Your search keyword '"Carlos H. Trasviña-Arenas"' showing total 19 results

1. Cellular Repair of Synthetic Analogs of Oxidative DNA Damage Reveals a Key Structure–Activity Relationship of the Cancer-Associated MUTYH DNA Repair Glycosylase

Author

Savannah G. Conlon, Cindy Khuu, Carlos H. Trasviña-Arenas, Tian Xia, Michelle L. Hamm, Alan G. Raetz, and Sheila S. David

Subjects

Chemistry, QD1-999

Published

2024

2. Corrigendum: The sole DNA ligase in Entamoeba histolytica is a high-fidelity DNA ligase involved in DNA damage repair

Author

Elisa Azuara-Liceaga, Abigail Betanzos, Cesar S. Cardona-Felix, Elizabeth J. Castañeda-Ortiz, Helios Cárdenas, Rosa E. Cárdenas-Guerra, Guillermo Pastor-Palacios, Guillermina García-Rivera, David Hernández-Álvarez, Carlos H. Trasviña-Arenas, Corina Diaz-Quezada, Esther Orozco, and Luis G. Brieba

Subjects

EhDNAligI, protozoan, DNA insults, ligation, repairing, 8-oxoG adduct, Microbiology, QR1-502

Published

2022

3. The Sole DNA Ligase in Entamoeba histolytica Is a High-Fidelity DNA Ligase Involved in DNA Damage Repair

Author

Elisa Azuara-Liceaga, Abigail Betanzos, Cesar S. Cardona-Felix, Elizabeth J. Castañeda-Ortiz, Helios Cárdenas, Rosa E. Cárdenas-Guerra, Guillermo Pastor-Palacios, Guillermina García-Rivera, David Hernández-Álvarez, Carlos H. Trasviña-Arenas, Corina Diaz-Quezada, Esther Orozco, and Luis G. Brieba

Subjects

EhDNAligI, protozoan, DNA insults, ligation, repairing, 8-oxoG adduct, Microbiology, QR1-502

Abstract

The protozoan parasite Entamoeba histolytica is exposed to reactive oxygen and nitric oxide species that have the potential to damage its genome. E. histolytica harbors enzymes involved in DNA repair pathways like Base and Nucleotide Excision Repair. The majority of DNA repairs pathways converge in their final step in which a DNA ligase seals the DNA nicks. In contrast to other eukaryotes, the genome of E. histolytica encodes only one DNA ligase (EhDNAligI), suggesting that this ligase is involved in both DNA replication and DNA repair. Therefore, the aim of this work was to characterize EhDNAligI, its ligation fidelity and its ability to ligate opposite DNA mismatches and oxidative DNA lesions, and to study its expression changes and localization during and after recovery from UV and H2O2 treatment. We found that EhDNAligI is a high-fidelity DNA ligase on canonical substrates and is able to discriminate erroneous base-pairing opposite DNA lesions. EhDNAligI expression decreases after DNA damage induced by UV and H2O2 treatments, but it was upregulated during recovery time. Upon oxidative DNA damage, EhDNAligI relocates into the nucleus where it co-localizes with EhPCNA and the 8-oxoG adduct. The appearance and disappearance of 8-oxoG during and after both treatments suggest that DNA damaged was efficiently repaired because the mainly NER and BER components are expressed in this parasite and some of them were modulated after DNA insults. All these data disclose the relevance of EhDNAligI as a specialized and unique ligase in E. histolytica that may be involved in DNA repair of the 8-oxoG lesions.

Published

2018

4. Structural snapshots of base excision by the cancer-associated variant MutY N146S reveal a retaining mechanism

Author

Merve Demir, L Peyton Russelburg, Wen-Jen Lin, Carlos H Trasviña-Arenas, Beili Huang, Philip K Yuen, Martin P Horvath, and Sheila S David

Subjects

Genetics

Abstract

DNA glycosylase MutY plays a critical role in suppression of mutations resulted from oxidative damage, as highlighted by cancer-association of the human enzyme. MutY requires a highly conserved catalytic Asp residue for excision of adenines misinserted opposite 8-oxo-7,8-dihydroguanine (OG). A nearby Asn residue hydrogen bonds to the catalytic Asp in structures of MutY and its mutation to Ser is an inherited variant in human MUTYH associated with colorectal cancer. We captured structural snapshots of N146S Geobacillus stearothermophilus MutY bound to DNA containing a substrate, a transition state analog and enzyme-catalyzed abasic site products to provide insight into the base excision mechanism of MutY and the role of Asn. Surprisingly, despite the ability of N146S to excise adenine and purine (P) in vitro, albeit at slow rates, N146S-OG:P complex showed a calcium coordinated to the purine base altering its conformation to inhibit hydrolysis. We obtained crystal structures of N146S Gs MutY bound to its abasic site product by removing the calcium from crystals of N146S-OG:P complex to initiate catalysis in crystallo or by crystallization in the absence of calcium. The product structures of N146S feature enzyme-generated β-anomer abasic sites that support a retaining mechanism for MutY-catalyzed base excision.

