首页> 外文期刊>Journal of Molecular Biology >INFORMATIONAL SUPPRESSION TO INVESTIGATE STRUCTURAL FUNCTIONAL AND EVOLUTIONARY ASPECTS OF THE ERWINIA CHRYSANTHEMI CELLULASE EGZ
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INFORMATIONAL SUPPRESSION TO INVESTIGATE STRUCTURAL FUNCTIONAL AND EVOLUTIONARY ASPECTS OF THE ERWINIA CHRYSANTHEMI CELLULASE EGZ

机译:信息抑制以研究ERWINIA CHRYSANTHEMI纤维素酶EGZ的结构功能和进化方面

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The cellulase EGZ produced by the plant pathogen Erwinia chrysanthemi belongs to family 5 of the beta-glycohydrolases (also referred to as cellulase family A), which contains over 40 members from Gram-negative and Gram-positive bacteria and fungi. Amber mutations were introduced into 16 codons of the celZ gene encoding EGZ. Targeted residues included: (1) two Glu, two His and one Arg residue, strictly conserved throughout family 5; (2) one Arg and one His residue conserved in sub-family 5-2; and (3) one His and six Arg residues not conserved at all. Each amber allele was introduced into 13 Escherichia coli strains each carrying a different suppresser tRNA that inserts an amino acid at the mutated position. In vivo stability of the mutated forms of EGZ and their cellulase activity were analysed as well as suppression efficiency For some positions of particular interest, missense mutations were introduced into the celZ gene either to confirm the effect of the suppressor-mediated amino acid substitution or to broaden the spectrum of mutations available. The substitution patterns of the two Glu positions were interpretable in the light of the stereospecificity of the reaction catalysed by EGZ: Glu133 and Glu220 are proposed to act as a proton donor and as a nucleophile, respectively, forming the glycosyl-enzyme intermediate. Substitution at His-occupied positions, including two non-conserved positions, yielded proteins affected in their catalytic activity but not their in vivo stability; In particular, evidence was obtained for His at position 98 to be involved in interactions with the substrate. The view that Arg residues are important in stabilizing proteins was supported by the identification of three Arg residues, whose substitution yielded thermosensitive forms of EGZ. In addition, Pro substitutions of any of the six Arg residues altered protein stability in vivo but the substitutions scored almost neutral for activity. Five positions, predicted to be within alpha-helices, were found to be susceptible to Pro substitutions (but not to Ala) with respect to stability in vivo. Overall, the systematic alteration of all His and Arg residues coupled with the simultaneous analysis of activity and in vivo stability allowed us to demonstrate that substitution matrices vary at each position and for each biological property considered. Ideally, therefore, substitution matrices used in sequence alignment procedures should be reconsidered as position-specific and as property-specific. Allowed amino acid substitutions at conserved and non-conserved positions were compared. with natural variability occurring in the set of 40 cellulases present in family 5, thereby providing us with a direct comparison between laboratory-induced and naturally occurring evolution and between experimentally and theoretically based substitution matrices. [References: 57]
机译:植物病原体菊花欧文氏菌产生的纤维素酶EGZ属于β-糖水解酶家族5(也称为纤维素酶家族A),其中包含40多个革兰氏阴性和革兰氏阳性细菌和真菌成员。将琥珀色突变引入编码EGZ的celZ基因的16个密码子中。目标残基包括:(1)在整个家族5中严格保守的两个Glu,两个His和一个Arg残基; (2)在亚族5-2中保守的一个Arg和一个His残基; (3)一个根本不保守的His残基和六个Arg残基。将每个琥珀色等位基因引入13个大肠杆菌菌株中,每个菌株均带有在突变位置插入氨基酸的不同抑制子tRNA。分析了EGZ突变形式的体内稳定性及其纤维素酶活性以及抑制效率。对于某些特别感兴趣的位置,将错义突变引入celZ基因中,以确认抑制子介导的氨基酸取代的作用或拓宽可用突变的范围。根据EGZ催化的反应的立体特异性,可以解释两个Glu位置的取代方式:提议Glu133和Glu220分别充当质子供体和亲核试剂,形成糖基酶中间体。在His占据的位置(包括两个非保守位置)进行取代,所产生的蛋白质的催化活性受到影响,但体内稳定性不受影响;特别地,获得了关于98位的His参与与底物相互作用的证据。鉴定三个残基的观点支持了Arg残基在稳定蛋白质中很重要的观点,这三个Arg残基的取代产生了热敏形式的EGZ。此外,六个Arg残基中任何一个的Pro取代都改变了体内蛋白质的稳定性,但该取代的活性几乎为中性。就体内稳定性而言,发现五个位置预计在α-螺旋内,易于被Pro取代(但对Ala不敏感)。总的来说,所有His和Arg残基的系统性改变,以及对活性和体内稳定性的同时分析,使我们能够证明取代矩阵在每个位置和所考虑的每个生物学特性上都不同。因此,理想情况下,应该将序列比对程序中使用的取代矩阵重新考虑为位置特异性和属性特异性。比较了在保守和非保守位置上允许的氨基酸取代。家族5中存在的40个纤维素酶存在自然可变性,从而为我们提供了实验室诱导的进化与自然发生的进化以及基于实验和理论的替代矩阵之间的直接比较。 [参考:57]

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