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Maintenance Role of a Glutathionyl-Hydroquinone Lyase (PcpF) in Pentachlorophenol Degradation by Sphingobium chlorophenolicum ATCC 39723
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ABSTRACT
Pentachlorophenol (PCP) is a toxic pollutant. Its biodegradation has been extensively studied in
Sphingobium chlorophenolicum
ATCC 39723. All enzymes required to convert PCP to a common metabolic intermediate before entering the tricarboxylic acid cycle have been characterized. One of the enzymes is tetrachloro-
p
-hydroquinone (TeCH) reductive dehalogenase (PcpC), which is a glutathione (GSH)
S
-transferase (GST). PcpC catalyzes the GSH-dependent conversion of TeCH to trichloro-
p
-hydroquinone (TriCH) and then to dichloro-
p
-hydroquinone (DiCH) in the PCP degradation pathway. PcpC is susceptible to oxidative damage, and the damaged PcpC produces glutathionyl (GS) conjugates, GS-TriCH and GS-DiCH, which cannot be further metabolized by PcpC. The fate and effect of GS-hydroquinone conjugates were unknown. A putative GST gene (
pcpF
) is located next to
pcpC
on the bacterial chromosome. The
pcpF
gene was cloned, and the recombinant PcpF was purified. The purified PcpF was able to convert GS-TriCH and GS-DiCH conjugates to TriCH and DiCH, respectively. The GS-hydroquinone lyase reactions catalyzed by PcpF are rather unusual for a GST. The disruption of
pcpF
in
S. chlorophenolicum
made the mutant lose the GS-hydroquinone lyase activities in the cell extracts. The mutant became more sensitive to PCP toxicity and had a significantly decreased PCP degradation rate, likely due to the accumulation of the GS-hydroquinone conjugates inside the cell. Thus, PcpF played a maintenance role in PCP degradation and converted the GS-hydroquinone conjugates back to the intermediates of the PCP degradation pathway.
American Society for Microbiology
Title: Maintenance Role of a Glutathionyl-Hydroquinone Lyase (PcpF) in Pentachlorophenol Degradation by
Sphingobium chlorophenolicum
ATCC 39723
Description:
ABSTRACT
Pentachlorophenol (PCP) is a toxic pollutant.
Its biodegradation has been extensively studied in
Sphingobium chlorophenolicum
ATCC 39723.
All enzymes required to convert PCP to a common metabolic intermediate before entering the tricarboxylic acid cycle have been characterized.
One of the enzymes is tetrachloro-
p
-hydroquinone (TeCH) reductive dehalogenase (PcpC), which is a glutathione (GSH)
S
-transferase (GST).
PcpC catalyzes the GSH-dependent conversion of TeCH to trichloro-
p
-hydroquinone (TriCH) and then to dichloro-
p
-hydroquinone (DiCH) in the PCP degradation pathway.
PcpC is susceptible to oxidative damage, and the damaged PcpC produces glutathionyl (GS) conjugates, GS-TriCH and GS-DiCH, which cannot be further metabolized by PcpC.
The fate and effect of GS-hydroquinone conjugates were unknown.
A putative GST gene (
pcpF
) is located next to
pcpC
on the bacterial chromosome.
The
pcpF
gene was cloned, and the recombinant PcpF was purified.
The purified PcpF was able to convert GS-TriCH and GS-DiCH conjugates to TriCH and DiCH, respectively.
The GS-hydroquinone lyase reactions catalyzed by PcpF are rather unusual for a GST.
The disruption of
pcpF
in
S.
chlorophenolicum
made the mutant lose the GS-hydroquinone lyase activities in the cell extracts.
The mutant became more sensitive to PCP toxicity and had a significantly decreased PCP degradation rate, likely due to the accumulation of the GS-hydroquinone conjugates inside the cell.
Thus, PcpF played a maintenance role in PCP degradation and converted the GS-hydroquinone conjugates back to the intermediates of the PCP degradation pathway.
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