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1.
J Mol Evol, v. 29, n. 2024, 317-328, mai. 2024
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-5430

RESUMEN

Snakes in the family Elapidae largely produce venoms rich in three-fnger toxins (3FTx) that bind to the α1 subunit of nicotinic acetylcholine receptors (nAChRs), impeding ion channel activity. These neurotoxins immobilize the prey by disrupting muscle contraction. Coral snakes of the genus Micrurus are specialist predators who produce many 3FTx, making them an interesting system for examining the coevolution of these toxins and their targets in prey animals. We used a bio-layer interferometry technique to measure the binding interaction between 15 Micrurus venoms and 12 taxon-specifc mimotopes designed to resemble the orthosteric binding region of the muscular nAChR subunit. We found that Micrurus venoms vary greatly in their potency on this assay and that this variation follows phylogenetic patterns rather than previously reported patterns of venom composition. The long-tailed Micrurus tend to have greater binding to nAChR orthosteric sites than their short-tailed relatives and we conclude this is the likely ancestral state. The repeated loss of this activity may be due to the evolution of 3FTx that bind to other regions of the nAChR. We also observed variations in the potency of the venoms depending on the taxon of the target mimotope. Rather than a pattern of prey-specifcity, we found that mimotopes modeled after snake nAChRs are less susceptible to Micrurus venoms and that this resistance is partly due to a characteristic tryptophan→serine mutation within the orthosteric site in all snake mimotopes. This resistance may be part of a Red Queen arms race between coral snakes and their prey.

2.
J. Mol. Evol., v. 92, n. 2024, 317–328, maio 2024
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-5401

RESUMEN

Snakes in the family Elapidae largely produce venoms rich in three-fnger toxins (3FTx) that bind to the α1 subunit of nicotinic acetylcholine receptors (nAChRs), impeding ion channel activity. These neurotoxins immobilize the prey by disrupting muscle contraction. Coral snakes of the genus Micrurus are specialist predators who produce many 3FTx, making them an interesting system for examining the coevolution of these toxins and their targets in prey animals. We used a bio-layer interferometry technique to measure the binding interaction between 15 Micrurus venoms and 12 taxon-specifc mimotopes designed to resemble the orthosteric binding region of the muscular nAChR subunit. We found that Micrurus venoms vary greatly in their potency on this assay and that this variation follows phylogenetic patterns rather than previously reported patterns of venom composition. The long-tailed Micrurus tend to have greater binding to nAChR orthosteric sites than their short-tailed relatives and we conclude this is the likely ancestral state. The repeated loss of this activity may be due to the evolution of 3FTx that bind to other regions of the nAChR. We also observed variations in the potency of the venoms depending on the taxon of the target mimotope. Rather than a pattern of prey-specifcity, we found that mimotopes modeled after snake nAChRs are less susceptible to Micrurus venoms and that this resistance is partly due to a characteristic tryptophan→serine mutation within the orthosteric site in all snake mimotopes. This resistance may be part of a Red Queen arms race between coral snakes and their prey.

3.
Toxins, v. 15, n. 7, 415, jun. 2023
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-4974

RESUMEN

Snakes of the Philodryadini tribe are included in the Dipsadidae family, which is a diverse group of rear-fanged snakes widespread in different ecological conditions, including habitats and diet. However, little is known about the composition and effects of their venoms despite their relevance for understanding the evolution of these snakes or even their impact on the occasional cases of human envenoming. In this study, we integrated venom gland transcriptomics, venom proteomics and functional assays to characterize the venoms from eight species of the Philodryadini tribe, which includes the genus Philodryas, Chlorosoma and Xenoxybelis. The most abundant components identified in the venoms were snake venom metalloproteinases (SVMPs), cysteine-rich secretory proteins (CRISPs), C-type lectins (CTLs), snake endogenous matrix metalloproteinases type 9 (seMMP-9) and snake venom serinoproteinases (SVSPs). These protein families showed a variable expression profile in each genus. SVMPs were the most abundant components in Philodryas, while seMMP-9 and CRISPs were the most expressed in Chlorosoma and Xenoxybelis, respectively. Lineage-specific differences in venom composition were also observed among Philodryas species, whereas P. olfersii presented the highest amount of SVSPs and P. agassizii was the only species to express significant amounts of 3FTx. The variability observed in venom composition was confirmed by the venom functional assays. Philodryas species presented the highest SVMP activity, whereas Chlorosoma species showed higher levels of gelatin activity, which may correlate to the seMMP-9 enzymes. The variability observed in the composition of these venoms may be related to the tribe phylogeny and influenced by their diets. In the presented study, we expanded the set of venomics studies of the Philodryadini tribe, which paves new roads for further studies on the evolution and ecology of Dipsadidae snakes.

