Your browser doesn't support javascript.
loading
Show: 20 | 50 | 100
Results 1 - 3 de 3
Filter
1.
Rev. colomb. biotecnol ; 13(2): 39-50, dic 1, 2011. tab, graf
Article in Spanish | LILACS | ID: lil-645166

ABSTRACT

El objetivo de esta investigación fue evaluar dos protocolos de propagación vía embriogénesis somática a partir de explantes florales en dos clones élite BIOB e ICS95 de Theobroma cacao L. Se obtuvo un 50 y 32% de callo embriogénico en ICS95 y BIOB respectivamente con el protocolo de Fontanel et al. (2002), modificado después de un periodo de cultivo de tres meses. Los embriones pasaron por fases que se correspondieron con medios de cultivo diferenciales: Inducción, Formación, Maduración y Mantenimiento. Para la embriogénesis somática secundaria se obtuvo un 23% de embriones a partir de embriones somáticos primarios en un medio, conteniendo 1mg/L de 2,4,5 T (2,4,5 Triclorofenoxiacético). Se logró, además, desarrollar enraizamiento adventicio aplicando pulsos de IBA (Ácido Indol Butírico) a 0.5mg/L y 0.5g/L durante un minuto. Las plantas enraizadas se llevaron a una mezcla de tierra: arena (1:1) para su adaptación ex vitro, obteniéndose un 66% de plantas aclimatadas. Los estudios histológicos mostraron diferentes características típicas del desarrollo embriogénico. Este es el primer reporte en el que se logra de manera exitosa la conversión hasta plántula (68%) y la adaptación ex vitro de una variedad colombiana de cacao vía embriogénesis somática primaria y secundaria.


In this research we evaluate two protocols of propagation via somatic embryogenesis from floral explants using two elite clones BIOB and ICS95 of Theobroma cacao L. We obtained 50 and 32% of embryogenic callus on ICS95 and BIOB respectively with Fontanel et al., (2002) protocol modified after three months of culture. The embryos went through four phases; Induction, Formation, Maduration and Mantenimiento which corresponded each one with different media culture. For secondary somatic embryogenesis we obtained 23% of embryos from primary somatic embryos in a medium with 1mg/L of 2,4,5 T (2,4,5 Triclorofenoxiacetic). Also we obtained plants that developed new roots applying pulses with IBA (Indol Butiric Acid) 0.5mg/L and 0.5g/L for a minute. The developed plants were moved to a mix of potting soil and sand (1:1) for their ex vitro adaptation, getting 66% of acclimatized plants. The histological analysis showed the typical characteristics of the embryogenic development. This is the first report where it is achieved the successful conversion to plantlets (68%) and ex vitro adaptation of a colombian cocoa variety via primary and secondary embryogenesis.


Subject(s)
Animals , Embryonic Development/genetics , Embryonic Development/immunology , Plant Somatic Embryogenesis Techniques/classification , Plant Somatic Embryogenesis Techniques/statistics & numerical data , Plant Somatic Embryogenesis Techniques/instrumentation , Plant Somatic Embryogenesis Techniques/methods , Plant Somatic Embryogenesis Techniques
2.
Rev. colomb. biotecnol ; 11(2): 40-47, dic. 2009.
Article in Spanish | LILACS | ID: lil-550518

ABSTRACT

La obtención de un sistema de regeneración eficiente por medio de la embriogénesis somática en las Musaceas, es hoy una gran herramienta ante los enormes problemas que presenta este género con el ataque de enfermedades como la sigatoka negra. El objetivo del trabajo es determinar las densidades celulares adecuadas para las etapas de multiplicación de suspensiones celulares embriogénicas y formación de los embriones somáticos en medios de cultivo líquidos. Como material vegetal se usaron brotes inmaduros de la inflorescencia masculina de Musa AAAB, cv. FHIA-18. Los resultados demostraron que es posible el establecimiento de suspensiones celulares homogéneas a partir de embriones somáticos en etapa globular, y obtener los mayores volúmenes de biomasa celular al multiplicar dichas suspensionescon una densidad del 3% del volumen de células sedimentadas. A partir del decimoquinto día en el medio de cultivo de formación de embriones comenzaron a formarse estructuras compuestas por proembriones y embriones somáticos en etapa globular; entre las densidades estudiadas los mejores resultados se obtuvieron con 100 mgMF en la cual se formaron 1 871 ES.l-1 con un peso de 248 mgMF.l-1.


An extremely useful tool for dealing with the enormous problems involved in banana growing (Musaceae) caused by the attack of diseases such as black Sigatoka can be obtained today by ensuring an efficient regeneobration system via somatic embryogenesis. The work was aimed at defining appropriate cell densities for embryogenic cell suspension growth stages and somatic embryo formation in liquid culture medium. Immature male inflorescence buds from Musa AAAB cf FHIA-18 were used as vegetal material. The results showed that it is possible to establish homogeneous cell suspensions from somatic embryos in globular stage andobtain greater cell biomass volume by multiplying the suspension with 3% sedimented cell volume (density).Embryos began to form structures in culture medium consisting of globular stage somatic proembryos and embryos from the fifteenth day onwards. The best results amongst the densities studied were obtained with 100 mgMF, in which 1,871 ES.l -1 were formed weighing 248 mgMF.l-1.


Subject(s)
Embryonic Development/genetics , Embryonic Development/immunology
3.
Article in English | WPRIM | ID: wpr-162124

ABSTRACT

Heat shock proteins (HSP) have been identified as an important factor of a very complex and highly conserved cellular defense mechanism to preserve cell survival under adverse environmental conditions. HSP 60 are immunodominant antigens of microbe such as Chlamydia trachomatis and have a potentiality to become a target antigen due to antigenic similarity between chlamydial and human HSP. This study was conducted to investigate the effects of Vero cell coculture to anti-HSP 60 on the early mouse embryo development in vitro. The 2-cell mouse embryos (ICR) were cultured and mouse embryo development was observed every 24 hr for 3 days. 45% and 22.1% of the embryos cultured in Ham's F-10 plus anti HSP 60 with Vero cells developed to the 4- to 8- cell stage (day 1) and morular stage (day 2) as compared with 29.2% and 2.7% of those cultured without Vero cells respectively. But at day 3, the beneficial effect of Vero cells was not noted. These findings suggest that Vero cells have some roles to overcome the detrimental effect of anti-HSP 60 to some degree. These results suggest that Vero cells coculture will promote reproductive outcome in patient previously sensitized to microbial (e.g. Chlamydia trachomatis) HSP 60.


Subject(s)
Pregnancy , Mice , Male , Female , Animals , Vero Cells , Mice, Inbred ICR , Infertility, Female/etiology , Immunodominant Epitopes , Embryonic Development/immunology , Coculture Techniques , Chlamydia trachomatis/immunology , Chaperonin 60/immunology , Chlorocebus aethiops , Antigens, Bacterial , Antibodies, Monoclonal/administration & dosage
SELECTION OF CITATIONS
SEARCH DETAIL