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首页> 美国卫生研究院文献>Journal of Bacteriology >Protein Engineering of the Archetypal Nitroarene Dioxygenase of Ralstonia sp. Strain U2 for Activity on Aminonitrotoluenes and Dinitrotoluenes through Alpha-Subunit Residues Leucine 225 Phenylalanine 350 and Glycine 407
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Protein Engineering of the Archetypal Nitroarene Dioxygenase of Ralstonia sp. Strain U2 for Activity on Aminonitrotoluenes and Dinitrotoluenes through Alpha-Subunit Residues Leucine 225 Phenylalanine 350 and Glycine 407

机译:Ralstonia sp。的原型硝基亚硝基双加氧酶的蛋白质工程。 U2菌株通过α亚基残基亮氨酸225苯丙氨酸350和甘氨酸407对氨基硝基甲苯和二硝基甲苯的活性

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Naphthalene dioxygenase (NDO) from Ralstonia sp. strain U2 has not been reported to oxidize nitroaromatic compounds. Here, saturation mutagenesis of NDO at position F350 of the α-subunit (NagAc) created variant F350T that produced 3-methyl-4-nitrocatechol from 2,6-dinitrotoluene (26DNT), that released nitrite from 23DNT sixfold faster than wild-type NDO, and that produced 3-amino-4-methyl-5-nitrocatechol and 2-amino-4,6-dinitrobenzyl alcohol from 2-amino-4,6-dinitrotoluene (2A46DNT) (wild-type NDO has no detectable activity on 26DNT and 2A46DNT). DNA shuffling identified the beneficial NagAc mutation G407S, which when combined with the F350T substitution, increased the rate of NDO oxidation of 26DNT, 23DNT, and 2A46DNT threefold relative to variant F350T. DNA shuffling of NDO nagAcAd also generated the NagAc variant G50S/L225R/A269T with an increased rate of 4-amino-2-nitrotoluene (4A2NT; reduction product of 2,4-dinitrotoluene) oxidation; from 4A2NT, this variant produced both the previously uncharacterized oxidation product 4-amino-2-nitrocresol (enhanced 11-fold relative to wild-type NDO) as well as 4-amino-2-nitrobenzyl alcohol (4A2NBA; wild-type NDO does not generate this product). G50S/L225R/A269T also had increased nitrite release from 23DNT (14-fold relative to wild-type NDO) and generated 2,3-dinitrobenzyl alcohol (23DNBA) fourfold relative to wild-type NDO. The importance of position L225 for catalysis was confirmed through saturation mutagenesis; relative to wild-type NDO, NDO variant L225R had 12-fold faster generation of 4-amino-2-nitrocresol and production of 4A2NBA from 4A2NT as well as 24-fold faster generation of nitrite and 15-fold faster generation of 23DNBA from 23DNT. Hence, random mutagenesis discovered two new residues, G407 and L225, that influence the regiospecificity of Rieske non-heme-iron dioxygenases.
机译:来自Ralstonia sp。的萘双加氧酶(NDO)。尚未报道菌株U2会氧化硝基芳族化合物。在这里,NDO在α亚基(NagAc)F350位置的饱和诱变产生了变体F350T,该变体从2,6-二硝基甲苯(26DNT)产生3-甲基-4-硝基邻苯二酚,从23DNT释放亚硝酸盐的速度比野生型快六倍NDO,以及由2-氨基-4,6-二硝基甲苯(2A46DNT)生成3-氨基-4-甲基-5-硝基邻苯二酚和2-氨基-4,6-二硝基苄醇的化合物(野生型NDO在26DNT和2A46DNT)。 DNA改组确定了有益的NagAc突变G407S,当与F350T替代物结合使用时,其26DNT,23DNT和2A46DNT的NDO氧化速率相对于变体F350T增加了三倍。 NDO nagAcAd的DNA改组还生成了NagAc变体G50S / L225R / A269T,其4-氨基-2-硝基甲苯(4A2NT; 2,4-二硝基甲苯的还原产物)的氧化速率增加;由4A2NT产生,此变体既产生了以前未表征的氧化产物4-氨基-2-硝基甲酚(相对于野生型NDO增强了11倍),也产生了4-氨基-2-硝基苄醇(4A2NBA;野生型NDO产生了无法生成此产品)。 G50S / L225R / A269T的亚硝酸盐从23DNT的释放也有所增加(相对于野生型NDO是14倍),并且生成的2,3-二硝基苄醇(23DNBA)是野生型NDO的四倍。通过饱和诱变证实了位置L225对于催化的重要性;相对于野生型NDO,NDO变体L225R产生4-氨基-2-硝基甲酚的速度快12倍,从4A2NT产生4A2NBA的速度更快,亚硝酸盐的产生速度快24倍,从23DNT的23DNBA产生速度快15倍。因此,随机诱变发现了两个新的残基,G407和L225,它们影响Rieske非血红素铁双加氧酶的区域特异性。

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