute of Molecular Biology, University of Oregon, Eugene 97403.

出版信息

Biochemistry. 1991 Feb 26;30(8):2012-7. doi: 10.1021/bi00222a001.

DOI:10.1021/bi00222a001
PMID:1998663
Abstract

In an attempt to simplify the protein folding problem, and also to further investigate the role of alanine as a helix-stabilizing residue, a series of alanines was introduced within the alpha-helix that includes residues 126-134 of T4 lysozyme. In wild-type lysozyme this alpha-helix contains alanine residues at positions 129, 130, and 134. Mutant lysozymes with alanines substituted at positions 128, 131, 132, and 133, either as single substitutions or in selected combinations, were constructed by oligonucleotide-directed mutagenesis. With the exception of the replacement of Leu 133, which is buried within the hydrophobic core of the protein, all the variants were more stable than wild-type lysozyme. The variant with alanines substituted at positions 128, 131, and 132 (E128A/V131A/N132A), which incorporates the sequence Ala 128-Ala 129-Ala 130-Ala 131-Ala 132-Leu 133-Ala 134, has a melting temperature 3.3 degrees C above that of wild-type lysozyme. Determination of the crystal structure of this mutant lysozyme shows that the replacement of Glu 128, Val 131, and Asn 132 with alanine causes alpha-helix 126-134 to rotate 3.4 degrees about an axis parallel to its own axis. This rotation seems to be triggered primarily by the loss of a hydrogen bond between Asn 132 and Ser 117 and is associated with the repacking of several side chains at the interface between alpha-helix 126-134 and the adjacent alpha-helix 115-122.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

为了简化蛋白质折叠问题,并进一步研究丙氨酸作为螺旋稳定残基的作用,在包含T4溶菌酶126 - 134位残基的α - 螺旋中引入了一系列丙氨酸。在野生型溶菌酶中,该α - 螺旋在129、130和134位含有丙氨酸残基。通过寡核苷酸定向诱变构建了在128、131、132和133位被丙氨酸取代的突变溶菌酶,这些取代可以是单个取代或选定的组合。除了取代位于蛋白质疏水核心内的Leu 133外,所有变体都比野生型溶菌酶更稳定。在128、131和132位被丙氨酸取代的变体(E128A/V131A/N132A),其序列为Ala 128 - Ala 129 - Ala 130 - Ala 131 - Ala 132 - Leu 133 - Ala 134,其解链温度比野生型溶菌酶高3.3摄氏度。对该突变溶菌酶晶体结构的测定表明,用丙氨酸取代Glu 128、Val 131和Asn 132会使α - 螺旋126 - 134绕与其自身轴平行的轴旋转3.4度。这种旋转似乎主要是由Asn 132和Ser 117之间氢键的丧失引发的,并且与α - 螺旋126 - 134和相邻α - 螺旋115 - 122之间界面处几个侧链的重新排列有关。(摘要截短于250字)

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