4.
Syst Biol, v. 20, n. 1, p. 1-25, jan. 2022
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-4119

RESUMEN

Brazilian continental islands represent a natural laboratory to study speciation driven by recent phenotypic and genotypic divergence. The Bothrops jararaca species group is distributed in the Brazilian Atlantic Forest and on most of the Brazilian continental islands. The group is currently composed of the mainland common lancehead (B. jararaca) and four insular species (B. alcatraz, B. insularis, B. otavioi, and B. sazimai). Here, we evaluate mitochondrial DNA and morphological diversity of the B. jararaca species group and aim to provide additional evidence to understand insularization processes on the Brazilian coast. Our results, interpreted together with a comprehensive review of geomorphological data, provide a new conceptual framework for understanding the colonization process of the Brazilian continental islands. This framework suggests a history of multiple rounds of periodic isolation and reconnection between insular populations and their mainland relatives throughout the last 420,000 years. Furthermore, although some insular populations may have speciated prior to the last glacial maximum, other species likely diverged within the last 11,000 years. Additionally, the repeated evolution of size and dietary shift in the B. jararaca species group suggests a remarkable case of convergent adaptation. Our study provides evidence that the Bothrops from Ilha da Moela (Brazilian state of São Paulo) represents an undescribed species, presenting a distinct phenotype, and an exclusive history of isolation and adaptation. We describe this unique lancehead as a new species and we suggest it should be listed as critically endangered based on its endemicity to a small island that is severely impacted by constant and longstanding human presence.

5.
Toxicol Lett, v. 337, p. 91-97, fev. 2021
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-3309

RESUMEN

Snakebite is a neglected tropical disease with a massive global burden of injury and death. The best current treatments, antivenoms, are plagued by a number of logistical issues that limit supply and access in remote or poor regions. We explore the anticoagulant properties of venoms from the genus Micrurus (coral snakes), which have been largely unstudied, as well as the effectiveness of antivenom and a small-molecule phospholipase inhibitor—varespladib—at counteracting these effects. Our in vitro results suggest that these venoms likely interfere with the formation or function of the prothrombinase complex. We find that the anticoagulant potency varies widely across the genus and is especially pronounced in M. laticollaris. This variation does not appear to correspond to previously described patterns regarding the relative expression of the three-finger toxin and phospholipase A2 (PLA2) toxin families within the venoms of this genus. The coral snake antivenom Coralmyn, is largely unable to ameliorate these effects except for M. ibiboboca. Varespladib on the other hand completely abolished the anticoagulant activity of every venom. This is consistent with the growing body of results showing that varespladib may be an effective treatment for a wide range of toxicity caused by PLA2 toxins from many different snake species. Varespladib is a particularly attractive candidate to help alleviate the burden of snakebite because it is an approved drug that possesses several logistical advantages over antivenom including temperature stability and oral availability.

6.
PLoS Negl Trop Dis ; 14(6): e0008299, 2020 06.
Artículo en Inglés | MEDLINE | ID: mdl-32511239

RESUMEN

Snake venoms are complex mixtures of proteins with toxic activities, with many distinct isoforms, affecting different physiological targets, comprised in a few protein families. It is currently accepted that this diversity in venom composition is an adaptive advantage for venom efficacy on a wide range of prey. However, on the other side, variability on isoforms expression has implications in the clinics of human victims of snakebites and in the efficacy of antivenoms. B. atrox snakes are responsible for most of the human accidents in Brazilian Amazon and the type and abundance of protein families on their venoms present individual variability. Thus, in this study we attempted to correlate the individual venom proteome of the snake brought to the hospital by the patient seeking for medical assistance with the clinical signs observed in the same patient. Individual variability was confirmed in venoms of the 14 snakes selected for the study. The abundance of each protein family was quite similar among the venom samples, while the isoforms composition was highly variable. Considering the protein families, the SVMP group presented the best correlation with bleeding disorders and edema. Considering individual isoforms, some isoforms of venom metalloproteinase (SVMP), C-type lectin-like toxins (CTL) and snake venom serine proteinases (SVSP) presented expression levels that with statistically significant positive correlation to signs and symptoms presented by the patients as bleeding disorders, edema, ecchymosis and blister formation. However, some unexpected data were also observed as the correlation between a CTL, CRISP or LAAO isoforms with blister formation, still to be confirmed with a larger number of samples. Although this is still a small number of patient samples, we were able to indicate that venom composition modulates clinical manifestations of snakebites, to confirm at the bedside the prominent role of SVMPs and to include new possible toxin candidates for the development of toxin inhibitors or to improve antivenom selectiveness, important actions for the next generation treatments of snakebites.


