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来自日本慢生根瘤菌的双功能PutA同源物的表征以及调节黄素腺嘌呤二核苷酸辅因子脯氨酸还原的活性位点残基的鉴定。

Characterization of a bifunctional PutA homologue from Bradyrhizobium japonicum and identification of an active site residue that modulates proline reduction of the flavin adenine dinucleotide cofactor.

作者信息

Krishnan Navasona, Becker Donald F

机构信息

Department of Biochemistry, Redox Biology Center, University of Nebraska, Lincoln, Nebraska 68588, USA.

出版信息

Biochemistry. 2005 Jun 28;44(25):9130-9. doi: 10.1021/bi050629k.

Abstract

PutA is a bifunctional flavoenzyme in bacteria that catalyzes the four-electron oxidation of proline to glutamate. In certain prokaryotes such as Escherichia coli, PutA is also a transcriptional repressor of the proline utilization (put) genes and thus is trifunctional. In this work, we have begun to assess differences between bifunctional and trifunctional PutA enzymes by examining the PutA protein from Bradyrhizobium japonicum (BjPutA). Primary structure analysis of BjPutA shows it lacks the DNA-binding domain of E. coli PutA (EcPutA). Consistent with this prediction, purified BjPutA does not exhibit DNA-binding activity in native gel mobility shift assays with promoter regions of the putA gene from B. japonicum. The catalytic and redox properties of BjPutA were characterized and a reduction potential (E(m)) value of -0.132 V (pH 7.5) was determined for the bound FAD/FADH(2) couple in BjPutA that is significantly more negative ( approximately 55 mV) than the E(m) for EcPutA-bound FAD. The more negative E(m) value thermodynamically limits proline reduction of the FAD cofactor in BjPutA. In the presence of phospholipids, reduction of BjPutA is stimulated, suggesting lipids influence the FAD redox environment. Accordingly, an E(m) value of -0.114 V (pH 7.5) was determined for BjPutA-bound FAD in the presence of polar lipids. The molecular basis for the lower reduction potential of FAD in BjPutA relative to EcPutA was explored by site-directed mutagenesis. Amino acid sequence alignment between BjPutA and EcPutA indicates only one difference in active site residues near the isoalloxazine ring of FAD: Val402 in EcPutA is substituted at the analogous position in BjPutA with Ala310. Replacement of A310 by Val in the BjPutA mutant A310V raised the reduction potential of bound FAD relative to wild-type BjPutA to an E(m) value of -0.09 V (pH 7.5). The >40-mV positive shift in the potential of the BjPutA mutant A310V suggests that the corresponding Val residue in EcPutA helps poise the FAD redox potential for thermodynamically favored proline reduction thereby allowing EcPutA to be efficiently regulated by proline availability. Limited proteolysis of BjPutA under reducing conditions shows FAD reduction does not influence BjPutA conformation indicating further that the redox dependent regulation observed with EcPutA may be limited to trifunctional PutA homologues.

摘要

PutA是细菌中的一种双功能黄素酶,可催化脯氨酸四电子氧化生成谷氨酸。在某些原核生物如大肠杆菌中,PutA还是脯氨酸利用(put)基因的转录阻遏物,因此具有三功能。在这项研究中,我们通过研究日本慢生根瘤菌(BjPutA)的PutA蛋白,开始评估双功能和三功能PutA酶之间的差异。BjPutA的一级结构分析表明,它缺乏大肠杆菌PutA(EcPutA)的DNA结合结构域。与该预测一致,在使用来自日本慢生根瘤菌的putA基因启动子区域进行的天然凝胶迁移率变动分析中,纯化的BjPutA未表现出DNA结合活性。对BjPutA的催化和氧化还原特性进行了表征,并确定了BjPutA中结合的FAD/FADH₂ 对的还原电位(E(m))值为-0.132 V(pH 7.5),该值比EcPutA结合的FAD的E(m)值明显更负(约55 mV)。更负的E(m)值在热力学上限制了BjPutA中FAD辅因子的脯氨酸还原。在磷脂存在下,BjPutA的还原受到刺激,表明脂质影响FAD氧化还原环境。因此,在极性脂质存在下,确定BjPutA结合的FAD的E(m)值为-0.114 V(pH 7.5)。通过定点诱变探索了BjPutA中FAD还原电位低于EcPutA的分子基础。BjPutA和EcPutA之间的氨基酸序列比对表明,在FAD异咯嗪环附近的活性位点残基中只有一个差异:EcPutA中的Val402在BjPutA的类似位置被Ala310取代。在BjPutA突变体A310V中将A310替换为Val,使结合的FAD的还原电位相对于野生型BjPutA提高到E(m)值-0.09 V(pH 7.5)。BjPutA突变体A310V的电位正向偏移>40 mV,表明EcPutA中相应的Val残基有助于平衡FAD氧化还原电位,以利于热力学上有利的脯氨酸还原,从而使EcPutA能够被脯氨酸可用性有效调节。在还原条件下对BjPutA进行有限的蛋白酶解表明,FAD还原不影响BjPutA的构象,这进一步表明在EcPutA中观察到的氧化还原依赖性调节可能仅限于三功能PutA同源物。

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