Published

2023

5. Evolution of Base Excision Repair in Entamoeba histolytica is shaped by gene loss, gene duplication, and lateral gene transfer

Author

Carlos H. Trasviña-Arenas, Luis G. Brieba, Elisa Azuara-Liceaga, Sheila S. David, and Luis Delaye

Subjects

Models, Molecular, DNA Repair, Gene Transfer, Horizontal, Protein Conformation, DNA repair, Genes, Protozoan, Biochemistry, DNA Glycosylases, Evolution, Molecular, 03 medical and health sciences, Entamoeba histolytica, 0302 clinical medicine, Gene Duplication, parasitic diseases, Gene duplication, Humans, AP site, Amino Acid Sequence, Molecular Biology, Gene, 030304 developmental biology, Genetics, chemistry.chemical_classification, 0303 health sciences, DNA ligase, biology, Cell Biology, Base excision repair, biology.organism_classification, chemistry, DNA glycosylase, 030220 oncology & carcinogenesis

Abstract

During its life cycle, the protist parasite Entamoeba histolytica encounters reactive oxygen and nitrogen species that alter its genome. Base excision repair (BER) is one of the most important pathways for the repair of DNA base lesions. Analysis of the E. histolytica genome revealed the presence of most of the BER components. Surprisingly, this included a gene encoding an apurinic/apyrimidinic (AP) endonuclease that previous studies had assumed was absent. Indeed, our analysis showed that the genome of E. histolytica harbors the necessary genes needed for both short and long-patch BER sub-pathways. These genes include DNA polymerases with predicted 5'-dRP lyase and strand-displacement activities and a sole DNA ligase. A distinct feature of the E. histolytica genome is the lack of several key damage-specific BER glycosylases, such as OGG1/MutM, MDB4, Mag1, MPG, SMUG, and TDG. Our evolutionary analysis indicates that several E. histolytica DNA glycosylases were acquired by lateral gene transfer (LGT). The genes that encode for MutY, AlkD, and UDG (Family VI) are included among these cases. Endonuclease III and UNG (family I) are the only DNA glycosylases with a eukaryotic origin in E. histolytica. A gene encoding a MutT 8-oxodGTPase was also identified that was acquired by LGT. The mixed composition of BER genes as a DNA metabolic pathway shaped by LGT in E. histolytica indicates that LGT plays a major role in the evolution of this eukaryote. Sequence and structural prediction of E. histolytica DNA glycosylases, as well as MutT, suggest that the E. histolytica DNA repair proteins evolved to harbor structural modifications that may confer unique biochemical features needed for the biology of this parasite.

Published

2019

6. Structure, function and evolution of the Helix-hairpin-Helix DNA glycosylase superfamily: Piecing together the evolutionary puzzle of DNA base damage repair mechanisms

Author

Sheila S. David, Merve Demir, Carlos H. Trasviña-Arenas, and Wen-Jen Lin

Subjects

DNA Repair, DNA repair, Deamination, Cell Biology, Computational biology, Base excision repair, DNA, Biology, Biochemistry, Nucleobase, DNA Glycosylases, chemistry.chemical_compound, chemistry, DNA glycosylase, Helix, DNA-(Apurinic or Apyrimidinic Site) Lyase, AP site, Molecular Biology, DNA Damage

Abstract

The Base Excision Repair (BER) pathway is a highly conserved DNA repair system targeting chemical base modifications that arise from oxidation, deamination and alkylation reactions. BER features lesion-specific DNA glycosylases (DGs) which recognize and excise modified or inappropriate DNA bases to produce apurinic/apyrimidinic (AP) sites and coordinate AP-site hand-off to subsequent BER pathway enzymes. The DG superfamilies identified have evolved independently to cope with a wide variety of nucleobase chemical modifications. Most DG superfamilies recognize a distinct set of structurally related lesions. In contrast, the Helix-hairpin-Helix (HhH) DG superfamily has the remarkable ability to act upon structurally diverse sets of base modifications. The versatility in substrate recognition of the HhH-DG superfamily has been shaped by motif and domain acquisitions during evolution. In this paper, we review the structural features and catalytic mechanisms of the HhH-DG superfamily and draw a hypothetical reconstruction of the evolutionary path where these DGs developed diverse and unique enzymatic features.

Published

2021

7. Plant organellar DNA polymerases repair double-stranded breaks by microhomology-mediated end-joining

Author

Luis G. Brieba, Antolín Peralta-Castro, Alfredo Torres-Larios, Carlos H. Trasviña-Arenas, Noe Baruch-Torres, and Paola L. García-Medel

Subjects

Mitochondrial DNA, DNA End-Joining Repair, DNA polymerase, Arabidopsis, DNA-Directed DNA Polymerase, DNA-binding protein, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Genetics, DNA Breaks, Double-Stranded, Homologous Recombination, Polymerase, 030304 developmental biology, Organelles, 0303 health sciences, biology, Nucleotides, Nucleic Acid Enzymes, fungi, food and beverages, Gene rearrangement, Cell biology, DNA-Binding Proteins, Microhomology-mediated end joining, chemistry, biology.protein, Homologous recombination, 030217 neurology & neurosurgery, DNA

