Antibioticoterapia em microplantas de abacaxizeiro (Ananas comosus) / Antibiotic therapy in Pineapple (Ananas comosus) microplants

RESUMO: Com o intuito de avaliar os efeitos da antibioticoterapia no crescimento de plantas micropropagadas de abacaxizeiros, bem como na comunidade bacteriana endofítica da espécie, realizaram-se análises moleculares. Verificou-se a presença de endófitos no interior das microplantas, mesmo após 30 dias de cultivo em meio de cultura MS, suplementado com diferentes antibióticos, e analisou-se o crescimento da parte aérea e radicular das microplantas. Decorrido o período de 30 dias de cultivo, constatou-se ainda a presença de bactérias endofíticas, no entanto, as microplantas apresentaram acentuada redução no crescimento da parte aérea e radicular, evidenciando assim a influência da microbiota endofítica no crescimento das microplantas in vitro e a importância da manutenção do equilíbrio endofítos/microplanta.

ABSTRACT: This research aimed to evaluate the antibiotic therapy effects in the growing of micropropagated pineapple plants as well as in the community of the endophytic bacterial of the species. It was performed molecular analyzes and verified the presence of endophytes within microplants even after 30 days of culture on MS medium supplemented with different antibiotics and analyzed the development growth of shoots and roots of microplants. After the period of 30 days of cultivation, even being checked the presence of endophytic bacteria, it was verified that the microplants showed reduction of the growing of shoots and roots, thereby demonstrating the influence of in vitro endophytic microorganisms in the development of microplants, and the importance of maintaining it in equilibrium with endophytes/ microplants.

Cambios morfológicos, proteicos, glicoproteicos y antigénicos de Trypanosoma cruzi cultivado en medio axénico con tensiones de oxígeno diferentes / Morphological, protein, glycoprotein and antigenic changes of Trypanosoma cruzi cultured in axenic medium with different oxygen tensions

Se ha reportado cultivo axénico de amastigotas de Trypanosoma cruzi derivados de epimastigotas. Se cuestiona si formas redondas en cultivos axénicos son verdaderos amastigotas. Aquí se compararon los cambios biológicos y moleculares de epimastigotas creciendo en alta y baja tensión de oxígeno. T. cruzi (EPm6) se creció en frascos con diferentes alturas de medio LITB (condición horizontal 3 mm y vertical 83 mm). Se colectaron masas de parásitos de diferentes tiempos de crecimiento para análisis proteico, glicoproteico y antigénico. Se estudiaron los cambios morfológicos, incremento de inóculo y resistencia al complemento por microscopia de fases y tinción con Giemsa. Los cambios proteicos y glicoproteicos se compararon por SDS-PAGE. Los cambios antigénicos se analizaron por Western blot con suero de conejo y anticuerpos IgY contra formas amastigotas. En condición vertical, los epimastigotas mantuvieron su morfología típica a lo largo de la curva de crecimiento y no mostraron cambios moleculares significativos. En condición horizontal al 4to y 6to día predominaron formas redondas con capacidad de resistir la lisis por complemento. A partir del 4to día se observaron cambios en los perfiles proteicos y glicoproteicos, concomitantemente con los cambios morfológicos. El suero anti-amastigotas reveló un antígeno amastigota-específico transitorio de 55 kDa en parásitos de 4 días en la condición horizontal, mientras el anticuerpo IgY anti-amastigotas no reveló diferencias entre parásitos creciendo en ambas condiciones. Estas evidencias sugieren que epimastigotas de T. cruzi condicionados a sobrevivir en alta tensión de oxígeno puede mimetizar propiedades biológicas y antigénicas propias del estadio amastigota.

Axenic culture of epimastigote-derived amastigotes of Trypanosoma cruzi has been reported. Have been inquired why round forms appear in culture media and if are true amastigotes. Our proposal was study molecular and biological changes in epimastigotes growing in high and low oxygen tension. T. cruzi (EPm6) were grown in flasks with different height of LITB medium (horizontal condition 3 mm and vertical 83 mm). Parasites were collected masses of different times of growth for proteins, glycoproteins and antigenic analysis. Morphological changes, increase of inoculum and resistance to complement lyses were studied in phase’s microscopy and Giemsa-stained smears. Protein and glycoprotein changes were compared by SDS-PAGE. Antigenic changes were analyzed by Western blot with rabbit serum and IgY antibody against amastigote forms. In vertical condition, the epimastigote maintained its typical morphology along the growth curve and not showed significant molecular changes. In horizontal condition round forms prevailed at 4 and 6 days with capacity to resist lyses by complement. From the 4th day changes in proteins and glycoproteins profiles were observed, concomitantly with the morphological changes. Anti-amastigotes serum revealed a 55 kDa transitory amastigote-specific antigen in four day parasites’ from horizontal condition, while IgY antibody anti-amastigotes don’t revealed differences between parasites grown in both conditions. These evidences suggest that epimastigotes of T. cruzi conditioned to survive in high oxygen tension can mimic biological and antigenic properties own the amastigote-stage.

