The catechol 1,2 dioxygenase system of Acinetobacter radioresistens: isoenzymes, inductors and gene localization

Two different isozymes (Iso A and Iso B) of catechol 1,2 dioxygenase (C1,2O) were isolated from cultures of A. radioresistens grown in two different media, containing phenol and benzoate respectively. In the phenol medium the bacteria expressed about 90% of Iso A, whereas in the benzoate medium the Iso A/Iso B ratio was 40:60. The two proteins have different molecular masses, isoelectric points and N-terminal sequences that are not consistent with simple post-translational modifications. Furthermore, their behaviour differs at high temperatures (42 degrees C-47 degrees C) and at moderately acidic pH (pH 6.0): Iso A proved to be the more stable under conditions of environmental stress. Hybridisation analysis with an A. calcoaceticus catA-derived probe revealed that A. radioresistens C1,2O proteins are encoded by two chromosomally located genes. Bidimensional electrophoresis (2DE) maps of crude extracts of cells grown in different carbon sources (phenol, benzoate and acetate) clearly demonstrated a differential induction pattern for the two proteins. The hypothesis of a double set of genes, one for benzoate catabolism and the other for phenol catabolism, is discussed, and analogies are drawn with other known C1,2Os.

Titolo: The catechol 1,2 dioxygenase system of Acinetobacter radioresistens: isoenzymes, inductors and gene localization
Autori Riconosciuti: 
PESSIONE, Enrica  
MAZZOLI, Roberto  
CAPOSIO, Patrizia  
LANDOLFO, Santo Giuseppe  
GIUNTA, Carlo  
GRIBAUDO, Giorgio  
mostra contributor esterni 
Autori: E. PESSIONE; GIUFFRIDA M.G.; MAZZOLI R.; CAPOSIO P.; LANDOLFO S.; CONTI A.; GIUNTA C.; GRIBAUDO G.
Data di pubblicazione: 2001
Abstract: Two different isozymes (Iso A and Iso B) of catechol 1,2 dioxygenase (C1,2O) were isolated from cultures of A. radioresistens grown in two different media, containing phenol and benzoate respectively. In the phenol medium the bacteria expressed about 90% of Iso A, whereas in the benzoate medium the Iso A/Iso B ratio was 40:60. The two proteins have different molecular masses, isoelectric points and N-terminal sequences that are not consistent with simple post-translational modifications. Furthermore, their behaviour differs at high temperatures (42 degrees C-47 degrees C) and at moderately acidic pH (pH 6.0): Iso A proved to be the more stable under conditions of environmental stress. Hybridisation analysis with an A. calcoaceticus catA-derived probe revealed that A. radioresistens C1,2O proteins are encoded by two chromosomally located genes. Bidimensional electrophoresis (2DE) maps of crude extracts of cells grown in different carbon sources (phenol, benzoate and acetate) clearly demonstrated a differential induction pattern for the two proteins. The hypothesis of a double set of genes, one for benzoate catabolism and the other for phenol catabolism, is discussed, and analogies are drawn with other known C1,2Os.
Volume: 382
Pagina iniziale: 1253
Pagina finale: 1261
Rivista: BIOLOGICAL CHEMISTRY
Appare nelle tipologie:03A-Articolo su Rivista

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http://hdl.handle.net/2318/1853
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