首页> 外文OA文献 >Assessment of Toluene/Biphenyl Dioxygenase Gene Diversity in Benzene-Polluted Soils: Links between Benzene Biodegradation and Genes Similar to Those Encoding Isopropylbenzene Dioxygenases†
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Assessment of Toluene/Biphenyl Dioxygenase Gene Diversity in Benzene-Polluted Soils: Links between Benzene Biodegradation and Genes Similar to Those Encoding Isopropylbenzene Dioxygenases†

机译:苯污染土壤中甲苯/联苯双加氧酶基因多样性的评估:苯生物降解与类似于编码异丙基苯双加氧酶的基因之间的联系†

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摘要

The PCR-single-strand conformation polymorphism (SSCP) technique was used to assess the diversity and distribution of Rieske nonheme iron oxygenases of the toluene/biphenyl subfamily in soil DNA and bacterial isolates recovered from sites contaminated with benzene, toluene, ethylbenzene, and xylenes (BTEX). The central cores of genes encoding the catalytic α subunits were targeted, since they are responsible for the substrate specificities of these enzymes. SSCP functional genotype fingerprinting revealed a substantial diversity of oxygenase genes in three differently BTEX-contaminated soil samples, and sequence analysis indicated that in both the soil DNA and the bacterial isolates, genes for oxygenases related to the isopropylbenzene (cumene) dioxygenase branch of the toluene/biphenyl oxygenase subfamily were predominant among the detectable genotypes. The peptide sequences of the two most abundant α subunit sequence types differed by only five amino acids (residues 258, 286, 288, 289, and 321 according to numbering in cumene dioxygenase α subunit CumA1 of Pseudomonas fluorescens IP01). However, a strong correlation between sequence type and substrate utilization pattern was observed in isolates harboring these genes. Two of these residues were located at positions contributing, according to the resolved crystal structure of cumene dioxygenase from Pseudomonas fluorescens IP01, to the inner surface of the substrate-binding pocket. Isolates containing an α subunit with isoleucine and leucine at positions 288 and 321, respectively, were capable of degrading benzene and toluene, whereas isolates containing two methionine substitutions were found to be incapable of degrading toluene, indicating that the more bulky methionine residues significantly narrowed the available space within the substrate-binding pocket.
机译:PCR单链构象多态性(SSCP)技术用于评估土壤DNA和从受苯,甲苯,乙苯和二甲苯污染的地点回收的细菌分离株中甲苯/联苯亚家族的Rieske非血红素铁加氧酶的多样性和分布(BTEX)。编码催化性α亚基的基因的核心被靶向了,因为它们负责这些酶的底物特异性。 SSCP功能基因型指纹图谱显示,在三个受BTEX污染的不同土壤样品中,加氧酶基因的多样性很大,序列分析表明,在土壤DNA和细菌分离株中,与甲苯的异丙苯(枯烯)双加氧酶分支有关的加氧酶基因/联苯加氧酶亚科是可检测的基因型中占主导地位。两种最丰富的α亚基序列类型的肽序列仅相差五个氨基酸(根据荧光假单胞菌IP01中枯烯双加氧酶α亚基CumA1的编号,残基258、286、288、289和321)。然而,在带有这些基因的分离株中观察到序列类型和底物利用模式之间的强烈关联。根据来自荧光假单胞菌IP01的枯烯双加氧酶的解析的晶体结构,这些残基中的两个位于有助于底物结合袋的内表面的位置。分别在288和321位处含有一个带有异亮氨酸和亮氨酸的α亚基的分离物能够降解苯和甲苯,而发现含有两个蛋氨酸取代基的分离物则不能降解甲苯,这表明更大的蛋氨酸残基大大缩小了分离范围。底物装订袋内的可用空间。

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