Abstract

Double-stranded breaks (DSBs) in plant organelles are repaired via genomic rearrangements characterized by microhomologous repeats. These microhomologous signatures predict the existence of an unidentified enzymatic machinery capable of repairing of DSBs via microhomology-mediated end-joining (MMEJ) in plant organelles. Here, we show that organellar DNA polymerases from Arabidopsis thaliana (AtPolIA and AtPolIB) perform MMEJ using microhomologous sequences as short as six nucleotides. AtPolIs execute MMEJ by virtue of two specialized amino acid insertions located in their thumb subdomains. Single-stranded binding proteins (SSBs) unique to plants, AtWhirly2 and organellar single-stranded binding proteins (AtOSBs), hinder MMEJ, whereas canonical mitochondrial SSBs (AtmtSSB1 and AtmtSSB2) do not interfere with MMEJ. Our data predict that organellar DNA rearrangements by MMEJ are a consequence of a competition for the 3′-OH of a DSBs. If AtWhirlies or AtOSBs gain access to the single-stranded DNA (ssDNA) region of a DSB, the reaction will shift towards high-fidelity routes like homologous recombination. Conversely MMEJ would be favored if AtPolIs or AtmtSSBs interact with the DSB. AtPolIs are not phylogenetically related to metazoan mitochondrial DNA polymerases, and the ability of AtPolIs to execute MMEJ may explain the abundance of DNA rearrangements in plant organelles in comparison to animal mitochondria.

Published

2019

8. Proliferating cell nuclear antigen restores the enzymatic activity of a DNA ligase I deficient in DNA binding

Author

Cesar S. Cardona-Felix, Elisa Azuara-Liceaga, Carlos H. Trasviña-Arenas, Luis G. Brieba, and Corina Diaz-Quezada

Subjects

0301 basic medicine, chemistry.chemical_classification, DNA ligase, DNA clamp, HMG-box, Okazaki fragments, DNA repair, Biology, DNA polymerase delta, Molecular biology, General Biochemistry, Genetics and Molecular Biology, Proliferating cell nuclear antigen, 03 medical and health sciences, 030104 developmental biology, protein–protein interaction, chemistry, PIP box, biology.protein, PCNA, DNA mismatch repair, Research Articles, Research Article

Abstract

Proliferating cell nuclear antigen (PCNA) coordinates multi-enzymatic reactions by interacting with a variety of protein partners. Family I DNA ligases are multidomain proteins involved in sealing of DNA nicks during Okazaki fragment maturation and DNA repair. The interaction of DNA ligases with the inter-domain connector loop (IDCL) of PCNA through its PCNA interacting peptide (PIP box) is well studied but the role of the interacting surface between both proteins is not well characterized. In this work, we used a minimal DNA ligase I and two N-terminal deletions to establish that DNA binding and nick-sealing stimulation of DNA ligase I by PCNA are not solely dependent on the PIP box–IDCL interaction. We found that a truncated DNA ligase I with a deleted PIP box is stimulated by PCNA. Furthermore, the activity of a DNA ligase defective in DNA binding is rescued upon PCNA addition. Since the rate constants for single-turnover ligation for the full-length and truncated DNA ligases are not affected by PCNA, our data suggest that PCNA stimulation is achieved by increasing the affinity for nicked DNA substrate and not by increasing catalytic efficiency. Surprisingly C-terminal mutants of PCNA are not able to stimulate nick-sealing activity of Entamoeba histolytica DNA ligase I. Our data supports the notion that the C-terminal region of PCNA may be involved in promoting an allosteric transition in E. histolytica DNA ligase I from a spread-shaped to a ring-shaped structure. This study suggests that the ring-shaped PCNA is a binding platform able to stabilize co-evolved protein–protein interactions, in this case an interaction with DNA ligase I. This article is protected by copyright. All rights reserved.

Published

2017

9. Modeling of pathogenic variants of mitochondrial DNA polymerase: insight into the replication defects and implication for human disease

Author

Nallely Hoyos-Gonzalez, Luis G. Brieba, Pedro Jimenez-Sandoval, Corina Diaz-Quezada, Enrico Baruffini, Antolín Peralta-Castro, Atzimaba Y. Castro-Lara, Carlos H. Trasviña-Arenas, Andrea Degiorgi, and Tiziana Lodi

Subjects

DNA Replication, Models, Molecular, Mitochondrial DNA, Mitochondrial Diseases, DNA polymerase, Biophysics, Biochemistry, DNA, Mitochondrial, 03 medical and health sciences, Humans, Molecular Biology, Gene, Polymerase, 030304 developmental biology, 0303 health sciences, biology, Chemistry, 030305 genetics & heredity, DNA replication, Processivity, Stop codon, DNA Polymerase gamma, Mutation, biology.protein, Primer (molecular biology)

