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Embryogenic calli induction from nucellar tissue of Citrus cultivars

Indução de calos embriogênicos a partir de nucelos de variedades de Citrus

Abstracts

Nucellar tissues of seven Citrus varieties were introduced onto three growth media to produce embryogenic callus. The media tested were: EME [MT, modified, with the addition of malt extract (500 mg.L-1)]; 1/2-EME [half concentration of MT macronutrients + half concentration of BH3 macronutrients + 500 mg.L-1 malt extract + 1.55 g.L-1 of glutamine]; and EBA [EME + 0.44 muM 6-benzyladenine + 0.04 muM 2,4 D]. Soft friable calli were obtained from 'Cravo' and 'Ponkan' mandarins (Citrus reticulata, Blanco), 'Murcott' tangor (Citrus reticulata Blanco x Citrus sinensis L. Osbeck), 'Serra d'água' and 'Valencia' sweet oranges (Citrus sinensis, L. Osbeck) 120 days after callus induction. 'Natal' and 'Pera' sweet oranges (Citrus sinensis, L. Osbeck) produced hard non-friable calli in this period. EME and 1/2-EME media had the best results for 'Cravo' mandarin, 'Ponkan' mandarin and 'Serra d'água' sweet orange, whereas EBA was the best media composition to induce soft friable calli on 'Murcott' tangor and 'Valencia' sweet orange. Friable callus cultures of 'Cravo' and 'Ponkan' mandarins, and 'Murcott' tangor yielded high quality protoplasts after isolation. Abbreviations: a.c. - activated charcoal; BA - 6-benzyladenine; IAA - indole-acetic acid; 2,4-D - 2,4-diclorophenoxyacetic acid; MT - Murashige & Tucker basal medium.

biotechnology; tissue culture; cultivar improvement; growth regulator; protoplast


Nucelos de sete variedades de Citrus foram introduzidos em três meios de cultura para produção de calos embriogênicos. Os meios de cultura testados foram: EME [MT, modificado pela adição de extrato de malte (500 mg.L-1)]; 1/2-EME [1/2 concentração de macronutrientes no meio MT + 1/2 concentração de macronutrientes no meio BH3 + 500 mg.L-1 extrato de malte + 1,55 g.L-1 de glutamina]; e EBA [EME + 0,44 miM 6-benziladenina + 0,04 miM 2,4 D]. Calos friáveis foram obtidos nas variedades tangerinas 'Cravo' e 'Ponkan' (Citrus reticulata, Blanco), tangor 'Murcote' (Citrus reticulata Blanco x Citrus sinensis L. Osbeck), laranja 'Valencia' (Citrus sinensis L. Osbeck) e lima 'Serra d'água' (Citrus sinensis L. Osbeck) 120 dias após a instalação do ensaio. As laranjas 'Natal' e 'Pera' (Citrus sinensis L. Osbeck) produziram calos duros de crescimento lento neste período. Os meios EME e 1/2-EME mostraram os melhores resultados para as tangerinas 'Cravo' e 'Ponkan' e lima 'Serra d'água', enquanto que EBA foi o melhor meio de cultura para indução de calos friáveis de tangor 'Murcote' e laranja 'Valencia'. Calos friáveis das variedades, tangerinas 'Cravo' e 'Pokan' e tangor 'Murcote' foram subcultivados e apresentaram bom rendimento e qualidade de protoplastos após isolamento.

biotecnologia; cultura de tecido; melhoramento; regulador de crescimento; protoplasto


EMBRYOGENIC CALLI INDUCTION FROM NUCELLAR TISSUE OF CITRUS CULTIVARS

Fernanda Januzzi Mendes-da-Glória1,5; Francisco de Assis Alves Mourão Filho2,6*; Clarice Garcia Borges Demétrio3,6; Beatriz Madalena Januzzi Mendes4,6

1Graduate Student. Depto. de Produção Vegetal - ESALQ/USP.

2Depto. de Produção Vegetal - ESALQ/USP, C.P. 9 - CEP: 13418-900 - Piracicaba, SP.

3Depto. de Ciências Exatas - ESALQ/USP.

4Laboratório de Biotecnologia Vegetal - CENA/USP, C.P. 96 - CEP: 13400-970 - Piracicaba, SP.

5Bolsista da FAPESP.

6Bolsista do CNPq.

