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醋酸钙不动杆菌NCIB8250中苯酚降解调节因子MopR的表达、诱导物谱、结构域结构及功能

Expression, inducer spectrum, domain structure, and function of MopR, the regulator of phenol degradation in Acinetobacter calcoaceticus NCIB8250.

作者信息

Schirmer F, Ehrt S, Hillen W

机构信息

Lehrstuhl für Mikrobiologie, Institut für Mikrobiologie, Biochemie und Genetik der Friedrich-Alexander Universität Erlangen-Nürnberg, Erlangen, Germany.

出版信息

J Bacteriol. 1997 Feb;179(4):1329-36. doi: 10.1128/jb.179.4.1329-1336.1997.

Abstract

Degradation of phenol by Acinetobacter calcoaceticus NCIB8250 involves (sigma54-dependent expression of a multicomponent phenol hydroxylase and catechol 1,2-dioxygenase encoded by the mop operon. Complementation of a new mutant deficient in phenol utilization yielded the regulatory locus mopR. It is located in divergent orientation next to the mop operon. MopR is constitutively expressed at a low level from a sigma70-type promoter and belongs to the NtrC family of regulators. The amino acid sequence is similar to that of XylR regulating xylene degradation and to that of DmpR regulating dimethylphenol degradation in Pseudomonas spp. However, it shows a different effector profile for substituted phenols than DmpR. MopR activates phenol hydroxylase expression in the presence of phenol in Escherichia coli, indicating that it binds the effector. The phenol binding A domains of MopR and DmpR have fewer identical residues than the A domains of DmpR and XylR, despite the fact that XylR recognizes different effectors. This suggests that sequence conservation in the A domain does not reflect the potential to bind the respective effectors. Overexpression of the MopR A domain in the presence of wild-type MopR causes loss of mop inducibility by phenol, establishing its negative transdominance over MopR. Deletion of 110 residues from the N terminus did not affect transdominance of the truncated domain, whereas deletion of 150 residues abolished it completely. This result establishes the distinction of two subdomains, A(N) and A(C), which together constitute the A domain. The C-terminal portion of the A domain, A(C), shows considerable affinity for the C domain, even in the presence of the trigger phenol.

摘要

乙酸钙不动杆菌NCIB8250对苯酚的降解涉及由mop操纵子编码的多组分苯酚羟化酶和儿茶酚1,2-双加氧酶的σ54依赖性表达。对一个新的苯酚利用缺陷型突变体进行互补分析得到了调控基因座mopR。它位于mop操纵子旁边,转录方向相反。MopR由一个σ70型启动子组成型低水平表达,属于NtrC家族调控因子。其氨基酸序列与调节二甲苯降解的XylR以及假单胞菌属中调节二甲基苯酚降解的DmpR相似。然而,与DmpR相比,它对取代苯酚表现出不同的效应物谱。MopR在苯酚存在的情况下能激活大肠杆菌中苯酚羟化酶的表达,表明它能结合效应物。尽管XylR识别不同的效应物,但MopR和DmpR的苯酚结合A结构域中相同的残基比DmpR和XylR的A结构域更少。这表明A结构域中的序列保守性并不反映结合相应效应物的潜力。在野生型MopR存在的情况下过表达MopR的A结构域会导致苯酚对mop的诱导性丧失,确立了其对MopR的负显性作用。从N端缺失110个残基并不影响截短结构域的显性作用,而缺失150个残基则完全消除了这种作用。这一结果确定了两个亚结构域A(N)和A(C)的区别,它们共同构成了A结构域。即使在存在触发苯酚的情况下,A结构域的C端部分A(C)对C结构域也表现出相当高的亲和力。

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Phenol degradation by Acinetobacter calcoaceticus NCIB 8250.
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