In vitro plant regeneration from quality protein maize (QPM)

被引:0
|
作者
Gerardo Armando Aguado-Santacruz
Edmundo García-Moya
José Luis Aguilar-Acuña
Blanca Moreno-Gómez
Ernesto Solís-Moya
Ernesto Ricardo Preciado-Ortiz
Juan Francisco Jiménez-Bremont
Quintín Rascón-Cruz
机构
[1] Instituto Nacional de Investigaciones Forestales y Agropecuarias,Unidad de Biotecnología, Campo Experimental Bajío
[2] Colegio de Postgraduados,Postgrado en Botánica
[3] Instituto Nacional de Investigaciones Forestales y Agropecuarias,Campo Experimental Bajío
[4] Instituto Nacional de Investigaciones Forestales y Agropecuarias,Programa de Mejoramiento Genético de Maíz, Campo Experimental Bajío
[5] Instituto Potosino de Investigacíon Científica y Tecnológica,Departamento de Biología Molecular
[6] A.C.,Facultad de Ciencias Químicas
[7] Universidad Autónoma de Chihuahua,undefined
关键词
Somatic Embryogenesis; Organogenesis; Tissue Culture; Immature Embryos; Genetic Transformation;
D O I
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中图分类号
学科分类号
摘要
Breeding efforts to obtain more nutritious maize materials aimed at alleviating dietary deficiencies in developing countries have resulted in an improved maize germplasm known as quality protein maize (QPM). Quality protein maize has higher contents of tryptophan, lysine, and leucine than common maize, but suffers from some major agronomic drawbacks found in common inbred maize lines, such as susceptibility to insect pests and fungal and bacterial diseases and herbicide sensitivity. The development of a reproducible and efficient protocol for tissue culture of QPM is expected to solve some of these deficiencies. In this work, we have evaluated different formulations for in vitro induction of morphogenic responses in three QPM lines developed by the International Maize and Wheat Improvement Center (CIMMYT): CML (CIMMYT maize line)-145, CML-176, and CML-186. Only CML-176 and CML-186 have proven to be responsive to the in vitro conditions considered in this work, with CML-176 showing the highest efficiency in regenerable callus formation and growth. N6C1 medium was found to be efficient for in vitro culture of QPM, whereas no plants could be regenerated by using MPC medium. From CML-176 embyogenic calli cultured on N6C1 medium, we were able to regenerate up to 0.3 plants per 500 mg fresh weight (FW) callus. Further modifications in this experimental protocol, including the replacement of 3,6-dichloro-o-anisic acid with 2,4-dichlorophenoxyacetic acid and modification of the N6C1 vitamin balance, significantly increased the regeneration response of the induced calli, with up to 16.8 and 9.3 plants recovered per 500 mg FW callus for CML-176 and CML-186, respectively.
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页码:215 / 224
页数:9
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