19 research outputs found
Synthetic enzymes for synthetic substrates
In recent years, hydrolases like cutinases, esterases and lipases have been recognized as powerful tools for hydrolysis of synthetic polymers such as polyethylene terephthalate (PET) as an environmentally friendly alternative for environmentally harmful chemical recycling methods1. PET is currently the most common type of aromatic polyester, with widespread application as packaging material, beverage bottles, and synthetic textile fibers. So far, cutinases have been the most active enzyme class regarding PET degradation. In nature, cutinases catalyze the hydrolysis of the aliphatic biopolyester cutin, the structural component of plant cuticle. Although cutinases are able to act on natural insoluble polyesters, their activities on non-natural substrates are quit low. For this reason, different engineering strategies were established to optimize âpolyesterasesâ for synthetic polymers (Fig.1). Thereby, development of rationale enzyme-engineering strategies led to remarkable enhancement of hydrolytic activities on polyesters and clearly showed that the affinity between the enzyme and the substrate plays a key role in the enzymatic hydrolysis of synthetic polyester.
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A fungal ascorbate oxidase with unexpected laccase activity
Ascorbate oxidases are an enzyme group that has not been explored to a large extent. So far, mainly ascorbate oxidases from plants and only a few from fungi have been described. Although ascorbate oxidases belong to the well-studied enzyme family of multi-copper oxidases, their function is still unclear. In this study, Af_AO1, an enzyme from the fungus Aspergillus flavus, was characterized. Sequence analyses and copper content determination demonstrated Af_AO1 to belong to the multi-copper oxidase family. Biochemical characterization and 3D-modeling revealed a similarity to ascorbate oxidases, but also to laccases. Af_AO1 had a 10-fold higher affinity to ascorbic acid (KM = 0.16 ± 0.03 mM) than to ABTS (KM = 1.89 ± 0.12 mM). Furthermore, the best fitting 3D-model was based on the ascorbate oxidase from Cucurbita pepo var. melopepo. The laccase-like activity of Af_AO1 on ABTS (Vmax = 11.56 ± 0.15 ”M/min/mg) was, however, not negligible. On the other hand, other typical laccase substrates, such as syringaldezine and guaiacol, were not oxidized by Af_AO1. According to the biochemical and structural characterization, Af_AO1 was classified as ascorbate oxidase with unusual, laccase-like activityPeer ReviewedPostprint (published version
Characterization of organelles from the yeast Pichia pastoris
Sabine ZitzenbacherZsfassung in dt. SpracheGraz, Univ., Masterarb., 2009(VLID)24573
Biomimetic Approach to Enhance Enzymatic Hydrolysis of the Synthetic Polyester Poly(1,4-butylene adipate): Fusing Binding Modules to Esterases
Mimicking a concept of nature for
the hydrolysis of biopolymers,
the <i>Thermobifida cellulosilytica</i> cutinase 1 (Thc_Cut1)
was fused to a polymer binding module (PBM) to enhance the hydrolysis
of the polyester polyÂ(1,4-butylene adipate) (PBA). Namely, the binding
module of a polyhydroxyalkanoate depolymerase from <i>Alcaligenes
faecalis</i> (Thc_Cut1_PBM) was attached to the cutinase via
two different linker sequences varying in length. In order to investigate
the adsorption behavior, catalytically inactive mutants both of Thc_Cut1
and Thc_Cut1_PBM were successfully constructed by site-directed mutagenesis
of serine 131 to alanine. Quartz crystal microbalance with dissipation
monitoring (QCM-D) analysis revealed that the initial mass increase
during enzyme adsorption was larger for the inactive enzymes linked
with the PBM as compared to the enzyme without the PBM. The hydrolysis
rates of PBA were significantly enhanced when incubated with the active,
engineered Thc_Cut1_PBM as compared to the native Thc_Cut1. Thc_Cut1_PBM
completely hydrolyzed PBA thin films on QCM-D sensors within approximately
40 min, whereas twice as much time was required for the complete hydrolysis
by the native Thc_Cut1
Hydrolysis of Ionic Phthalic Acid Based Polyesters by Wastewater Microorganisms and Their Enzymes
Water-soluble
polyesters are used in a range of applications today
and enter wastewater treatment plants after product utilization. However,
little is known about extracellular enzymes and aquatic microorganisms
involved in polyester biodegradation and mineralization. In this study,
structurally different ionic phthalic acid based polyesters (the number-average
molecular weights (<i>M</i><sub>n</sub>) 1770 to 10âŻ000
g/mol and semi crystalline with crystallinity below 1%) were synthesized
in various combinations. Typical wastewater microorganisms like <i>Pseudomonas</i> sp. were chosen for <i>in-silico</i> screening toward polyester hydrolyzing enzymes. Based on the <i>in-silico</i> search, a cutinase from <i>Pseudomonas pseudoalcaligenes</i> (PpCutA) and a putative lipase from <i>Pseudomonas pelagia</i> (PpelaLip) were identified. The enzymes PpCutA and PpelaLip were
demonstrated to hydrolyze all structurally different polyesters. Activities
on all the polyesters were also confirmed with the strains <i>P. pseudoalcaligenes</i> and <i>P. pelagia</i>. Parameters
identified to enhance hydrolysis included increased water solubility
and polyester hydrophilicity as well as shorter diol chain lengths.
