ABSTRACT
RESUMEN La quinasa dependiente de ciclina 5 (CDK5) regula diversas funciones en neuronas, células endoteliales y epiteliales, entre ellas la dinámica del citoesqueleto. Así mismo, se ha reportado que componentes del citoesqueleto, tales como, filamentos de actina y microtúbulos juegan un rol importante durante la infección por el virus dengue (DENV). El objetivo del presente trabajo fue evaluar por dos métodos, inhibición química y silenciamiento génico, la participación de CDK5 durante la infección por DENV-2. La actividad antiviral de roscovitina fue evaluada usando ensayos de Unidades Formadoras de Placa (PFU). La eficiencia de transfección y el silenciamiento de CDK5, empleando miARNs artificiales, se determinó por citometría de flujo. El efecto sobre la proteína de envoltura viral y elementos del citoesqueleto se evidenció mediante microscopia avanzada de fluorescencia y análisis de imágenes. Roscovitina mostró actividad antiviral en etapas pre y post-infectivas en una forma dependiente de la dosis. El tratamiento con roscovitina y miRCDK5 mostró ser efectivo reduciendo la cantidad de CDK5 en células no infectadas. En células infectadas y transfectadas con miRCDK5, así como tratadas con el inhibidor, se observó una reducción significativa de la proteína de envoltura viral; sin embargo, no se encontró reducción significativa de CDK5. Además, el tratamiento con roscovitina indujo cambios celulares morfológicos evidentes en células infectadas. Los resultados indican la potencial participación de CDK5 durante la infección por DENV-2, posiblemente mediando la traducción proteica o la replicación del genoma viral a través de la regulación de la dinámica del citoesqueleto. Se requieren datos adicionales para esclarecer la mecanística del fenómeno usando métodos alternativos.
ABSTRACT Cyclin-Dependent Kinase 5 (CDK5) regulates several functions in neurons, endothelial, and epithelial cells, including the cytoskeleton dynamics. Likewise, it has been reported that some cytoskeleton elements, such as actin filaments and microtubules, play an essential role during Dengue virus (DENV) infection. This work aimed to evaluate the role of CDK5 during DENV-2 infection by two methods, chemical inhibition, and gene silencing. The antiviral activity of roscovitine was evaluated using Plaque Forming Units (PFU) assay. The transfection efficiency and knockdown of CDK5, using artificial miRNAs, was carried out by flow cytometry. The effect on the viral envelope protein and cytoskeleton elements was evidenced by advanced fluorescence microscopy and image analysis. Roscovitine showed antiviral activity in pre and post-infection stages in a dose-dependent manner. Treatment with roscovitine and miRCDK5 decrease the amount of CDK5 in uninfected cells. In cells infected and transfected with miRCDK5, as well as treated with the inhibitor, a significant reduction of the viral envelope protein was observed; however, no significant reduction of CDK5 was found. Also, evident morphological cellular changes were observed during the treatment with roscovitine in infected cells. The results indicate the potential participation of CDK5 during DENV-2 infection, possibly mediating protein translation or replication of the viral genome through the cytoskeletal dynamics regulation. Additional data are required to clarify the mechanistic of these phenomena using alternative methods.
ABSTRACT
O objetivo deste estudo foi avaliar a maturação e o desenvolvimento embrionário após a fecundação in vitro de oócitos bovinos que tiveram a maturação bloqueada com Butirolactona I e Roscovitina em meio de pré-maturação suplementado com soro fetal bovino (SFB). Oócitos foram divididos em 4 grupos: Controle 0 hora, Controle (maturação por 24 horas), Butirolactona I (bloqueio da maturação com 150μM de Butirolactona I por 24 horas, seguido de 24 horas de maturação) e Roscovitina (bloqueio da maturação com 50μM de Roscovitina por 24 horas, seguido de 24 horas de maturação). Para avaliar a maturação nuclear, os oócitos foram fixados e corados em aceto orceína. Parte dos oócitos dos grupos Controle 24 horas, Roscovitina e Butirolactona I após o período de maturação, foi fecundado in vitro. O desenvolvimento embrionário foi avaliado pelos índices de clivagem (D3) e formação de blastocistos (D7). Oócitos do grupo Butirolactona I apresentaram índices de Vesícula Germinativa após o bloqueio e de Metáfase 2 após a maturação semelhantes ao dos grupos Controle 0 hora e Controle, respectivamente. Por outro lado, a Roscovitina apresentou menores índices de Vesícula Germinativa e Metáfase 2. Os grupos Controle e Butirolactona I apresentaram maiores índices de clivagens. O grupo Controle apresentou maior produção de blastocistos que o Roscovitina e não diferiu do grupo Butirolactona I. Conclui-se que a Butiroloactona I pode ser utilizada no sistema de pré-maturação em meio contendo SFB, pois apresentou resultados semelhantes ao do grupo Controle o mesmo não ocorrendo com a Roscovitina, que apresentou menores índices de maturação oocitária e de desenvolvimento embrionário.
This study evaluated the bovine oocyte maturation and embryo development after in vitro fertilization. The maturation of the oocytes was blocked using Butyrolactone I and Roscovitine using pre-maturation medium supplemented with fetal calf serum (FCS). The ocytes were divided in four groups: Control 0 hour, Control (24 hours of maturation), Roscovitine (maturation blockage with 50mM Roscovitine during 24 hours followed by 24 hours of maturation), and Butyrolactone I (maturation blockage with 150mM Butyrolactone I during 24 hours followed by 24 hours of maturation). The oocytes were fixed and stained with aceto orcein to evaluate the nuclear maturation. After the maturation period, the remaining oocytes of the Control group, Roscovitine, and Butyrolactone I were fertilized in vitro. Embryo development was assessed by the cleavage rate (D3) and blastocysts formation (D7). The Butyrolactone I group had similar rates of germinal vesical stage oocytes during blockage, and Metaphase 2 after maturation, comparing to Control group at 0 hour and Control group, respectively. On the other hand, the Roscovitine group had lower rates of vesical stage oocytes during blockage, and Metaphase 2 after maturation comparing to Control groups. After in vitro fertilization, higher rates of cleavage were observed in Control and Butyrolactone I groups. For the blastocyst formation rate, the Control group showed better results than Roscovitine group. In summary, Butyrolactone I group had similar results to the Control group, and for this reason, is suitable for pre-maturation of bovine oocytes using FCS. In contrast, Roscovitine group had lower oocyte maturation and embryo development.