*e-mail: famourao@carpa.ciagri.usp.br

ABSTRACT: Nucellar tissues of seven Citrus varieties were introduced onto three growth media to produce embryogenic callus. The media tested were: EME [MT, modified, with the addition of malt extract (500 mg.L-1)]; 1/2-EME [half concentration of MT macronutrients + half concentration of BH3macronutrients + 500 mg.L-1 malt extract + 1.55 g.L-1 of glutamine]; and EBA [EME + 0.44 mM 6-benzyladenine + 0.04 mM 2,4 D]. Soft friable calli were obtained from 'Cravo' and 'Ponkan' mandarins (Citrus reticulata, Blanco), 'Murcott' tangor (Citrus reticulata Blanco x Citrus sinensis L. Osbeck), 'Serra d'água' and 'Valencia' sweet oranges (Citrus sinensis, L. Osbeck) 120 days after callus induction. 'Natal' and 'Pera' sweet oranges (Citrus sinensis, L. Osbeck) produced hard non-friable calli in this period. EME and 1/2-EME media had the best results for 'Cravo' mandarin, 'Ponkan' mandarin and 'Serra d'água' sweet orange, whereas EBA was the best media composition to induce soft friable calli on 'Murcott' tangor and 'Valencia' sweet orange. Friable callus cultures of 'Cravo' and 'Ponkan' mandarins, and 'Murcott' tangor yielded high quality protoplasts after isolation.

Abbreviations: a.c. - activated charcoal; BA – 6-benzyladenine; IAA – indole-acetic acid; 2,4-D – 2,4-diclorophenoxyacetic acid; MT – Murashige & Tucker basal medium.

Key words: biotechnology, tissue culture, cultivar improvement, growth regulator, protoplast

Indução de calos embriogênicos a partir de nucelos de variedades de Citrus

RESUMO: Nucelos de sete variedades de Citrus foram introduzidos em três meios de cultura para produção de calos embriogênicos. Os meios de cultura testados foram: EME [MT, modificado pela adição de extrato de malte (500 mg.L-1)]; 1/2-EME [1/2 concentração de macronutrientes no meio MT + 1/2 concentração de macronutrientes no meio BH3 + 500 mg.L-1 extrato de malte + 1,55 g.L-1 de glutamina]; e EBA [EME + 0,44 mM 6-benziladenina + 0,04 mM 2,4 D]. Calos friáveis foram obtidos nas variedades tangerinas 'Cravo' e 'Ponkan' (Citrus reticulata, Blanco), tangor 'Murcote' (Citrus reticulata Blanco x Citrus sinensis L. Osbeck), laranja 'Valencia' (Citrus sinensis L. Osbeck) e lima 'Serra d'água' (Citrus sinensis L. Osbeck) 120 dias após a instalação do ensaio. As laranjas 'Natal' e 'Pera' (Citrus sinensis L. Osbeck) produziram calos duros de crescimento lento neste período. Os meios EME e 1/2-EME mostraram os melhores resultados para as tangerinas 'Cravo' e 'Ponkan' e lima 'Serra d'água', enquanto que EBA foi o melhor meio de cultura para indução de calos friáveis de tangor 'Murcote' e laranja 'Valencia'. Calos friáveis das variedades, tangerinas 'Cravo' e 'Pokan' e tangor 'Murcote' foram subcultivados e apresentaram bom rendimento e qualidade de protoplastos após isolamento.

Palavras-chave: biotecnologia, cultura de tecido, melhoramento, regulador de crescimento, protoplasto

INTRODUCTION

Brazil leads Citrus world production (FAO, 1998), but, in spite of this position, the Brazilian varieties still lack fruit quality and high yields. Other factors such as disease and pest problems require the development of new Citrus varieties. Conventional Citrus breeding has been carried out, but not with much success for the release of new scion and rootstocks varieties (Grosser & Gmitter Jr., 1990).

Although there is a great diversity in the genus, the majority of new important Citrus varieties, originated as bud sport mutations from existing cultivars. The lack of good results through conventional Citrus breeding can be explained by various aspects of the biology of the genus Citrus and its relatives, including high heterozygozity, pollen and ovule sterility, sexual incompatibility, nucellar polyembryony and juvenility (Grosser & Gmitter Jr., 1990).

Somatic hybridization through protoplast fusion allows the hybridization of sexually incompatible genera and species, which is often difficult or not possible by conventional breeding (Grosser & Gmitter Jr., 1990; Grosser et al., 1996). Protoplast fusion can also be applied to Citrus scion improvement by producing tetraploid breeding parents to be used in 4X x 2X crosses to develop new triploid seedless cultivars (Mourão Filho et al., 1996). Protoplasts can be isolated from different kinds of tissues, including leaf mesophyll, embryogenic callus, embryogenic suspension cultures and non-embryogenic callus (Grosser & Gmitter Jr., 1990).

