Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Pivot Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Target Concepts:
Gene/Protein
Disease
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Drug
Enzyme
Compound
Query: EC:1.10.3.2 (
laccase
)
4,656
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
A new
laccase
isoenzyme (POXA1b, where
POX
is phenol oxidase), produced by Pleurotus ostreatus in cultures supplemented with copper sulphate, has been purified and fully characterized. The main characteristics of this protein (molecular mass in native and denaturing conditions, pI and catalytic properties) are almost identical to the previously studied
laccase
POXA1w. However, POXA1b contains four copper atoms per molecule instead of one copper, two zinc and one iron atom per molecule of POXA1w. Furthermore, POXA1b shows an unusually high stability at alkaline pH. The gene and cDNA coding for POXA1b have been cloned and sequenced. The gene coding sequence contains 1599 bp, interrupted by 15 introns. Comparison of the structure of the poxa1b gene with the two previously studied P. ostreatus
laccase
genes (pox1 and poxc) suggests that these genes belong to two different subfamilies. The amino acid sequence of POXA1b deduced from the cDNA sequence has been almost completely verified by means of matrix-assisted laser desorption ionization MS. It has been demonstrated that three out of six putative glycosylation sites are post-translationally modified and the structure of the bound glycosidic moieties has been determined, whereas two other putative glycosylation sites are unmodified.
...
PMID:Protein and gene structure of a blue laccase from Pleurotus ostreatus1. 1041 29
Pleurotus ostreatus is a white rot basidiomycete that produces several extracellular
laccase
isoenzymes, including phenol oxidase A1b (POXA1b), POXA2, and POXC. POXC was the most abundant isoenzyme produced under all of the growth conditions examined in this study. Copper was the most efficient inducer of
laccase
activity among the putative inducers tested. The amounts of all of the previously described
laccase
isoenzymes increased substantially in copper-supplemented cultures. Under these conditions expression of
POX
isoenzymes was regulated at the level of gene transcription. It is worth noting that poxa1b mRNA was the most abundant induced transcript at all of the growth times analyzed, and the amount of this mRNA increased until day 7. The discrepancy between the poxa1b transcript and protein amounts can be explained by the presence of a high level of the protein in P. ostreatus cellular extract, which indicated that the POXA1b isoenzyme could be inefficiently secreted and/or that its physiological activity could occur inside the cell or on the cell wall. Moreover, the POXA1b isoenzyme behaved uniquely, as its activity was maximal on the second day of growth and then decreased. An analysis performed with protease inhibitors revealed that the loss of extracellular POXA1b activity could have been due to the presence of specific proteases secreted into the copper-containing culture medium that affected the extracellular POXA1b isoenzyme.
...
PMID:Copper induction of laccase isoenzymes in the ligninolytic fungus Pleurotus ostreatus. 1069 52
The oxidation of benzyl alcohols with the enzyme
laccase
, under mediation by appropriate mediator compounds, yields carbonylic products, whereas
laccase
can not oxidise these non-phenolic substrates directly. The oxidation step is performed by the oxidised form of the mediator (Med(ox)), generated on its interaction with
laccase
. The Med(ox) can follow either an electron transfer (ET) or a radical hydrogen atom transfer (HAT) route of oxidation of the substrates. Experimental evidence is reported that enables unambiguous assessment of the occurrence of either one the oxidation routes with each of the investigated mediators, namely, ABTS, HBT,
HPI
and VLA. Support to the conclusions is provided by (i) investigating the intermolecular selectivity of oxidation with appropriate substrates, (ii) attempting Hammett correlations for the oxidation of a series of 4-X-substituted benzyl alcohols, (iii) measuring the kinetic isotope effect, (iv) investigating the product pattern with suitable probe precursors. Based on these points, a HAT mechanism results to be followed by the
laccase
-HBT,
laccase
-
HPI
and
laccase
-VLA systems, whereas an ET route appears feasible in the case of the
laccase
-ABTS system.
...
PMID:Promoting laccase activity towards non-phenolic substrates: a mechanistic investigation with some laccase-mediator systems. 1292 10
Laccase (EC 1.10.3.1) activity was measured in regenerating and non-regenerating protoplasts isolated from tobacco (Nicotiana tabacum, L.) leaves. Laccase activity diminished soon after isolation: thereafter,it steadily increased in regenerating protoplasts during a 6-day culture period, whereas it was undetectable in non-regenerating protoplasts. A different pattern of isoforms was expressed in protoplasts by comparison with the donor tissue. Polyphenol oxidizing activity was detected also in the spent medium but it was not possible to definitely determine if it was due to
laccase
or to peroxidase (
POX
, EC 1.11.1.7) activity. New isoPOXs were quickly expressed soon after protoplast isolation as well, but
POX
activity remained negligible during the first day in culture. Leaf wounding induced an immediate stimulation of
laccase
activity whereas
POX
activity increased very slowly and peaked only after 4 days. Therefore,
laccase
could be the only effective polymerizing enzyme during the first day of protoplast culture and could contribute in the first steps of healing in wounded leaves, substituting for
POX
activity in cell wall reconstitution when hydrogen peroxide is not yet available.
...
PMID:Laccase activity could contribute to cell-wall reconstitution in regenerating protoplasts. 2462 2