Asunto(s)
Bothrops , Venenos de Crotálidos/análisis , Proteoma/análisis , Serina Proteasas/análisis , Animales , Antivenenos , Brasil , Metaloproteasas/análisis , Isoformas de Proteínas/análisis , Proteómica , Mordeduras de Serpientes/terapia
7.
Toxins, v. 12, n. 12, 791, dez. 2020
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-3414

RESUMEN

Ontogenetic changes in venom composition have been described in Bothrops snakes, but only a few studies have attempted to identify the targeted paralogues or the molecular mechanisms involved in modifications of gene expression during ontogeny. In this study, we decoded B. jararacussu venom gland transcripts from six specimens of varying sizes and analyzed the variability in the composition of independent venom proteomes from 19 individuals. We identified 125 distinct putative toxin transcripts, and of these, 73 were detected in venom proteomes and only 10 were involved in the ontogenetic changes. Ontogenetic variability was linearly related to snake size and did not correspond to the maturation of the reproductive stage. Changes in the transcriptome were highly predictive of changes in the venom proteome. The basic myotoxic phospholipases A2 (PLA2s) were the most abundant components in larger snakes, while in venoms from smaller snakes, PIII-class SVMPs were the major components. The snake venom metalloproteinases (SVMPs) identified corresponded to novel sequences and conferred higher pro-coagulant and hemorrhagic functions to the venom of small snakes. The mechanisms modulating venom variability are predominantly related to transcriptional events and may consist of an advantage of higher hematotoxicity and more efficient predatory function in the venom from small snakes.

8.
Int J Mol Sci, v. 21, n. 19, 7377, out. 2020
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-3272

RESUMEN

The evolution of an aquatic lifestyle from land dwelling venomous elapids is a radical ecological modification, bringing about many evolutionary changes from morphology to diet. Diet is an important ecological facet which can play a key role in regulating functional traits such as venom composition and prey-specific targeting of venom. In addition to predating upon novel prey (e.g., fish, fish eggs and invertebrates), the venoms of aquatic elapids also face the challenge of increased prey-escape potential in the aquatic environment. Thus, despite the independent radiation into an aquatic niche on four separate occasions, the venoms of aquatic elapids are evolving under convergent selection pressures. Utilising a biolayer interferometry binding assay, this study set out to elucidate whether crude venoms from representative aquatic elapids were target-specific to the orthosteric site of postsynaptic nicotinic acetylcholine receptor mimotopes of fish compared to other terrestrial prey types. Representatives of the four aquatic lineages were: aquatic coral snakes representative was Micrurus surinamensis;, sea kraits representative was Laticauda colubrina; sea snakes representatives were two Aipysurus spp. and eight Hydrophis spp; and water cobras representative was Naja annulata. No prey-specific differences in crude venom binding were observed from any species tested, except for Aipysurus laevis, which showed slight evidence of prey-potency differences. For Hydrophis caerulescens, H. peronii, H. schistosus and M. surinamensis, there was a lack of binding to the orthosteric site of any target lineage. Subsequent testing on the in vitro chick-biventer cervicis muscle preparation suggested that, while the venoms of these species bound postsynaptically, they bound to allosteric sites rather than orthosteric. Allosteric binding is potentially a weaker but faster-acting form of neurotoxicity and we hypothesise that the switch to allosteric binding is likely due to selection pressures related to prey-escape potential. This research has potentially opened up the possibility of a new functional class of toxins which have never been assessed previously while shedding light on the selection pressures shaping venom evolution.