Abstract

Background: Mutations in human gene encoding the mitochondrial DNA polymerase γ (HsPolγ) are associated with a broad range of mitochondrial diseases. Here we studied the impact on DNA replication by disease variants clustered around residue HsPolγ-K1191, a residue that in several family-A DNA polymerases interacts with the 3′ end of the primer. Methods Specifically, we examined the effect of HsPolγ carrying pathogenic variants in residues D1184, I1185, C1188, K1191, D1196, and a stop codon at residue T1199, using as a model the yeast mitochondrial DNA polymerase protein, Mip1p. Results The introduction of pathogenic variants C1188R (yV945R), and of a stop codon at residue T1199 (yT956X) abolished both polymerization and exonucleolysis in vitro. HsPolγ substitutions in residues D1184 (yD941), I1185 (yI942), K1191 (yK948) and D1196 (yD953) shifted the balance between polymerization and exonucleolysis in favor of exonucleolysis. HsPolγ pathogenic variants at residue K1191 (yK948) and D1184 (yD941) were capable of nucleotide incorporation albeit with reduced processivity. Structural analysis of mitochondrial DNAPs showed that residue HsPolγ-N864 is placed in an optimal distance to interact with the 3′ end of the primer and the phosphate backbone previous to the 3′ end. Amino acid changes in residue HsPolγ-N864 to Ala, Ser or Asp result in enzymes that did not decrease their polymerization activity on short templates but exhibited a substantial decrease for processive DNA synthesis. Conclusion Our data suggest that in mitochondrial DNA polymerases multiple amino acids are involved in the primer-stand stabilization.

Published

2019

10. Amino and carboxy-terminal extensions of yeast mitochondrial DNA polymerase assemble both the polymerization and exonuclease active sites

Author

Nallely Hoyos-Gonzalez, Enrico Baruffini, María E. Sanchez-Sandoval, Carlos H. Trasviña-Arenas, Annia Rodríguez-Hernández, Tiziana Lodi, Pedro Jimenez-Sandoval, Luis G. Brieba, Víctor M. Ayala-García, Corina Diaz-Quezada, and Atzimba Y. Castro-Lara

Subjects

Exonuclease, Mitochondrial DNA, Saccharomyces cerevisiae Proteins, DNA polymerase, Mutant, Saccharomyces cerevisiae, DNA, Mitochondrial, Mitochondrial Proteins, chemistry.chemical_compound, Catalytic Domain, Humans, DNA, Fungal, Molecular Biology, Polymerase, chemistry.chemical_classification, biology, DNA replication, Cell Biology, DNA Polymerase I, Amino acid, DNA Polymerase gamma, chemistry, Biochemistry, biology.protein, Molecular Medicine, DNA

Abstract

Human and yeast mitochondrial DNA polymerases (DNAPs), POLG and Mip1, are related by evolution to bacteriophage DNAPs. However, mitochondrial DNAPs contain unique amino and carboxyl-terminal extensions that physically interact. Here we describe that N-terminal deletions in Mip1 polymerases abolish polymerization and decrease exonucleolytic degradation, whereas moderate C-terminal deletions reduce polymerization. Similarly, to the N-terminal deletions, an extended C-terminal deletion of 298 amino acids is deficient in nucleotide addition and exonucleolytic degradation of double and single-stranded DNA. The latter observation suggests that the physical interaction between the amino and carboxyl-terminal regions of Mip1 may be related to the spread of pathogenic POLG mutant along its primary sequence.

Published

2019

11. Plant Organellar DNA Polymerases Evolved Multifunctionality through the Acquisition of Novel Amino Acid Insertions

Author

Antolín Peralta-Castro, Víctor Juarez-Quintero, Carlos H. Trasviña-Arenas, Carlos M. Morales-Vazquez, Luis G. Brieba, Paola L. García-Medel, and Noe Baruch-Torres

Subjects

0106 biological sciences, 0301 basic medicine, DNA End-Joining Repair, lcsh:QH426-470, DNA Repair, DNA polymerase, DNA repair, Arabidopsis, Review, DNA-Directed DNA Polymerase, Multifunctional Enzymes, DNA replication, 01 natural sciences, Evolution, Molecular, 03 medical and health sciences, chloroplast, Genetics, Amino Acids, Genetics (clinical), Polymerase, Plant Proteins, Organelles, plant organellar DNA polymerases, biology, DNA synthesis, Arabidopsis Proteins, Base excision repair, Processivity, Cell biology, mitochondria, lcsh:Genetics, 030104 developmental biology, biology.protein, 010606 plant biology & botany

Abstract

The majority of DNA polymerases (DNAPs) are specialized enzymes with specific roles in DNA replication, translesion DNA synthesis (TLS), or DNA repair. The enzymatic characteristics to perform accurate DNA replication are in apparent contradiction with TLS or DNA repair abilities. For instance, replicative DNAPs incorporate nucleotides with high fidelity and processivity, whereas TLS DNAPs are low-fidelity polymerases with distributive nucleotide incorporation. Plant organelles (mitochondria and chloroplast) are replicated by family-A DNA polymerases that are both replicative and TLS DNAPs. Furthermore, plant organellar DNA polymerases from the plant model Arabidopsis thaliana (AtPOLIs) execute repair of double-stranded breaks by microhomology-mediated end-joining and perform Base Excision Repair (BER) using lyase and strand-displacement activities. AtPOLIs harbor three unique insertions in their polymerization domain that are associated with TLS, microhomology-mediated end-joining (MMEJ), strand-displacement, and lyase activities. We postulate that AtPOLIs are able to execute those different functions through the acquisition of these novel amino acid insertions, making them multifunctional enzymes able to participate in DNA replication and DNA repair.

