Karandikar Rohini, Badri Abinaya, Phale Prashant S
Department of Biosciences and Bioengineering, Indian Institute of Technology- Bombay, Powai, Mumbai, 400076, India.
Appl Biochem Biotechnol. 2015 Sep;177(2):318-33. doi: 10.1007/s12010-015-1744-6. Epub 2015 Jul 23.
The first step involved in the degradation of phthalate isomers (phthalate, isophthalate and terephthalate) is the double hydroxylation by respective aromatic-ring hydroxylating dioxygenases. These are two component enzymes consisting of 'oxygenase' and 'reductase' components. Soil isolate Pseudomonas aeruginosa strain PP4 degrades phthalate isomers via protocatechuate and benzoate via catechol 'ortho' ring cleavage pathway. Metabolic studies suggest that strain PP4 has carbon source-specific inducible phthalate isomer dioxygenase and benzoate dioxygenase. Thus, it was of interest to study the properties of reductase components of these enzymes. Reductase activity from phthalate isomer-grown cells was 3-5-folds higher than benzoate grown cells. In-gel activity staining profile showed a reductase activity band of R f 0.56 for phthalate isomer-grown cells as compared to R f 0.73 from benzoate-grown cells. Partially purified reductase components from phthalate isomer grown cells showed K m in the range of 30-40 μM and V max = 34-48 μmol min(-1) mg(-1). However, reductase from benzoate grown cells showed K m = 49 μM and V max = 10 μmol min(-1) mg(-1). Strikingly similar molecular and kinetic properties of reductase component from phthalate isomer-grown cells suggest that probably the same reductase component is employed in three phthalate isomer dioxygenases. However, reductase component is different, with respect to kinetic properties and zymogram analysis, from benzoate-grown cells when compared to that from phthalate isomer grown cells of PP4.
邻苯二甲酸酯异构体(邻苯二甲酸酯、间苯二甲酸酯和对苯二甲酸酯)降解过程的第一步是由各自的芳香环羟化双加氧酶进行双羟基化。这些是由“加氧酶”和“还原酶”组分组成的双组分酶。土壤分离株铜绿假单胞菌PP4菌株通过原儿茶酸降解邻苯二甲酸酯异构体,并通过儿茶酚“邻位”环裂解途径降解苯甲酸。代谢研究表明,PP4菌株具有碳源特异性诱导型邻苯二甲酸酯异构体双加氧酶和苯甲酸双加氧酶。因此,研究这些酶的还原酶组分的特性很有意义。邻苯二甲酸酯异构体生长细胞的还原酶活性比苯甲酸生长细胞高3至5倍。凝胶内活性染色图谱显示,邻苯二甲酸酯异构体生长细胞的还原酶活性带Rf为0.56,而苯甲酸生长细胞的Rf为0.73。从邻苯二甲酸酯异构体生长细胞中部分纯化的还原酶组分的Km在30 - 40μM范围内,Vmax = 34 - 48μmol min(-1) mg(-1)。然而,苯甲酸生长细胞的还原酶Km = 49μM,Vmax = 10μmol min(-1) mg(-1)。邻苯二甲酸酯异构体生长细胞的还原酶组分在分子和动力学特性上惊人地相似,这表明三种邻苯二甲酸酯异构体双加氧酶可能使用相同的还原酶组分。然而,与PP4菌株邻苯二甲酸酯异构体生长细胞相比,苯甲酸生长细胞的还原酶组分在动力学特性和酶谱分析方面有所不同。