Biochemical and biophysical characterisation of haloalkane dehalogenases DmrA and DmrB in M ycobacterium strain JS 60 and their role in growth on haloalkanes
Haloalkane dehalogenases ( HLDs ) catalyse the hydrolysis of haloalkanes to alcohols, offering a biological solution for toxic haloalkane industrial wastes. Hundreds of putative HLD genes have been identified in bacterial genomes, but relatively few enzymes have been characterised. We identified two...
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Veröffentlicht in: | Molecular microbiology 2015-08, Vol.97 (3), p.439-453 |
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Format: | Artikel |
Sprache: | eng |
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Zusammenfassung: | Haloalkane dehalogenases (
HLDs
) catalyse the hydrolysis of haloalkanes to alcohols, offering a biological solution for toxic haloalkane industrial wastes. Hundreds of putative
HLD
genes have been identified in bacterial genomes, but relatively few enzymes have been characterised. We identified two novel
HLDs
in the genome of
M
ycobacterium rhodesiae
strain JS60, an isolate from an organochlorine‐contaminated site:
DmrA
and
DmrB
. Both recombinant enzymes were active against
C
2–
C
6 haloalkanes, with a preference for brominated linear substrates. However,
DmrA
had higher activity against a wider range of substrates. The kinetic parameters of
DmrA
with 4‐bromobutyronitrile as a substrate were
K
m
= 1.9 ± 0.2 mM,
k
cat
= 3.1 ± 0.2 s
−1
.
DmrB
showed the highest activity against 1‐bromohexane.
DmrA
is monomeric, whereas
DmrB
is tetrameric. We determined the crystal structure of selenomethionyl
DmrA
to 1.7 Å resolution. A spacious active site and alternate conformations of a methionine side‐chain in the slot access tunnel may contribute to the broad substrate activity of
DmrA
. We show that
M
. rhodesiae
JS
60 can utilise 1‐iodopropane, 1‐iodobutane and 1‐bromobutane as sole carbon and energy sources. This ability appears to be conferred predominantly through
DmrA
, which shows significantly higher levels of upregulation in response to haloalkanes than
DmrB
. |
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ISSN: | 0950-382X 1365-2958 |
DOI: | 10.1111/mmi.13039 |