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通过甲苯2,3-双加氧酶降解甲苯的细菌的活性依赖型荧光标记。

Activity-dependent fluorescent labeling of bacteria that degrade toluene via toluene 2,3-dioxygenase.

作者信息

Keener W K, Watwood M E, Apel W A

机构信息

Idaho National Engineering and Environmental Laboratory, Idaho Falls 83415, USA.

出版信息

Appl Microbiol Biotechnol. 1998 Apr;49(4):455-62. doi: 10.1007/s002530051198.

DOI:10.1007/s002530051198
PMID:9615486
Abstract

Alternative substrates for the toluene 2,3-dioxygenase pathway of several pseudomonads served as enzyme-activity-dependent fluorescent probes for the bacteria. Phenylacetylene and cinnamonitrile were transformed to fluorescent and brightly colored products by Pseudomonas putida F1, Pseudomonas fluorescens CFS215, and Burkholderia (Pseudomonas) strain JS150. Active bacteria transformed phenylacetylene, producing bright yellow solutions containing the putative product 2-hydroxy-6-oxo-7-octyn-2,4-dienoate. Transformation of cinnamonitrile resulted in bright orange solutions due to accumulation of the putative product 2-hydroxy-6-oxo-8-cyanoocta-2,4,7-trienoate. Chemical and physical properties of the products supported their identification, which indicated that the first three enzymes of the pathway catalyzed product formation. Phenylacetylene labeled bacteria with green fluorescence emission; bacteria were concentrated on black 0.2-micron-pore-size polycarbonate filters containing polyvinylpyrrolidone (PVP) as a wetting agent. Bacteria labeled with cinnamonitrile were fluorescent orange; labeling was effective with bacteria trapped on PVP-free polycarbonate filters. Production of the enzymes involved in labeling of P. putida F1 and P. fluorescens CFS215 was induced by growth (on arginine) in the presence of toluene; cells grown on arginine without toluene were not labeled. Labeling of P. putida F1 by phenylacetylene was inhibited by toluene, indicating that the same enzymatic pathway was required for transformations of both substrates. Bacteria expressing other toluene-degrading enzymatic pathways were not fluorescently labeled with phenylacetylene.

摘要

几种假单胞菌甲苯2,3-双加氧酶途径的替代底物可作为这些细菌的酶活性依赖性荧光探针。恶臭假单胞菌F1、荧光假单胞菌CFS215和伯克霍尔德菌(假单胞菌)菌株JS150将苯乙炔和肉桂腈转化为荧光且颜色鲜艳的产物。活性细菌将苯乙炔转化,产生含有推定产物2-羟基-6-氧代-7-辛炔-2,4-二烯酸酯的亮黄色溶液。肉桂腈的转化导致溶液呈亮橙色,这是由于推定产物2-羟基-6-氧代-8-氰基辛-2,4,7-三烯酸酯的积累。产物的化学和物理性质支持了它们的鉴定,这表明该途径的前三种酶催化了产物的形成。苯乙炔标记的细菌发出绿色荧光;细菌被浓缩在含有作为湿润剂的聚乙烯吡咯烷酮(PVP)的黑色0.2微米孔径聚碳酸酯滤膜上。用肉桂腈标记的细菌呈荧光橙色;对于捕获在不含PVP的聚碳酸酯滤膜上的细菌,标记效果良好。恶臭假单胞菌F1和荧光假单胞菌CFS215标记过程中所涉及的酶的产生是由在甲苯存在下(以精氨酸为培养基)生长诱导的;在不含甲苯的精氨酸培养基上生长的细胞未被标记。甲苯抑制了苯乙炔对恶臭假单胞菌F1的标记,这表明两种底物的转化需要相同的酶促途径。表达其他甲苯降解酶途径的细菌未被苯乙炔荧光标记。

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