Published

2020

12. Solution structure of the inhibitor of cysteine proteases 1 from Entamoeba histolytica reveals a possible auto regulatory mechanism

Author

Luis G. Brieba, Claudia G. Benítez-Cardoza, Itzel Rentería-González, Carlos H. Trasviña-Arenas, David Flores-Solis, Federico del Río-Portilla, Pedro Jimenez-Sandoval, Angeles Mendoza, and Luz E. Casados-Vázquez

Subjects

Proteases, medicine.medical_treatment, 030303 biophysics, Protozoan Proteins, Biophysics, Cysteine Proteinase Inhibitors, Biochemistry, Analytical Chemistry, 03 medical and health sciences, chemistry.chemical_compound, Papain, Escherichia coli, medicine, Cloning, Molecular, Molecular Biology, Cellular localization, 030304 developmental biology, 0303 health sciences, Protease, biology, Chemistry, Entamoeba histolytica, Active site, Cysteine protease, Solutions, Mutagenesis, Site-Directed, biology.protein, Cysteine

Abstract

The genome of Entamoeba histolytica encodes approximately 50 Cysteine Proteases (CPs) whose activity is regulated by two Inhibitors of Cysteine Proteases (ICPs), EhICP1 and EhICP2. The main difference between both EhICPs is the acquisition of a 17 N-terminal targeting signal in EhICP2 and three exposed cysteine residues in EhICP1. The three exposed cysteines in EhICP1 potentiate the formation of cross-linking species that drive heterogeneity. Here we solved the NMR structure of EhICP1 using a mutant protein without accessible cysteines. Our structural data shows that EhICP1 adopts an immunoglobulin fold composed of seven β-strands, and three solvent exposed loops that resemble the structures of EhICP2 and chagasin. EhICP1 and EhICP2 are able to inhibit the archetypical cysteine protease papain by intercalating their BC loops into the protease active site independently of the character of the residue (serine or threonine) responsible to interact with the active site of papain. EhICP1 and EhICP2 present signals of functional divergence as they clustered in different clades. Two of the three exposed cysteines in EhICP1 are located at the DE loop that intercalates into the CP substrate-binding cleft. We propose that the solvent exposed cysteines of EhICP1 play a role in regulating its inhibitory activity and that in oxidative conditions, the cysteines of EhICP1 react to form intra and intermolecular disulfide bonds that render an inactive inhibitor. EhICP2 is not subject to redox regulation, as this inhibitor does not contain a single cysteine residue. This proposed redox regulation may be related to the differential cellular localization between EhICP1 and EhICP2.

Published

2020

13. Dispensability of the [4Fe-4S] cluster in novel homologues of adenine glycosylase MutY

Author

Eugenia Sánchez-Sandoval, Luis G. Brieba, Laura Margarita López-Castillo, and Carlos H. Trasviña-Arenas

Subjects

Iron-Sulfur Proteins, Models, Molecular, 0301 basic medicine, DNA repair, DNA polymerase, Guanine, Levilactobacillus brevis, Molecular Sequence Data, Sequence alignment, medicine.disease_cause, Biochemistry, DNA Glycosylases, 03 medical and health sciences, chemistry.chemical_compound, Escherichia coli, medicine, Amino Acid Sequence, Molecular Biology, Peptide sequence, Phylogeny, 030102 biochemistry & molecular biology, biology, Entamoeba histolytica, Cell Biology, 030104 developmental biology, chemistry, DNA glycosylase, biology.protein, Sequence Alignment, DNA

Abstract

7,8-Dihydro-8-deoxyguanine (8oG) is one of the most common oxidative lesions in DNA. DNA polymerases misincorporate an adenine across from this lesion. Thus, 8oG is a highly mutagenic lesion responsible for G:C→T:A transversions. MutY is an adenine glycosylase, part of the base excision repair pathway that removes adenines, when mispaired with 8oG or guanine. Its catalytic domain includes a [4Fe-4S] cluster motif coordinated by cysteinyl ligands. When this cluster is absent, MutY activity is depleted and several studies concluded that the [4Fe-4S] cluster motif is an indispensable component for DNA binding, substrate recognition and enzymatic activity. In the present study, we identified 46 MutY homologues that lack the canonical cysteinyl ligands, suggesting an absence of the [4Fe-4S] cluster. A phylogenetic analysis groups these novel MutYs into two different clades. One clade is exclusive of the order Lactobacillales and another clade has a mixed composition of anaerobic and microaerophilic bacteria and species from the protozoan genus Entamoeba. Structural modeling and sequence analysis suggests that the loss of the [4Fe-4S] cluster is compensated by a convergent solution in which bulky amino acids substitute the [4Fe-4S] cluster. We functionally characterized MutYs from Lactobacillus brevis and Entamoeba histolytica as representative members from each clade and found that both enzymes are active adenine glycosylases. Furthermore, chimeric glycosylases, in which the [4Fe-4S] cluster of Escherichia coli MutY is replaced by the corresponding amino acids of LbY and EhY, are also active. Our data indicates that the [4Fe-4S] cluster plays a structural role in MutYs and evidences the existence of alternative functional solutions in nature.