9.
PLoS Negl Trop Dis, v. 14, n. 6, e0008299, jun. 2020
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-3060

RESUMEN

Snake venoms are complex mixtures of proteins with toxic activities, with many distinct isoforms, affecting different physiological targets, comprised in a few protein families. It is currently accepted that this diversity in venom composition is an adaptive advantage for venom efficacy on a wide range of prey. However, on the other side, variability on isoforms expression has implications in the clinics of human victims of snakebites and in the efficacy of antivenoms. B. atrox snakes are responsible for most of the human accidents in Brazilian Amazon and the type and abundance of protein families on their venoms present individual variability. Thus, in this study we attempted to correlate the individual venom proteome of the snake brought to the hospital by the patient seeking for medical assistance with the clinical signs observed in the same patient. Individual variability was confirmed in venoms of the 14 snakes selected for the study. The abundance of each protein family was quite similar among the venom samples, while the isoforms composition was highly variable. Considering the protein families, the SVMP group presented the best correlation with bleeding disorders and edema. Considering individual isoforms, some isoforms of venom metalloproteinase (SVMP), C-type lectin-like toxins (CTL) and snake venom serine proteinases (SVSP) presented expression levels that with statistically significant positive correlation to signs and symptoms presented by the patients as bleeding disorders, edema, ecchymosis and blister formation. However, some unexpected data were also observed as the correlation between a CTL, CRISP or LAAO isoforms with blister formation, still to be confirmed with a larger number of samples. Although this is still a small number of patient samples, we were able to indicate that venom composition modulates clinical manifestations of snakebites, to confirm at the bedside the prominent role of SVMPs and to include new possible toxin candidates for the development of toxin inhibitors or to improve antivenom selectiveness, important actions for the next generation treatments of snakebites.

10.
Toxins (Basel) ; 10(3)2018 03 13.
Artículo en Inglés | MEDLINE | ID: mdl-29533989

RESUMEN

Despite numerous studies concerning morphology and venom production and secretion in the main venom gland (and some data on the accessory gland) of the venom glandular apparatus of Viperidae snakes, the primary duct has been overlooked. We characterized the primary duct of the Bothrops jararaca snake by morphological analysis, immunohistochemistry and proteomics. The duct has a pseudostratified epithelium with secretory columnar cells with vesicles of various electrondensities, as well as mitochondria-rich, dark, basal, and horizontal cells. Morphological analysis, at different periods after venom extraction, showed that the primary duct has a long cycle of synthesis and secretion, as do the main venom and accessory glands; however, the duct has a mixed mode venom storage, both in the lumen and in secretory vesicles. Mouse anti-B. jararaca venom serum strongly stained the primary duct's epithelium. Subsequent proteomic analysis revealed the synthesis of venom toxins-mainly C-type lectin/C-type lectin-like proteins. We propose that the primary duct's toxin synthesis products complement the final venom bolus. Finally, we hypothesize that the primary duct and the accessory gland (components of the venom glandular apparatus) are part of the evolutionary path from a salivary gland towards the main venom gland.


Asunto(s)
Bothrops/metabolismo , Venenos de Crotálidos/metabolismo , Glándulas Exocrinas/metabolismo , Animales , Bothrops/anatomía & histología , Glándulas Exocrinas/anatomía & histología , Glándulas Exocrinas/ultraestructura , Femenino , Microscopía Electrónica de Transmisión , Proteómica , Proteínas de Reptiles/metabolismo
11.
J Proteomics ; 177: 137-147, 2018 04 15.
Artículo en Inglés | MEDLINE | ID: mdl-29325991

RESUMEN

In Viperidae snakes, it has been attributed to the main venom gland, a component of the venom gland apparatus, the function of synthesizing all venom toxins and storing them inside a basal-central lumen. However, the role of the accessory gland is still unknown. Here, we analyzed the proteome and the transcriptome of the accessory gland during venom production and secretion cycle. We showed that the accessory gland expresses and synthesizes toxins that are similar to those produced by the main venom gland such as C-type lectin/C-type lectin-like proteins, metalloproteinase, phospholipase A2, cysteine rich secretory protein, nerve growth factor, vascular endothelial growth factor, serine proteinase, and l-amino acid oxidase. Our data have shown that toxin synthesis in the accessory gland is asynchronous when compared to the same process in the venom gland. Moreover, this gland also expresses inhibitors of venom phospholipases A2 and metalloproteinases. Transcriptome analysis showed that the transcripts that correspond to toxins in the accessory gland have a good correlation to the main venom gland transcripts. Therefore, it is proposed that the accessory gland is an ancillary source of toxins to the snake, and provides inhibitors that could control venom toxicity (and integrity) during storage. SIGNIFICANCE: In this study, we propose that the accessory venom gland acts as an important ancillary source of toxins to the snake, in lieu of a depleted main venom gland, and provides inhibiting agents that control venom toxicity (and integrity) during its storage.


