Please use this identifier to cite or link to this item: http://hdl.handle.net/10553/122190
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dc.contributor.authorCardona Machado, Cristian David-
dc.contributor.authorAlarcón Torrecillas, Claudia-
dc.contributor.authorPericacho, Miguel-
dc.contributor.authorRodríguez Escolar, Ivan-
dc.contributor.authorCarretón Gómez, Elena-
dc.contributor.authorMontoya Alonso, José Alberto-
dc.contributor.authorMorchón, Rodrigo-
dc.date.accessioned2023-05-03T10:32:05Z-
dc.date.available2023-05-03T10:32:05Z-
dc.date.issued2023-
dc.identifier.issn0304-4017-
dc.identifier.otherScopus-
dc.identifier.urihttp://hdl.handle.net/10553/122190-
dc.description.abstractAngiogenesis is a process by which new vessels are formed from pre-existing ones when the hysiological conditions of the vascular endothelium are altered. Heartworm disease, caused by Dirofilaria immitis, causes changes in the vascular endothelium of the pulmonary arteries due to obstruction, friction, and hypoxia. The aim of this study was to analyze whether the excretory/secretory and surface-associated antigens of adult worms interact and modulates the angiogenic mechanism, viable cell number and cell migration, as well as the formation of pseudo-capillaries. Cultures of human vascular endothelial cells (HUVECs) stimulated with excretory/secretory antigens (DiES), surface-associated antigens (Cut) from D. immitis adult worms, VEFG-A (Vascular Endothelial Growth Factor A), as well as DiES+VEFG-A and Cut+VEFG-A were used. The production of VEFG-A and other proangiogenic [soluble VEFGR-2 (sVEFGR-2), membrane Endoglin (mEndoglin)] and antiangiogenic [VEFGR-1/soluble Flt (sFlt), soluble Endoglin (sEndoglin)] molecules was assessed using commercial ELISA kits. Cell viability was analyzed by live cell count and cytotoxicity assays by a commercial kit. In addition, viable cell number by MTT-based assay, cell migration by wound-healing assay carrying out scratched wounds, and the capacity of pseudo-capillary formation to analyze cell connections and cell groups in Matrigel cell cultures, were evaluated. In all cases, non‑stimulated cultures were used as controls. DiES+VEFG-A and Cut+VEFG-A significantly increased the production of VEFG-A and sVEFGR-2, and only Cut+VEFG-A significantly increased the production of VEFGR-1/sFlt compared to other groups and non-stimulated cultures. Moreover, only DiES+VEFG- A produced a significant increase in viable cell number and significant decrease cell migration, as well as in the organization and number of cell connections. Excretory/secretory and surface-associated antigens of adult D. immitis activated the angiogenic mechanism by mainly stimulating the synthesis of proangiogenic factors, and only excretory/secretory antigens increased viable cell number, activated cell migration and the formation of pseudo-capillaries. These processes could lead to vascular endothelial remodeling of the infected host and favor the long-term survival of the parasite.-
dc.languageeng-
dc.relation.ispartofVeterinary Parasitology-
dc.sourceVeterinary Parasitology [ISSN 0304-4017], v. 318, 109939, (Junio 2023)-
dc.subject240112 Parasitología animal-
dc.subject310904 Medicina interna-
dc.subject.otherAngiogenesis-
dc.subject.otherExcretory/secretory antigens-
dc.subject.otherSurface-associated antigens-
dc.subject.otherAdult Dirofilaria immitis worms-
dc.subject.otherCell proliferation and migration-
dc.subject.otherPseudo-capillary formation-
dc.titleInvolvement of the excretory/secretory and surface-associated antigens of Dirofilaria immitis adult worms in the angiogenic response in an in-vitro endothelial cell model-
dc.typeinfo:eu-repo/semantics/article-
dc.typeArticle-
dc.identifier.doi10.1016/j.vetpar.2023.109939-
dc.identifier.scopus85153606014-
dc.contributor.orcidNO DATA-
dc.contributor.orcidNO DATA-
dc.contributor.orcidNO DATA-
dc.contributor.orcidNO DATA-
dc.contributor.orcidNO DATA-
dc.contributor.orcidNO DATA-
dc.contributor.orcidNO DATA-
dc.contributor.authorscopusid58138883700-
dc.contributor.authorscopusid57415433200-
dc.contributor.authorscopusid12242328100-
dc.contributor.authorscopusid57390862000-
dc.contributor.authorscopusid36143929200-
dc.contributor.authorscopusid6504331949-
dc.contributor.authorscopusid6507293463-
dc.identifier.eissn1873-2550-
dc.relation.volume318-
dc.investigacionCiencias de la Salud-
dc.type2Artículo-
dc.description.numberofpages8-
dc.utils.revision-
dc.date.coverdateJunio 2023-
dc.identifier.ulpgc-
dc.contributor.buulpgcBU-VET-
dc.description.sjr0,732-
dc.description.jcr2,6-
dc.description.sjrqQ1-
dc.description.jcrqQ1-
dc.description.scieSCIE-
dc.description.miaricds11,0-
item.grantfulltextopen-
item.fulltextCon texto completo-
crisitem.author.deptGIR IUIBS: Medicina Veterinaria e Investigación Terapéutica-
crisitem.author.deptIU de Investigaciones Biomédicas y Sanitarias-
crisitem.author.deptDepartamento de Patología Animal, Producción Animal, Bromatología y Tecnología de Los Alimentos-
crisitem.author.deptGIR IUIBS: Medicina Veterinaria e Investigación Terapéutica-
crisitem.author.deptIU de Investigaciones Biomédicas y Sanitarias-
crisitem.author.deptDepartamento de Patología Animal, Producción Animal, Bromatología y Tecnología de Los Alimentos-
crisitem.author.orcid0000-0001-6509-910X-
crisitem.author.orcid0000-0002-2683-7592-
crisitem.author.parentorgIU de Investigaciones Biomédicas y Sanitarias-
crisitem.author.parentorgIU de Investigaciones Biomédicas y Sanitarias-
crisitem.author.fullNameCarretón Gómez, Elena-
crisitem.author.fullNameMontoya Alonso, José Alberto-
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