Published

2016

14. Identification of a unique insertion in plant organellar DNA polymerases responsible for 5'-dRP lyase and strand-displacement activities: Implications for Base Excision Repair

Author

Corina Diaz-Quezada, Francisco J. Cordoba-Andrade, Antolín Peralta-Castro, Víctor M. Ayala-García, Noe Baruch-Torres, Carlos H. Trasviña-Arenas, Paola L. García-Medel, José Juan Ordaz-Ortiz, and Luis G. Brieba

Subjects

0301 basic medicine, DNA Repair, DNA, Plant, DNA polymerase, Arabidopsis, DNA-Directed DNA Polymerase, Biochemistry, DNA, Mitochondrial, 03 medical and health sciences, chemistry.chemical_compound, Catalytic Domain, Arabidopsis thaliana, Amino Acid Sequence, Lyase activity, Molecular Biology, chemistry.chemical_classification, DNA ligase, biology, Arabidopsis Proteins, DNA, Chloroplast, food and beverages, Cell Biology, Base excision repair, biology.organism_classification, Lyase, Cell biology, Chloroplast, 030104 developmental biology, chemistry, biology.protein, Phosphorus-Oxygen Lyases, Sequence Alignment, DNA, DNA Damage

Abstract

Plant mitochondrial and chloroplast genomes encode essential proteins for oxidative phosphorylation and photosynthesis. For proper cellular function, plant organelles must ensure genome integrity. Although plant organelles repair damaged DNA using the multi-enzyme Base Excision Repair (BER) pathway, the details of this pathway in plant organelles are largely unknown. The initial enzymatic steps in BER produce a 5'-deoxyribose phosphate (5'-dRP) moiety that must be removed to allow DNA ligation and in plant organelles, the enzymes responsible for the removal of a 5'-dRP group are unknown. In metazoans, DNA polymerases (DNAPs) remove the 5'-dRP moiety using their intrinsic lyase and/or strand-displacement activities during short or long-patch BER sub-pathways, respectively. The plant model Arabidopsis thaliana encodes two family-A DNAPs paralogs, AtPolIA and AtPolIB, which are the sole DNAPs in plant organelles identified to date. Herein we demonstrate that both AtPolIs present 5'-dRP lyase activities. AtPolIB performs efficient strand-displacement on a BER-associated 1-nt gap DNA substrate, whereas AtPolIA exhibits only moderate strand-displacement activity. Both lyase and strand-displacement activities are dependent on an amino acid insertion that is exclusively present in plant organellar DNAPs. Within this insertion, we identified that residue AtPollB-Lys593 acts as nucleophile for lyase activity. Our results demonstrate that AtPolIs are functionally equipped to play a role in short-patch BER and suggest a major role of AtPolIB in a predicted long-patch BER sub-pathway. We propose that the acquisition of insertion 1 in the polymerization domain of AtPolIs was a key component in their evolution as BER associated and replicative DNAPs.

Published

2017

15. Cysteine Proteases Inhibitors with Immunoglobulin-Like Fold in Protozoan Parasites and their Role in Pathogenesis

Author

Luis G. Brieba, Carlos H. Trasviña-Arenas, Pedro Jimenez-Sandoval, and Laura Margarita López-Castillo

Subjects

Protein Conformation, alpha-Helical, 0301 basic medicine, Protein Folding, Proteases, Trypanosoma cruzi, Leishmania mexicana, Plasmodium falciparum, Protozoan Proteins, Gene Expression, Immunoglobulins, Plasma protein binding, Immunoglobulin domain, Cysteine Proteinase Inhibitors, Biology, Ligands, Biochemistry, 03 medical and health sciences, Protein Interaction Domains and Motifs, Binding site, Molecular Biology, chemistry.chemical_classification, Binding Sites, Virulence, Entamoeba histolytica, Cell Biology, General Medicine, Cysteine protease, Cell biology, 030104 developmental biology, Enzyme, chemistry, Protein Conformation, beta-Strand, Protein Binding, Cysteine

Abstract

The number of protein folds in nature is limited, thus is not surprising that proteins with the same fold are able to exert different functions. The cysteine protease inhibitors that adopt an immunoglobulin- like fold (Ig-ICPs) are inhibitors encoded in bacteria and protozoan parasites. Structural studies indicate that these inhibitors resemble the structure of archetypical proteins with an Ig fold, like antibodies, cadherins or cell receptors. The structure of Ig-ICPs from four different protozoan parasites clearly shows the presence of three loops that form part of a protein-ligand interaction surface that resembles the antigen binding sites of antibodies. Thus, Ig-ICPs bind to different cysteine proteases using a tripartite mechanism in which their BC, DE and FG loops are responsible for the main interactions with the target cysteine protease. Ig-ICPs from different protozoan parasites regulate the enzymatic activity of host or parasite's proteases and thus regulate virulence and pathogenesis.