Asunto(s)
Bothrops/fisiología , Venenos de Crotálidos/biosíntesis , Proteoma/análisis , Animales , Venenos de Crotálidos/antagonistas & inhibidores , Glándulas Exocrinas/química , Perfilación de la Expresión Génica , Metaloproteasas/antagonistas & inhibidores , Metaloproteasas/biosíntesis , Metaloproteasas/metabolismo , Inhibidores de Fosfolipasa A2/metabolismo , Fosfolipasas A2/biosíntesis , Fosfolipasas A2/metabolismo
12.
J Proteomics, v. 177, p. 137-147, abr. 2018
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-2506

RESUMEN

In Viperidae snakes, it has been attributed to the main venom gland, a component of the venom gland apparatus, the function of synthesizing all venom toxins and storing them inside a basal-central lumen. However, the role of the accessory gland is still unknown. Here, we analyzed the proteome and the transcriptome of the accessory gland during venom production and secretion cycle. We showed that the accessory gland expresses and synthesizes toxins that are similar to those produced by the main venom gland such as C-type lectin/C-type lectin-like proteins, metalloproteinase, phospholipase A(2), cysteine rich secretory protein, nerve growth factor, vascular endothelial growth factor, serine proteinase, and L-amino acid oxidase. Our data have shown that toxin synthesis in the accessory gland is asynchronous when compared to the same process in the venom gland. Moreover, this gland also expresses inhibitors of venom phospholipases A(2) and metalloproteinases. Transcriptome analysis showed that the transcripts that correspond to toxins in the accessory gland have a good correlation to the main venom gland transcripts. Therefore, it is proposed that the accessory gland is an ancillary source of toxins to the snake, and provides inhibitors that could control venom toxicity (and integrity) during storage. Significance: In this study, we propose that the accessory venom gland acts as an important ancillary source of toxins to the snake, in lieu of a depleted main venom gland, and provides inhibiting agents that control venom toxicity (and integrity) during its storage.

13.
J Proteomics, v. 181, p. 60-72, jun. 2018
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-2482

RESUMEN

Elucidating the molecular mechanisms underlying snake venom variability provides important clues for understanding how the biological functions of this powerful toxic arsenal evolve. We analyzed in detail individual transcripts and venom protein isoforms produced by five specimens of a venomous snake (Bothrops atrox) from two nearby but genetically distinct populations from the Brazilian Amazon rainforest which show functional similarities in venom properties. Individual variation was observed among the venoms of these specimens, but the overall abundance of each general toxin family was conserved both in transcript and in venom protein levels. However, when expression of independent paralogues was analyzed, remarkable differences were observed within and among each toxin group, both between individuals and between populations. Transcripts for functionally essential venom proteins ("core function" proteins) were highly expressed in all specimens and showed similar transcription/translation rates. In contrast, other paralogues ("adaptive" proteins) showed lower expression levels and the toxins they coded for varied among different individuals. These results provide support for the inferences that (a) expression and translational differences play a greater role in defining adaptive variation in venom phenotypes than does sequence variation in protein coding genes and (b) convergent adaptive venom phenotypes can be generated through different molecular mechanisms. Significance: Analysis of individual transcripts and venom protein isoforms produced by specimens of a venomous snake (Bothrops atrox), from the Brazilian Amazon rainforest, revealed that transcriptional and translational mechanisms contribute to venom phenotypic variation. Our finding of evidence for high expression of toxin proteins with conserved function supports the hypothesis that the venom phenotype consists of two kinds of proteins: conserved "core function" proteins that provide essential functional activities with broader relevance and less conserved "adaptive" proteins that vary in expression and may permit customization of protein function. These observations allowed us to suggest that genetic mechanisms controlling venom variability are not restricted to selection of gene copies or mutations in structural genes but also to selection of the mechanisms controlling gene expression, contributing to the plasticity of this important phenotype for venomous snakes.

14.
Toxins, v. 10, n. 3, 121, mar. 2018
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-2479

RESUMEN

Despite numerous studies concerning morphology and venom production and secretion in the main venom gland (and some data on the accessory gland) of the venom glandular apparatus of Viperidae snakes, the primary duct has been overlooked. We characterized the primary duct of the Bothrops jararaca snake by morphological analysis, immunohistochemistry and proteomics. The duct has a pseudostratified epithelium with secretory columnar cells with vesicles of various electrondensities, as well as mitochondria-rich, dark, basal, and horizontal cells. Morphological analysis, at different periods after venom extraction, showed that the primary duct has a long cycle of synthesis and secretion, as do the main venom and accessory glands; however, the duct has a mixed mode venom storage, both in the lumen and in secretory vesicles. Mouse anti-B. jararaca venom serum strongly stained the primary duct’s epithelium. Subsequent proteomic analysis revealed the synthesis of venom toxins—mainly C-type lectin/C-type lectin-like proteins. We propose that the primary duct’s toxin synthesis products complement the final venom bolus. Finally, we hypothesize that the primary duct and the accessory gland (components of the venom glandular apparatus) are part of the evolutionary path from a salivary gland towards the main venom gland.