The objective of this research was to produce new embryogenic callus lines to be used as alternative sources for protoplast isolation. These protoplasts could then be combined with other Citrus species in protoplast fusion experiments for somatic hybrid production.

MATERIAL AND METHODS

Nucellar tissue of the following Citrus cultivars were cultured for embryogenic callus induction: 'Cravo' mandarin (Citrus reticulata, Blanco), 'Murcott' tangor (Citrus reticulata, Blanco x Citrus sinensis L. Osbeck), 'Pera' sweet orange (Citrus sinensis L. Osbeck), 'Ponkan' mandarin (Citrus reticulata, Blanco), 'Natal' sweet orange (Citrus sinensis L. Osbeck), 'Serra d'água' sweet orange (Citrus sinensis L. Osbeck), and 'Valencia' sweet orange (Citrus sinensis L. Osbeck). Fruits from these cultivars were harvested from the germplasm collection at the "Centro de Citricultura Sylvio Moreira", in Cordeirópolis, SP, Brazil. 'Cravo' mandarin is a very early maturing cultivar and produces medium-large fruits, flattened in shape with loosely adhering rind, moderately to excessively seedy. 'Murcott' tangor is grown widely in Florida and Brazil. Trees are vigorous, bushy in shape with willowy leaves. Fruits are of medium size, slightly flattened at the base and apex, juicy and seedy (Saunt, 1990). 'Serra d'água' is an acidless sweet orange cultivar, mostly grown in Brazil. 'Pera' and 'Natal' sweet oranges are also very important cultivars in Brazil. The first is mid season variety. Fruits are slightly oval in shape, with a smooth thin rind. 'Natal' sweet orange resembles 'Valencia' sweet orange in most tree and fruit characteristics, and both are late maturing cultivars (Saunt, 1990).

Seeds in the initial stage of development (six months after fertilization) were excised from fruits and surface sterilized in 1.5% sodium hypochloride solution, for 15 minutes, and washed in sterilized distilled deionized water. The nucellus tissue was then extracted from the seeds with forceps and scalpel, under aseptic conditions and cultured onto three different media. Ten nucelli were introduced per Petri dish and 5 dishes per culture medium, in a total of 50 nucella per treatment and 150 nucella per Citrus cultivar. The culture media tested were: EME [Murashige & Tucker, modified (Murashige & Tucker, 1969), with the addition of malt extract (500 mg.L-1)] (Grosser & Gmitter Jr., 1990); 1/2-EME [half concentration of MT macronutrients + half concentration of BH3macronutrients + 500 mg.L-1 malt extract + 1.55 g.L-1 glutamine] (Grosser & Gmitter Jr., 1990); and EBA [EME + 0.44 mM 6-benzilaminopurine (BA) 0.04 mM 2,4 D] (Gmitter Jr. et al., 1992).

Explants were cultured in disposable Petri dishes (100 x 15 mm), sealed with plastic film, and maintained in the dark at 27oC. Initial calli were transferred to new media without any growth regulators (EME) approximately every four weeks.

Qualitative and quantitative evaluations were conducted 120 days after culture. The best growing calli were selected in an effort to establish long-term callus lines. These selections were then subcultured on EME medium, with or without activated charcoal (500 mg.L-1), for protoplast isolation, followed by an evaluation of protoplast yield. The general protoplast isolation protocol was adapted from Grosser & Gmitter Jr. (1990), and included approximately 500 mg of fresh cultured cells + 2.0 ml 0.7 M BH3 protoplast culture medium + 2.0 ml enzyme solution (Grosser & Gmitter Jr., 1990).

RESULTS AND DISCUSSION

Qualitative evaluations were conducted 120 days after culture, and calli were classified into three categories, based on their quality and vigor, as follows: slow-growing, hard callus; slow-growing, soft callus; and fast-growing, soft callus. Best results were obtained with 'Cravo' mandarin and 'Murcott' tangor, that produced fast-growing, friable calli on 1/2-EME and EBA media (Figure 1A). However, the same cultivars produced slow-growing, friable calli on EME medium (Figure 1B). Slow-growing, friable calli of 'Valencia' sweet orange was produced on 1/2-EME and EBA media. 'Pera' sweet orange produced hard calli (Figure 1C) on EME and EBA media. No callus induction of this cultivar was observed on 1/2-EME medium. 'Natal' sweet orange produced hard calli on all media tested. 'Serra d'água' sweet orange produced some slow-growing friable calli on EME and 1/2-EME, and hard calli on all media tested. 'Ponkan' mandarin produced slow-growing, friable calli on all media tested and also hard calli on EBA medium. The different source of nitrogen in 1/2-EME (Grosser & Gmitter Jr., 1990) or the addition of growth regulators on modified EME (EBA) may have positively influenced these results.