Published

2017

16. Structural Basis for Redox Regulation of Cytoplasmic and Chloroplastic Triosephosphate Isomerases from Arabidopsis thaliana

Author

Carlos H. Trasviña-Arenas, Pedro Jimenez-Sandoval, Noe Baruch-Torres, Luis G. Brieba, Robert Winkler, Corina Diaz-Quezada, Laura Margarita López-Castillo, and Samuel Lara-González

Subjects

Proteomics, 0301 basic medicine, Arabidopsis thaliana, structure-function relationships, thiol-based redox regulation, Plant Science, Isomerase, lcsh:Plant culture, Triosephosphate isomerase, redox regulation, 03 medical and health sciences, chemistry.chemical_compound, Glyceraldehyde, lcsh:SB1-1110, Site-directed mutagenesis, Dihydroxyacetone phosphate, biology, Glutathione, biology.organism_classification, 030104 developmental biology, chemistry, Biochemistry, X-ray structure, glutathionylation, Cysteine

Abstract

In plants triosephosphate isomerase (TPI) interconverts glyceraldehyde 3-phosphate (G3P) and dihydroxyacetone phosphate (DHAP) during glycolysis, gluconeogenesis, and the Calvin-Benson cycle. The nuclear genome of land plants encodes two tpi genes, one gene product is located in the cytoplasm and the other is imported into the chloroplast. Herein we report the crystal structures of the TPIs from the vascular plant Arabidopsis thaliana (AtTPIs) and address their enzymatic modulation by redox agents. Cytoplasmic TPI (cTPI) and chloroplast TPI (pdTPI) share more than 60% amino acid identity and assemble as (β-α)8 dimers with high structural homology. cTPI and pdTPI harbor two and one accessible thiol groups per monomer respectively. cTPI and pdTPI present a cysteine at an equivalent structural position (C13 and C15 respectively) and cTPI also contains a specific solvent accessible cysteine at residue 218 (cTPI-C218). Site directed mutagenesis of residues pdTPI-C15, cTPI-C13, and cTPI-C218 to serine substantially decreases enzymatic activity, indicating that the structural integrity of these cysteines is necessary for catalysis. AtTPIs exhibit differential responses to oxidative agents, cTPI is susceptible to oxidative agents such as diamide and H2O2, whereas pdTPI is resistant to inhibition. Incubation of AtTPIs with the sulfhydryl conjugating reagents methylmethane thiosulfonate (MMTS) and glutathione inhibits enzymatic activity. However, the concentration necessary to inhibit pdTPI is at least two orders of magnitude higher than the concentration needed to inhibit cTPI. Western-blot analysis indicates that residues cTPI-C13, cTPI-C218, and pdTPI-C15 conjugate with glutathione. In summary, our data indicate that AtTPIs could be redox regulated by the derivatization of specific AtTPI cysteines (cTPI-C13 and pdTPI-C15 and cTPI-C218). Since AtTPIs have evolved by gene duplication, the higher resistance of pdTPI to redox agents may be an adaptive consequence to the redox environment in the chloroplast.

Published

2016

17. Structural Basis for Redox Regulation of Cytoplasmic and Chloroplastic Triosephosphate Isomerases from

Author

Laura M, López-Castillo, Pedro, Jiménez-Sandoval, Noe, Baruch-Torres, Carlos H, Trasviña-Arenas, Corina, Díaz-Quezada, Samuel, Lara-González, Robert, Winkler, and Luis G, Brieba

Subjects

triosephosphate isomerase, Arabidopsis thaliana, thiol-based redox regulation, Plant Science, X-ray structure, glutathionylation, Original Research

Abstract

In plants triosephosphate isomerase (TPI) interconverts glyceraldehyde 3-phosphate (G3P) and dihydroxyacetone phosphate (DHAP) during glycolysis, gluconeogenesis, and the Calvin-Benson cycle. The nuclear genome of land plants encodes two tpi genes, one gene product is located in the cytoplasm and the other is imported into the chloroplast. Herein we report the crystal structures of the TPIs from the vascular plant Arabidopsis thaliana (AtTPIs) and address their enzymatic modulation by redox agents. Cytoplasmic TPI (cTPI) and chloroplast TPI (pdTPI) share more than 60% amino acid identity and assemble as (β-α)8 dimers with high structural homology. cTPI and pdTPI harbor two and one accessible thiol groups per monomer respectively. cTPI and pdTPI present a cysteine at an equivalent structural position (C13 and C15 respectively) and cTPI also contains a specific solvent accessible cysteine at residue 218 (cTPI-C218). Site directed mutagenesis of residues pdTPI-C15, cTPI-C13, and cTPI-C218 to serine substantially decreases enzymatic activity, indicating that the structural integrity of these cysteines is necessary for catalysis. AtTPIs exhibit differential responses to oxidative agents, cTPI is susceptible to oxidative agents such as diamide and H2O2, whereas pdTPI is resistant to inhibition. Incubation of AtTPIs with the sulfhydryl conjugating reagents methylmethane thiosulfonate (MMTS) and glutathione inhibits enzymatic activity. However, the concentration necessary to inhibit pdTPI is at least two orders of magnitude higher than the concentration needed to inhibit cTPI. Western-blot analysis indicates that residues cTPI-C13, cTPI-C218, and pdTPI-C15 conjugate with glutathione. In summary, our data indicate that AtTPIs could be redox regulated by the derivatization of specific AtTPI cysteines (cTPI-C13 and pdTPI-C15 and cTPI-C218). Since AtTPIs have evolved by gene duplication, the higher resistance of pdTPI to redox agents may be an adaptive consequence to the redox environment in the chloroplast.