15.
São Paulo; 2014. 129 p.
Tesis en Portugués | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP | ID: bud-3269

RESUMEN

The zinc-dependent metalloproteinases include families of proteins with essential function for homeostasis such as MMPs and ADAMs. These enzymes are involved in a wide variety of biological processes ranging from physiological cell proliferation and differentiation to pathological states associated with tumor metastasis, inflammation, tissue degeneration, and cell death. Snake Venom Metalloproteinases (SVMPs) are also zinc-dependent enzymes abundant in venoms of viper snakes. SVMPs are responsible for most local and systemic symptoms of human envenomings. As MMPs and ADAMs, SVMPs are synthesized as zymogens and the enzyme activation is regulated by hydrolysis of its pro-domain. However, very little is known about activation of SVMPs and where the hydrolysis of the pro-domain occurs. In this study, we attempted to identify and quantify the presence of pro-domains in different compartments of snake venom glands as zymogens or at free form, in order to enlighten some mechanism involved in SVMP activation. For this purpose, the prodomain of jararhagin (PD-Jar), a SVMP prevailing in the venom of Bothrops jararaca, was obtained in its recombinant form and used to immunize mice and rabbits to obtain antibodies specific to SVMP pro-domains, which were tested with samples of venom or glands tissues collected in different periods of the venom production cycle. By Western blotting, bands of 22 and 45 kDa, that correspond respectively to free pro-domains or zymogen of P-I SVMPs expected mobilities, were revealed in venom samples collected 4, 7 and 10 days after stimulus of venom production cycle. In venom glands, bands of zymogen molecular masses were detected in tissue extracts all along the cycle, but on the venom collected from the lumen these high molecularmass bands were detected only at the peak of venom production and not at the quiescent state. The antigens recognized by Western blots were immunoprecipitated with anti-PD-Jar and subjected to MS/MS. Pro-domain peptides were identified in all samples together with a few venom proteins that co-precipitated with SVMPs and the Glutamyl Peptide Cyclotransferase, involved in SVMP post-translational processing. In order to identify the location of these molecules within the venom secretory apparatus, gland tissues were submitted to immunofluorescence andimmunoelectronmicroscopy analysis. The results show positive staining of prodomain in secretory cells majorly at the secretory vesicles near the Golgi in the active glands. Taken together, our data shows that processing of SVMPs starts within secretory vesicles of venom gland secretory cells and occurs predominantly at the lumen of the venom gland just after the enzyme secretion. As such, SVMPactivation differs from ADAMs and MMPs, but can be used as a model for studying the relevance of peptides resulting from pro-domain processing and degradation for the control of metalloproteinases activity.


