Your search keyword '"Paul A.M. Michels"' showing total 4 results

1. The characterization and evolutionary relationships of a trypanosomal thiolase

Author

Pauline Morand, Frédéric Bringaud, Rik K. Wierenga, Muriel Mazet, Rajesh K. Harijan, Antti M. Haapalainen, Paul A.M. Michels, Jorge Morales, and Tiila R. Kiema

Subjects

Signal peptide, Trypanosoma, Gene Expression, Protein Sorting Signals, Glycosome, Escherichia coli, Cluster Analysis, Humans, Cloning, Molecular, Trypanosoma cruzi, Phylogeny, SCP2, Leishmania, Sequence Homology, Amino Acid, biology, Thiolase, Gene Expression Profiling, Computational Biology, Acetyl-CoA C-Acyltransferase, biology.organism_classification, Recombinant Proteins, Mitochondria, Isoenzymes, Metabolic pathway, Infectious Diseases, Biochemistry, Parasitology, Energy source

Abstract

Thiolases are enzymes that remove an acetyl-coenzyme A group from acyl-CoA in the catabolic β-oxidation of fatty acids, or catalyse the reverse condensation reaction for anabolic processes such as the biosynthesis of sterols and ketone bodies. In humans, six homologous isoforms of thiolase have been described, differing from each other in sequence, oligomeric state, substrate specificity and subcellular localization. A bioinformatics analysis of parasite genomes, being (i) different species of African trypanosomes, (ii) Trypanosoma cruzi and (iii) Leishmania spp., using the six human sequences as queries, showed that the distribution of thiolases in human and each of the studied Trypanosomatidae is completely different. Only one of these isoforms, called SCP2-thiolase, was found in each of the Trypanosomatidae, whereas the TFE-thiolase was also found in T. cruzi and Leishmania spp., and the AB-thiolase only in T. cruzi. Each of the trypanosomatid thiolases clusters with its orthologues from other organisms in a phylogenetic analysis and shares with them the isoform-specific sequence fingerprints. The single T. brucei SCP2-thiolase has been expressed in Escherichia coli and characterized. It shows activity in both the degradative and synthetic directions. Transcripts of this thiolase were detected in both bloodstream- and procyclic-form trypanosomes, but the protein was found only in the procyclic form. The encoded protein has both a predicted N-terminal mitochondrial signal peptide and a C-terminal candidate type 1 peroxisomal-targeting signal for sorting it into glycosomes. However experimentally, only a mitochondrial localization was found for both procyclic trypanosomes grown with glucose and cells cultured with amino acids as an energy source. When the thiolase expression in procyclic cells was knocked down by RNA interference, no important change in growth rate occurred, irrespective of whether the cells were grown with or without glucose, indicating that the metabolic pathway(s) involving this enzyme is/are not essential for the parasite under either of these growth conditions.

Published

2011

2. Enzymes of carbohydrate metabolism as potential drug targets

Author

Fred R. Opperdoes and Paul A.M. Michels

Subjects

chemistry.chemical_classification, Drug, Trypanosoma, media_common.quotation_subject, Computational biology, Carbohydrate metabolism, Biology, Trypanocidal Agents, Glycosome, Infectious Diseases, Enzyme, Drug development, chemistry, Biochemistry, Drug Design, Animals, Carbohydrate Metabolism, Chagas Disease, Parasitology, Enzyme Inhibitors, Protozoal disease, Glycolysis, media_common

Abstract

The potential for chemotherapeutic exploitation of carbohydrate metabolism in the Trypanosomatidae is reviewed. This review is based largely on discussions held at a meeting of the COST B9 Action, entitled 'Bioenergetics of Protozoan Parasites'. The major questions posed were: which enzymes are the best to target; what further information is required to allow their use for rational drug development; what compounds would constitute the best inhibitors and which of the enzymes of the pentose-phosphate pathway are present inside the glycosomes, as well? Only partial answers could be obtained in many cases, but the interactive discussion between the multidisciplinary group of participants, comprising chemists, biochemists and molecular biologists, provided thought-provoking ideas and will help direct future research.