Published

2016

18. Substrate-Induced Dimerization of Engineered Monomeric Variants of Triosephosphate Isomerase from Trichomonas vaginalis

Author

María E. Cruces, Priscilla Estrella, Corina Diaz-Quezada, Carmen J. Portillo, Armando Gómez-Puyou, Ana C. Migliorini-Figueira, Rossana Arroyo, Luis G. Brieba, Claudia G. Benítez-Cardoza, Samuel Lara-González, Eugenia Sánchez-Sandoval, Margarita Lopez-Castillo, Juliana Fattori, Pedro Jimenez-Sandoval, Jaime Ortega-López, Marisol López-Hidalgo, and Carlos H. Trasviña-Arenas

Subjects

Stereochemistry, Dimer, Protein subunit, Molecular Sequence Data, Protozoan Proteins, lcsh:Medicine, Plasma protein binding, Isomerase, Triosephosphate isomerase, chemistry.chemical_compound, Residue (chemistry), Catalytic Domain, Enzyme Stability, Trichomonas vaginalis, Amino Acid Sequence, lcsh:Science, Peptide sequence, Multidisciplinary, lcsh:R, Monomer, chemistry, Biochemistry, lcsh:Q, Protein Multimerization, Protein Binding, Triose-Phosphate Isomerase, Research Article

Abstract

The dimeric nature of triosephosphate isomerases (TIMs) is maintained by an extensive surface area interface of more than 1600 Å2. TIMs from Trichomonas vaginalis (TvTIM) are held in their dimeric state by two mechanisms: a ball and socket interaction of residue 45 of one subunit that fits into the hydrophobic pocket of the complementary subunit and by swapping of loop 3 between subunits. TvTIMs differ from other TIMs in their unfolding energetics. In TvTIMs the energy necessary to unfold a monomer is greater than the energy necessary to dissociate the dimer. Herein we found that the character of residue I45 controls the dimer-monomer equilibrium in TvTIMs. Unfolding experiments employing monomeric and dimeric mutants led us to conclude that dimeric TvTIMs unfold following a four state model denaturation process whereas monomeric TvTIMs follow a three state model. In contrast to other monomeric TIMs, monomeric variants of TvTIM1 are stable and unexpectedly one of them (I45A) is only 29-fold less active than wild-type TvTIM1. The high enzymatic activity of monomeric TvTIMs contrast with the marginal catalytic activity of diverse monomeric TIMs variants. The stability of the monomeric variants of TvTIM1 and the use of cross-linking and analytical ultracentrifugation experiments permit us to understand the differences between the catalytic activities of TvTIMs and other marginally active monomeric TIMs. As TvTIMs do not unfold upon dimer dissociation, herein we found that the high enzymatic activity of monomeric TvTIM variants is explained by the formation of catalytic dimeric competent species assisted by substrate binding.

Published

2015

19. White shrimp Litopenaeus vannamei catalase: gene structure, expression and activity under hypoxia and reoxygenation

Author

Alma B. Peregrino-Uriarte, Antonio García-Triana, Gloria Yepiz-Plascencia, and Carlos H. Trasviña-Arenas

Subjects

Gills, animal structures, Physiology, Molecular Sequence Data, Litopenaeus, medicine.disease_cause, Biochemistry, Gene Expression Regulation, Enzymologic, Penaeidae, medicine, Animals, Humans, Amino Acid Sequence, Molecular Biology, Phylogeny, chemistry.chemical_classification, Reactive oxygen species, Base Sequence, biology, Ecology, fungi, Hypoxia (medical), Catalase, biology.organism_classification, Molecular biology, Introns, Enzyme assay, Shrimp, Oxygen, chemistry, Organ Specificity, biology.protein, Hepatopancreas, medicine.symptom, Oxidative stress

Abstract

Catalase (EC 1.11.1.6) is an antioxidant enzyme involved in redox equilibrium, regulating hydrogen peroxide (H(2)O(2)) concentration, a harmful reactive oxygen species (ROS) that is produced during hypoxia. Hypoxia occurs commonly in aquatic environments and in shrimp farms. We studied the catalase gene of the shrimp Litopenaeus vannamei and tested its expression and enzyme activity during hypoxia (1.5mg/L O(2); 6 and 24h) and reoxygenation (1h after hypoxia). The complete gene is 2974bp long and has four introns of 821, 223, 114 and 298bp, respectively. The first intron has tree microsatellites, with GT and (T)AT(GT) repeated sequences. L. vannamei catalase is part of an invertebrate clade including crustaceans and rotifers. Catalase expression and activity is different in gills and hepatopancreas. Expression in gills increased 3.2 and 3-fold in response to hypoxia and reoxygenation (6 and 24h hypoxia, followed by 1h reoxygenation) compared to normoxia, while no differences were detected in the expression and activity in hepatopancreas. Catalase activity in gills had a contrary response to expression in hypoxia and reoxygenation.