Metaloproteinases incluem famílias de proteínas com funções essenciais para a homeostase em diferentes seres vivos, tais como as MMPs e ADAMs. Estas enzimas estão envolvidas em uma grande variedade de processos biológicos tanto fisiológicos, como proliferação e diferenciação celular, quanto estados patológicos associados com a metástase de tumores, inflamação, degeneração de tecidos e morte celular. Metaloproteinases do veneno de serpentes (SVMPs) também são enzimas dependentes de zinco abundantes em venenos de serpentes. SVMPs são responsáveis pela maioria dos sintomas locais e sistêmicos do envenenamento humano. Tal como as MMPs e ADAMs, as SVMPs são sintetizadas como zimogênios e a ativação da enzima é regulada por meio de hidrólise do seu pródomínio. No entanto, muito pouco se sabe sobre a ativação de SVMPs e onde a hidrólise do pró-domínio ocorre. Neste estudo, buscou-se identificar e quantificar a presença de pró-domínios como zimogênios ou de forma livre em diferentes compartimentos da glândula de veneno, a fim de esclarecer alguns mecanismos envolvidos na ativação da SMVP. Para esta finalidade, o pró-domínio da jararagina (PD-Jar), uma SVMP prevalente no veneno de Bothrops jararaca, foi obtido na sua forma recombinante e usado para imunizar camundongos e coelhos para a obtenção de anticorpos anti-pró- omínio que foram testados com amostras de veneno ou glândulas coletadas em diferentes períodos do ciclo de produção de veneno. Por western blotting, as bandas de 22 e 45 kDa, que correspondem, respectivamente, ao pró-domínio livre e ao zimogênio de SVMP de classe P-I, foram revelados em amostras de veneno coletadas 4, 7 e 10 dias após o estímulo do ciclo de produção de veneno. No veneno coletado a partir do lúmen, bandas de alta massa molecular foram detectadas apenas no pico da produção de veneno e não no estado quiescente. Em glândulas de veneno, foram detectadas predominantemente as bandas de massas moleculares de zimogênios, em tecidos extraídos ao longo do ciclo. Os antígenos reconhecidos por Western blotting foram imunoprecipitados com anticorpo anti-PD-Jar e submetidos a MS/MS. Peptídeos de pró-domínio foram identificados em todas as amostras, juntamente com algumas proteínas do veneno que foram co-precipitadas e também o GPC (glutamyl peptide cyclotransferase), que está envolvido em processamentos pós-traducionais das SMVPs. A fim de identificar a localização destas moléculas no interior da glândula de veneno, os tecidos das glândulas foram submetidos à análise por imunofluorescência e imunoeletromicroscopia. Os resultados mostram a coloração positiva de pró-domínio em células secretoras majoritariamente nas vesículas secretoras perto do Golgi. Tomados em conjunto, os nossos dados mostram que o processamento das SVMPs começa dentro de vesículas secretoras de veneno das células secretoras e ocorre predominantemente no lúmen da glândula de veneno após a secreção das enzimas. Como tal, a ativação das SMVPs difere de ADAMs e MMPs, mas pode ser utilizado como um modelo para o estudo da relevância dos peptídeos resultantes do processamento e degradação do pró-domínio para o controle da atividade de metaloproteinases.

16.
PLoS Negl Trop Dis ; 7(9): e2442, 2013.
Artículo en Inglés | MEDLINE | ID: mdl-24069493

RESUMEN

In Latin America, Bothrops snakes account for most snake bites in humans, and the recommended treatment is administration of multispecific Bothrops antivenom (SAB--soro antibotrópico). However, Bothrops snakes are very diverse with regard to their venom composition, which raises the issue of which venoms should be used as immunizing antigens for the production of pan-specific Bothrops antivenoms. In this study, we simultaneously compared the composition and reactivity with SAB of venoms collected from six species of snakes, distributed in pairs from three distinct phylogenetic clades: Bothrops, Bothropoides and Rhinocerophis. We also evaluated the neutralization of Bothrops atrox venom, which is the species responsible for most snake bites in the Amazon region, but not included in the immunization antigen mixture used to produce SAB. Using mass spectrometric and chromatographic approaches, we observed a lack of similarity in protein composition between the venoms from closely related snakes and a high similarity between the venoms of phylogenetically more distant snakes, suggesting little connection between taxonomic position and venom composition. P-III snake venom metalloproteinases (SVMPs) are the most antigenic toxins in the venoms of snakes from the Bothrops complex, whereas class P-I SVMPs, snake venom serine proteinases and phospholipases A2 reacted with antibodies in lower levels. Low molecular size toxins, such as disintegrins and bradykinin-potentiating peptides, were poorly antigenic. Toxins from the same protein family showed antigenic cross-reactivity among venoms from different species; SAB was efficient in neutralizing the B. atrox venom major toxins. Thus, we suggest that it is possible to obtain pan-specific effective antivenoms for Bothrops envenomations through immunization with venoms from only a few species of snakes, if these venoms contain protein classes that are representative of all species to which the antivenom is targeted.


Asunto(s)
Antivenenos/metabolismo , Bothrops/clasificación , Bothrops/genética , Filogenia , Venenos de Serpiente/análisis , Venenos de Serpiente/toxicidad , Animales , Antivenenos/inmunología , Cromatografía , Reacciones Cruzadas , Femenino , Humanos , América Latina , Masculino , Espectrometría de Masas , Ratones , Pruebas de Neutralización , Venenos de Serpiente/inmunología
17.
BMC Genet ; 12: 94, 2011 Nov 01.
Artículo en Inglés | MEDLINE | ID: mdl-22044657