For example, polyesters containing 1,2-ethanediol were hydrolyzed
faster than polyesters containing 1,8-octanediol. Interestingly, the
same trend was observed in biodegradation experiments. This information
is important to gain a better mechanistic understanding of biodegradation
processes of polyesters in WWTPs where the extracellular enzymatic
hydrolysis seems to be the limiting step
A New Esterase from Thermobifida halotolerans Hydrolyses Polyethylene Terephthalate (PET) and Polylactic Acid (PLA)
A new esterase from Thermobifida halotolerans (Thh_Est) was cloned and expressed in E. coli and investigated for surface hydrolysis of polylactic acid (PLA) and polyethylene terephthalate (PET). Thh_Est is a member of the serine hydrolases superfamily containing the -GxSxG- motif with 85â87% homology to an esterase from T. alba, to an acetylxylan esterase from T. fusca and to various Thermobifida cutinases. Thh_Est hydrolyzed the PET model substrate bis(benzoyloxyethyl)terephthalate and PET releasing terephthalic acid and mono-(2-hydroxyethyl) terephthalate in comparable amounts (19.8 and 21.5 mmol/mol of enzyme) while no higher oligomers like bis-(2-hydroxyethyl) terephthalate were detected. Similarly, PLA was hydrolyzed as indicated by the release of lactic acid. Enzymatic surface hydrolysis of PET and PLA led to a strong hydrophilicity increase, as quantified with a WCA decrease from 90.8° and 75.5° to 50.4° and to a complete spread of the water drop on the surface, respectively
DataSheet1_Dihydropyrimidinase from Saccharomyces kluyveri can hydrolyse polyamides.PDF
In Saccharomyces kluyveri, dihydropyrimidinase (DHPaseSK) is involved in the pyrimidine degradation pathway, which includes the reversible ring cleavage between nitrogen 3 and carbon 4 of 5,6-dihydrouracil. In this study, DPHaseSK was successfully cloned and expressed in E. coli BL-21 Gold (DE3) with and without affinity tags. Thereby, the Strep-tag enabled fastest purification and highest specific activity (9.5 ± 0.5 U/mg). The biochemically characterized DHPaseSK_Strep had similar kinetic parameters (Kcat/Km) on 5,6-dihydrouracil (DHU) and para-nitroacetanilide respectively, with 7,229 and 4060 Mâ1 sâ1. The hydrolytic ability of DHPaseSK_Strep to polyamides (PA) was tested on PA consisting of monomers with different chain length (PA-6, PA-6,6, PA-4,6, PA-4,10 and PA-12). According to LC-MS/TOF analysis, DHPaseSK_Strep showed a preference for films containing the shorter chain monomers (e.g., PA-4,6). In contrast, an amidase from Nocardia farcinica (NFpolyA) showed some preference for PA consisting of longer chain monomers. In conclusion, in this work DHPaseSK_Strep was demonstrated to be able to cleave amide bonds in synthetic polymers, which can be an important basis for development of functionalization and recycling processes for polyamide containing materials.</p