ELISA protocol for rapid screening of potential antitubercular drugs based on antigenic reactivity of mycobacterial ES-31 serine protease - a drug target supported by axenic culture of Mycobacterium tuberculosis H37 Ra strain in the presence of inhibitor.

Background: Mycobacterial ES-31 serine protease has been reported to be a drug target using protease and lipase inhibitors in axenic and macrophage cultures. Simple screening techniques are needed for rapid testing of anti-tubercular drugs. Aim: To demonstrate the usefulness of ELISA protocol based on antigenic reactivity of mycobacterial serine protease by indirect ELISA for detecting anti-tubercular activity. Material and Methods: Indirect ELISA for assessment of antigenic reactivity of mycobacterial ES-31 serine protease was standardized using ES-31Ag and anti-DSS-goat-serum and assessed the inhibition of the antigenic reactivity by isoniazid, an anti-tubercular drug and serine protease inhibitor and orlistat, a lipase inhibitor. Results: Optimal antigenic reactivity of mycobacterial ES-31 serine protease was observed at 5μg/well of ES-31 antigen and at 1:25 dilution of anti-DSS-goat-serum. Isoniazid showed 42% inhibition of ES-31 serine protease at 0.4μg/well, while orlistat showed inhibition of 60% at 0.5μg/well. Inhibition of Mtb H37Ra bacilli is further confirmed in axenic culture. 35% and 29% inhibition by isoniazid at 0.4μg/well and orlistat at 0.5μg/well were observed respectively on bacterial growth. Conclusion: Simple ELISA protocol based on assay of antigenic reactivity of mycobacterial ES-31 serine protease, a drug target, has been standardized for rapid screening of potential anti-tubercular drugs.

Apoptotic-like activity of staurosporine in axenic cultures of Trypanosoma evansi / Actividad proapoptótica de la estaurosporina en cultivos axénicos de Trypanosoma evansi

Trypanosoma evansi is a blood protozoan parasite of the genus Trypanosoma which is responsible for surra (Trypanosomosis) in domestic and wild animals. This study addressed apoptotic-like features in Trypanosoma evansi in vitro. The mechanism of parasite death was investigated using staurosporine as an inducing agent. We evaluated its effects through several cytoplasmic features of apoptosis, including cell shrinkage, phosphatidylserine exposure, maintenance of plasma membrane integrity, and mitochondrial trans-membrane potential. For access to these features we have used the flow cytometry and fluorescence microscopy with cultures in the stationary phase and adjusted to a density of 10(6) cells/mL. The apoptotic effect of staurosporine in T. evansi was evaluated at 20 nM final concentration. There was an increase of phosphatidylserine exposure, whereas mitochondrial potential was decreased. Moreover, no evidence of cell permeability increasing with staurosporine was observed in this study, suggesting the absence of a necrotic process. Additional studies are needed to elucidate the possible pathways associated with this form of cell death in this hemoparasite.

Trypanosoma evansi es un hemoparásito, el cual es el agente causal de la surra (tripanosomiasis) en mamíferos, perteneciente al orden Kinetoplastidae. Este estudio se oriento a caracterizar la muerte celular similar a apoptosis en cultivos in vitro de Trypanosoma evansi a través del uso del inductor esturosporina. Este efecto se evaluó a través de diversos aspectos fenotípicos de la apoptosis: el encogimiento celular, la exposición de fosfatidilserina, el mantenimiento de la integridad de la membrana plasmática y el potencial de membrana mitocondrial. Para evaluar estas características se utilizaron técnicas de citometría de flujo y microscopía de fluorescencia con cultivos en fase estacionaria ajustados a una densidad de 10(6) células/mL. El efecto apoptótico de la estaurosporina en Trypanosoma evansi fue evaluado a una concentración de 20 nM. Se evidenció un aumento de la exposición a fosfatidilserina, mientras que el potencial mitocondrial disminuyó. Por otra parte, no hay evidencias de aumento de la permeabilidad celular con estaurosporina, sugiriendo la ausencia de un proceso necrótico. Estudios adicionales son necesarios para dilucidar las posibles vías asociadas con esta forma de muerte celular en este hemoparásito.