RESUMEN

BACKGROUND: Snake venom metalloproteinases (SVMPs) are widely distributed in snake venoms and are versatile toxins, targeting many important elements involved in hemostasis, such as basement membrane proteins, clotting proteins, platelets, endothelial and inflammatory cells. The functional diversity of SVMPs is in part due to the structural organization of different combinations of catalytic, disintegrin, disintegrin-like and cysteine-rich domains, which categorizes SVMPs in 3 classes of precursor molecules (PI, PII and PIII) further divided in 11 subclasses, 6 of them belonging to PII group. This heterogeneity is currently correlated to genetic accelerated evolution and post-translational modifications. RESULTS: Thirty-one SVMP cDNAs were full length cloned from a single specimen of Bothrops neuwiedi snake, sequenced and grouped in eleven distinct sequences and further analyzed by cladistic analysis. Class P-I and class P-III sequences presented the expected tree topology for fibrinolytic and hemorrhagic SVMPs, respectively. In opposition, three distinct segregations were observed for class P-II sequences. P-IIb showed the typical segregation of class P-II SVMPs. However, P-IIa grouped with class P-I cDNAs presenting a 100% identity in the 365 bp at their 5' ends, suggesting post-transcription events for interclass recombination. In addition, catalytic domain of P-IIx sequences segregated with non-hemorrhagic class P-III SVMPs while their disintegrin domain grouped with other class P-II disintegrin domains suggesting independent evolution of catalytic and disintegrin domains. Complementary regions within cDNA sequences were noted and may participate in recombination either at DNA or RNA levels. Proteins predicted by these cDNAs show the main features of the correspondent classes of SVMP, but P-IIb and P-IIx included two additional cysteines cysteines at the C-termini of the disintegrin domains in positions not yet described. CONCLUSIONS: In B. neuwiedi venom gland, class P-II SVMPs were represented by three different types of transcripts that may have arisen by interclass recombination with P-I and P-III sequences after the divergence of the different classes of SVMPs. Our observations indicate that exon shuffling or post-transcriptional mechanisms may be driving these recombinations generating new functional possibilities for this complex group of snake toxins.


Asunto(s)
Bothrops/genética , Variación Genética , Metaloproteasas/genética , Venenos de Serpiente/genética , Secuencia de Aminoácidos , Animales , Secuencia de Bases , Dominio Catalítico/genética , Clonación Molecular , ADN Complementario , Metaloproteasas/química , Metaloproteasas/metabolismo , Filogenia , Procesamiento Proteico-Postraduccional , Recombinación Genética , Alineación de Secuencia , Análisis de Secuencia de ADN , Venenos de Serpiente/metabolismo
18.
BMC genet. (Online) ; BMC genet. (Online);1(12-94): 1-14, 2011.
Artículo en Inglés | Sec. Est. Saúde SP, SESSP-IBPROD, Sec. Est. Saúde SP, SESSP-IBACERVO | ID: biblio-1060408

RESUMEN

Snake venom metalloproteinases (SVMPs) are widely distributed in snake venoms and are versatiletoxins, targeting many important elements involved in hemostasis, such as basement membrane proteins, clottingproteins, platelets, endothelial and inflammatory cells. The functional diversity of SVMPs is in part due to thestructural organization of different combinations of catalytic, disintegrin, disintegrin-like and cysteine-rich domains,which categorizes SVMPs in 3 classes of precursor molecules (PI, PII and PIII) further divided in 11 subclasses, 6 ofthem belonging to PII group. This heterogeneity is currently correlated to genetic accelerated evolution and posttranslationalmodifications. Thirty-one SVMP cDNAs were full length cloned from a single specimen of Bothrops neuwiedi snake,sequenced and grouped in eleven distinct sequences and further analyzed by cladistic analysis. Class P-I and classP-III sequences presented the expected tree topology for fibrinolytic and hemorrhagic SVMPs, respectively. Inopposition, three distinct segregations were observed for class P-II sequences. P-IIb showed the typical segregationof class P-II SVMPs. However, P-IIa grouped with class P-I cDNAs presenting a 100% identity in the 365 bp at their5’ ends, suggesting post-transcription events for interclass recombination. In addition, catalytic domain of P-IIxsequences segregated with non-hemorrhagic class P-III SVMPs while their disintegrin domain grouped with otherclass P-II disintegrin domains suggesting independent evolution of catalytic and disintegrin domains.Complementary regions within cDNA sequences were noted and may participate in recombination either at DNAor RNA levels.


Asunto(s)
Animales , Metaloproteasas/clasificación , Serpientes/clasificación , Venenos de Serpiente
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