Published

2001

3. When, how and why glycolysis became compartmentalised in the Kinetoplastea. A new look at an ancient organelle

Author

Paul A.M. Michels, Frédéric Bringaud, Melisa Gualdrón-López, Juan Luis Concepción, Véronique Hannaert, Ana Brennand, Wilfredo Quiñones, and Ana J. Cáceres

Subjects

chemistry.chemical_classification, Euglenida, biology, Catabolism, Euglenozoa, Kinetoplastida, Peroxisome, biology.organism_classification, Glycosome, Biological Evolution, Microbodies, Infectious Diseases, Enzyme, chemistry, Biochemistry, Organelle, Protozoa, Parasitology, Glycolysis, Metabolic Networks and Pathways

Abstract

A characteristic, well-studied feature of the pathogenic protists belonging to the family Trypanosomatidae is the compartmentalisation of the major part of the glycolytic pathway in peroxisome-like organelles, hence designated glycosomes. Such organelles containing glycolytic enzymes appear to be present in all members of the Kinetoplastea studied, and have recently also been detected in a representative of the Diplonemida, but they are absent from the Euglenida. Glycosomes therefore probably originated in a free-living, common ancestor of the Kinetoplastea and Diplonemida. The initial sequestering of glycolytic enzymes inside peroxisomes may have been the result of a minor mistargeting of proteins, as generally observed in eukaryotic cells, followed by preservation and its further expansion due to the selective advantage of this specific form of metabolic compartmentalisation. This selective advantage may have been a largely increased metabolic flexibility, allowing the organisms to adapt more readily and efficiently to different environmental conditions. Further evolution of glycosomes involved, in different taxonomic lineages, the acquisition of additional enzymes and pathways - often participating in core metabolic processes - as well as the loss of others. The acquisitions may have been promoted by the sharing of cofactors and crucial metabolites between different pathways, thus coupling different redox processes and catabolic and anabolic pathways within the organelle. A notable loss from the Trypanosomatidae concerned a major part of the typical peroxisomal H(2)O(2)-linked metabolism. We propose that the compartmentalisation of major parts of the enzyme repertoire involved in energy, carbohydrate and lipid metabolism has contributed to the multiple development of parasitism, and its elaboration to complicated life cycles involving consecutive different hosts, in the protists of the Kinetoplastea clade.

Published

2011

4. Glycosomal ABC transporters of Trypanosoma brucei: characterisation of their expression, topology and substrate specificity

Author

Paul A.M. Michels, Pierre Wallemacq, Gladys Deumer, Muriel Mazet, and Mariana Igoillo-Esteve

Subjects

chemistry.chemical_classification, biology, Fatty Acids, Trypanosoma brucei brucei, Protozoan Proteins, Fatty acid, Gene Expression Regulation, Developmental, ATP-binding cassette transporter, Metabolism, Peroxisome, Trypanosoma brucei, biology.organism_classification, Glycosome, Microbodies, Substrate Specificity, Cytosol, Infectious Diseases, chemistry, Biochemistry, Organelle, Parasitology, ATP-Binding Cassette Transporters, Acyl Coenzyme A

Abstract

Metabolism in trypanosomatids is compartmentalised with major pathways, notably glycolysis, present in peroxisome-like organelles called glycosomes. To date, little information is available about the transport of metabolites through the glycosomal membrane. Previously, three ATP-binding cassette (ABC) transporters, called GAT1-3 for Glycosomal ABC Transporters 1 to 3, have been identified in the glycosomal membrane of Trypanosoma brucei. Here we report that GAT1 and GAT3 are expressed both in bloodstream and procyclic form trypanosomes, whereas GAT2 is mainly or exclusively expressed in bloodstream-form cells. Protease protection experiments showed that the nucleotide-binding domain of GAT1 and GAT3 is exposed to the cytosol, indicating that these transporters mediate the ATP-dependent uptake of solutes from the cytosol into the glycosomal lumen. Depletion of GAT1 and GAT3 by RNA interference in procyclic cells grown in glucose-containing medium did not affect growth. Surprisingly, GAT1 depletion enhanced the expression of the very different GAT3 protein. Expression knockdown of GAT1, but not GAT3, in procyclic cells cultured in glucose-free medium was lethal. Depletion of GAT1 in glucose-grown procyclic cells caused a modification of the total cellular fatty-acid composition. No or only minor changes were observed in the levels of most fatty acids, including oleate (C18:1), nevertheless the linoleate (C18:2) abundance was significantly increased upon GAT1 silencing. Furthermore, glycosomes purified from procyclic wild-type cells incorporate oleoyl-CoA in a concentration- and ATP-dependent manner, whilst this incorporation was severely reduced in glycosomes from cells in which GAT1 levels had been decreased. Together, these results strongly suggest that GAT1 serves to transport primarily oleoyl-CoA, but possibly also other fatty acids, from the cytosol into the glycosomal lumen and that its depletion results in a cellular linoleate accumulation, probably due to the presence of an active oleate desaturase. The role of intraglycosomal oleoyl-CoA and its essentiality when the trypanosomes are grown in the absence of glucose, are discussed.

Published

2010