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通过丙氨酸替换为α-氨基异丁酸提高蛋白质热稳定性。

Enhanced protein thermostability by Ala-->Aib replacement.

作者信息

De Filippis V, De Antoni F, Frigo M, Polverino de Laureto P, Fontana A

机构信息

CRIBI Biotechnology Centre, University of Padua, Italy.

出版信息

Biochemistry. 1998 Feb 10;37(6):1686-96. doi: 10.1021/bi971937o.

DOI:10.1021/bi971937o
PMID:9484240
Abstract

The introduction into peptide chains of alpha-aminoisobutyric acid (Aib) has proven to stabilize the helical structure in short peptides by restricting the available range of polypeptide backbone conformations. In order to evaluate the potential stabilizing effect of Aib at the protein level, we have studied the conformational and stability properties of Aib-containing analogs of the carboxy-terminal subdomain 255-316 of thermolysin. Previous NMR studies have shown that this disulfide-free 62-residue fragment forms a dimer in solution and that the global 3D structure of each monomer (3 alpha-helices encompassing residues 260-274, 281-295, and 301-311) is largely coincident with that of the corresponding region in the X-ray structure of intact thermolysin. The Aib analogs of fragment 255-316 were prepared by a semisynthetic approach in which the natural fragment 255-316 was coupled to synthetic analogs of peptide 303-316 using V8-protease in 50% (v/v) aqueous glycerol [De Filippis, V., and Fontana, A. (1990) Int. J. Pept. Protein Res. 35, 219-227]. The Ala residue in position 304, 309, or 312 of fragment 255-316 was replaced by Aib, leading to the singly substituted fragments Ala304Aib, Ala309Aib, and Ala312Aib. Moreover, fragment Ala304Aib/Ala309Aib with a double Ala-->Aib exchange in positions 304 and 309 was produced. Far- and near-UV circular dichroism measurements demonstrated that both secondary and tertiary structures of the natural fragment 255-316 are fully retained upon Ala-->Aib substitution(s). Thermal unfolding measurements, carried out by recording the ellipticity at 222 nm upon heating, showed that the melting temperatures (Tm) of analogs Ala304Aib and Ala309Aib were 2.2 and 5.4 degrees C higher than that of the Ala-containing natural species (Tm = 63.5 degrees C), respectively, whereas the Tm of the Ala312Aib analog was lowered by -0.6 degree C. The enhanced stability of the Ala304Aib analog can be quantitatively explained on the basis of a reduced backbone entropy of unfolding due to the restriction of the conformational space allowed to Aib in respect to Ala, while the larger stabilization observed for the Ala309Aib analog can be accounted for by both entropic and hydrophobic effects. In fact, whereas Ala304 is a surface residue, Ala309 is shielded from the solvent, and thus the enhanced stability of fragment Ala309Aib is also due to the burial of an additional -CH3 group with respect to the natural fragment. The slightly destabilizing effect of the Ala-->Aib exchange in position 312 appears to derive from unfavorable strain energy effects, since phi and psi values for Ala312 are out of the allowed angles for Aib. Of interest, the simultaneous incorporation of Aib at positions 304 and 309 leads to a significant and additive increase of +8 degrees C in Tm. The results of this study indicate that the rational incorporation of Aib into a polypeptide chain can be a general procedure to significantly stabilize proteins.

摘要

已证实,将α-氨基异丁酸(Aib)引入肽链可通过限制多肽主链构象的可用范围来稳定短肽中的螺旋结构。为了评估Aib在蛋白质水平上的潜在稳定作用,我们研究了嗜热菌蛋白酶羧基末端亚结构域255 - 316含Aib类似物的构象和稳定性特性。先前的核磁共振研究表明,这个不含二硫键的62个残基片段在溶液中形成二聚体,并且每个单体的整体三维结构(包含残基260 - 274、281 - 295和301 - 311的3个α-螺旋)与完整嗜热菌蛋白酶X射线结构中相应区域的结构基本一致。片段255 - 316的Aib类似物通过半合成方法制备,其中天然片段255 - 316在50%(v/v)甘油水溶液中使用V8蛋白酶与肽303 - 316的合成类似物偶联[De Filippis, V., and Fontana, A. (1990) Int. J. Pept. Protein Res. 35, 219 - 227]。片段255 - 316中位置304、309或312的丙氨酸残基被Aib取代,得到单取代片段Ala304Aib、Ala309Aib和Ala312Aib。此外,还制备了在位置304和309具有双重丙氨酸→Aib交换的片段Ala304Aib/Ala309Aib。远紫外和近紫外圆二色性测量表明,天然片段255 - 316的二级和三级结构在丙氨酸→Aib取代后完全保留。通过记录加热时222 nm处的椭圆率进行的热变性测量表明,类似物Ala304Aib和Ala309Aib的解链温度(Tm)分别比含丙氨酸的天然物种(Tm = 63.5℃)高2.2℃和5.4℃,而Ala312Aib类似物的Tm降低了0.6℃。Ala304Aib类似物稳定性的增强可以基于相对于丙氨酸,Aib的构象空间受限导致解链时主链熵降低来定量解释,而Ala309Aib类似物观察到的更大稳定性可以由熵效应和疏水效应共同解释。实际上,虽然Ala304是表面残基,但Ala309被溶剂屏蔽,因此片段Ala309Aib稳定性的增强也归因于相对于天然片段额外埋藏了一个-CH3基团。位置312处丙氨酸→Aib交换的轻微去稳定作用似乎源于不利的应变能效应,因为Ala312的φ和ψ值超出了Aib允许的角度范围。有趣的是,在位置304和309同时引入Aib导致Tm显著增加8℃且具有加和性。这项研究的结果表明,将Aib合理引入多肽链可以是一种显著稳定蛋白质的通用方法。

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