The addition of activated charcoal (500 mg l-1) seemed to enhance callus vigor and color for a few varieties, such as 'Natal', that had shown oxidation and slow growth. After two subcultures, better growth and friability were observed on these selections. Mourão Filho & Grosser (1992) also demonstrated the positive effect of activated charcoal on callus performance, quality and vigor in different species of the Rutaceae family.

In regard to quantitative evaluations, a logistic model with overdispersion was fitted to the proportions of nucelli response to fast- and slow-growing soft calli (combined), for five Citrus cultivars, i.e., for only those that did not present all counting numbers equal zero. It was considered that the number of soft friable calli have a binomial distribution with the index equal to the number of cultivated nucelli. The analysis of deviance shows that there was a significant interaction between cultivars and media composition (TABLE 1). EME and 1/2-EME media proved best for 'Cravo' mandarin, 'Ponkan' mandarin and 'Serra d'água sweet orange, whereas EBA was the best media composition for soft friable calli induction for 'Murcott' tangor and 'Valencia' sweet orange (Figure 2). There was no soft friable calli induction from 'Pera' and 'Natal' sweet oranges .


Effects of cultivar and media composition on Citrus callus induction, vigor and quality were previously reported. MT medium supplemented with malt extract also induced embryogenic calli of 'Shamouti' sweet orange (Citrus sinensis) but failed to do so with 'Valencia' sweet orange and 'Marsh grapefruit (Citrus paradisi) (Kochba et al., 1972). Mourão Filho & Grosser (1992) reported the results of non-embryogenic callus induction, friability and vigor of 30 selection of Citrus and its wild relatives from the Rutaceae family. Soft friable callus was obtained from several species, including Aegle marmelos (L.), Afraegle gabonensis (Swing.) Engl., Afraegle paniculata (Schum.) Engl., Balsamocitrus daweii Stapf., Citropsis gilletiana Swing. & M. Kell., Citrus jambhiri Lush. (rough lemon). Oliveira et al. (1994) also demonstrated the influence of genotype and media composition on embryogenic callus induction. MT supplemented with indole-acetic acid (IAA) and kinetin induced best nucella response for embryogenic calli formation in 'Cleopatra' mandarin (Citrus reticulata, Blanco) and 'Rangpur' lime (Citrus limonia, L. Osbeck). No callus induction was achieved with Poncirus trifoliata on any of the media tested (MT + malt extract, MT + IAA + kinetin, MT + BA).

Protoplasts were obtained from callus cultures of 5 of 7 cultivars tested (TABLE 2). However, high yields were obtained only from 'Cravo' mandarin, 'Murcott' tangor and 'Ponkan' mandarin.

Suspension cultures were initiated from the different callus lines. After three to four subcultures, suspension cultures of 'Valencia' sweet orange and 'Serra d'água' sweet orange produced a high number of embryos, proving their embryogenic capacity. Mourão Filho & Grosser (1992) have also demonstrated protoplast isolation soon after callus induction. The best results were always obtained from soft, friable calli.

CONCLUSIONS

The responses of the seven Citrus varieties on the three callus induction media were variable. 'Cravo' mandarin and 'Murcott' tangor showed the best results, producing friable fast-growing calli, 120 days after the initiation of the experiment. The other varieties, except 'Pera' sweet orange, also produced friable calli after several subcultures on culture media without any plant growth regulators. These selections can now be used for protoplast isolation and fusion for Citrus somatic hybridization.

ACKNOWLEDGMENT

This work was supported by Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP).

REFERENCES

FAO http://apps.fao.org 1998.

Received December 04, 1998

Accepted August 11, 1999

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  • MOURĂO FILHO, F.A.A.; GROSSER, J.W.; GMITTER JR., F.G. New tetraploid breeding parents for triploid seedless citrus cultivar development. Fruit Varieties Journal, v.50, n.2, p.76-80, 1996.
  • MURASHIGE, T.; TUCKER, D.P.H. Growth factor requirements of Citrus tissue culture. Proceedings of the First International Citrus Symposium, v.3, p.1155-1161, 1969.
  • OLIVEIRA, R.P.; MENDES, B.M.J.; TULMANM NETO, A. Obtençăo e cultura de calos nucelares de limăo Cravo, tangerina Cleopatra e Poncirus trifoliata Revista Brasileira de Fisiologia Vegetal, v.6, n.2, p.115-119, 1994.
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Publication Dates

  • Publication in this collection
    22 Dec 2000
  • Date of issue
    1999

History

  • Accepted
    11 Aug 1999
  • Received
    04 Dec 1998
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