Direct in vitro regeneration of castor bean plants (Ricinus communis) using epicotyls / Regeneração direta in-vitro de plantas de mamona ( Ricinus communis ) usando epicótilos

A regeneration protocol for castor bean plant (Ricinus communis) was successfully developed using epicotyl sections obtained from in vitro seedlings. The maximum number of induced shoots (4.3 shoots/explant) and highest shoots frequency (75,56%) was obtained in WPM medium supplemented with TDZ (1 mg/L) and zeatin (0.5 mg/L), whereas the minimum number (0.8 shoots/explant) and lowest shoots frequency (37,78%) was obtained in medium containing TDZ (1 mg/L) and BAP (0.5 mg/L). The highest percentage of rooting (93.3%) was obtained in a medium containing IBA (1 mg/L). These plants were transplanted in a mesh house and achieved a high adaptability to acclimatization, reaching 77% survival. On the other hand, the maximum elongation (height) during this stage was 7.9 cm in plants supplemented with WPM nutrients, whereas it was only 4.38 cm in control plants

Foi desenvolvido com sucesso um protocolo de regeneração para a planta de Mamona (Ricinus communis) utilizando seções de epicótilos, obtidas a partir de mudas in vitro. O número máximo de brotações induzidas (4.3 brotos/explante), assim como a maior frequência de brotações (75,56%), foi obtido em meio WPM suplementado com TDZ (1 mg/L) e zeatina (0,5 mg/L). Enquanto que o número mínimo (0,8 brotos/explante), como a menor freqüência de rebentos (37,78%), foi obtido em meio contendo TDZ (1 mg/L) e BAP (0,5 mg/L). Adicionalmente, a maior percentagem de enraizamento (93,3%) foi obtida em um meio contendo IBA (1 mg/L). Depois da regeneração, as plantas foram transplantadas em casa de vegetação e conseguiram uma alta adaptabilidade e aclimatização, atingindo 77% de sobrevivência. Por outro lado, oalongamento máximo (altura) durante este estágio foi de 7,9 cm em plantas suplementadas com nutrientes de WPM, enquanto as plantas de controle presentaram apenas 4,38 cm

In Vitro Organogenesis from Root Explants of Passiflora miniata Mast, an Amazonian Species with Ornamental Potential

ABSTRACT The present study reports a shoot organogenesis-based system for in vitro regeneration of Passiflora miniata, an Amazonia passion fruit species. Root segments were cultured in Murashige and Skoog (MS) medium supplemented with different concentrations (range 2-9 µM) of 6-benzyladenine (BA); thidiazuron (TDZ) or kinetin (KIN). Plant growth regulators were not added to the control treatment. Root explants have showed a high regenerative potential. After 30 days of in vitro culture, the root explants showed several shoots formed direct and indirectly. TDZ provided the best response in the differentiation adventitious shoots, mainly in the presence of 6.8 µM. The cytokinins BA and KIN responded producing a reduced number of shoots. After 120 days, rooted regenerated plants were transferred to a greenhouse for acclimatization. This regeneration system opens new perspectives for micropropagation and conservation of this wild Amazonic passion fruit species.

Efficient regeneration and genetic transformation platform applicable to five Musa varieties

Background: Banana (Musa spp.) is an important staple food, economic crop, and nutritional fruit worldwide. Conventional breeding has been seriously hampered by their long generation time, polyploidy, and sterility of most cultivated varieties. Establishment of an efficient regeneration and transformation system for banana is critical to its genetic improvement and functional genomics. Results: In this study, a vigorous and repeatable transformation system for banana using direct organogenesis was developed. The greatest number of shoots per explant for all five Musa varieties was obtained using Murashige and Skoog medium supplemented with 8.9 µM benzylaminopurine and 9.1 µM thidiazuron. One immature male flower could regenerate 380­456, 310­372, 200­240, 130­156, and 100­130 well-developed shoots in only 240­270 d for Gongjiao, Red banana, Rose banana, Baxi, and Xinglongnaijiao, respectively. Longitudinal sections of buds were transformed through particle bombardment combined with Agrobacterium-mediated transformation using a promoterless ß-glucuronidase (GUS) reporter gene; the highest transformation efficiency was 9.81% in regenerated Gongjiao plantlets in an optimized selection medium. Transgenic plants were confirmed by a histochemical assay of GUS, polymerase chain reaction, and Southern blot. Conclusions: Our robust transformation platform successfully generated hundreds of transgenic plants. Such a platform will facilitate molecular breeding and functional genomics of banana.

Indirect in vitro organogenesis of Hancornia speciosa Gomes / Organogênese indireta in vitro de Hancornia speciosa Gomes

Hancornia speciosa Gomes is a fruit species belonging to the Apocynaceae family and holds social, cultural and economic potential mostly due to its use in composition of many food industry products and the consumption its fruits in natura. Several aspects regarding their propagation need further studies, since the species is undergoing a continuous process of domestication. The objective was to obtain an in vitro protocol for indirect organogenesis and rooting with subsequent acclimatization of H. speciosa plants. To obtain indirect organogenesis, internodal segments were inoculated in WPM culture medium gelled with 7 g L-1 agar, added with 30 g L-1 sucrose, 0.4 g L -1 PVP, and supplied with different concentrations of 2,4-D (0.0; 2.46; 7.38; 12.30; and 17.22 µM), BAP (0.0; 4.92; 9.84; 14.76; and 19.68 µM), and TDZ (0.0; 4.92; 9.84; 14.76; and 19.68 µM). For the in vitro rooting, shootings with approximately 6.0 cm diameter length kept for 15 days in WPM medium with no plant growth regulator and, afterwards, subjected to treatments with different auxins (Control; 9.84 µM IBA; 9.84 µM NAA; and 9.84 µM IAA) as well as the combination among them, in order to verify their effects on percentage of rooting (%), number of roots, and average length of the largest root (cm). The formation of calluses was observed in all explants subjected to the concentrations of the regulators tested. The highest shooting regeneration occurred with 7.38 µM 2,4-D (73%). The highest percentage of shoot rooting (80%) and roots with the largest length (1.3 cm) were found in the culture medium with the combination of 4.92 µM NAA and 4.92 µM IBA. The in vitro regeneration of H. speciosa is feasible. The acclimatization of rooted shoots in Trospstrato® was accomplished with successful and 100% survival of plant material was observed during this stage.

Hancornia speciosa Gomes é uma frutífera pertencente à família Apocynaceae e possui grande potencial social, cultural e econômico, principalmente devido à utilização de seus frutos na composição de diversos produtos do setor alimentício e para consumo in natura. Vários aspectos de sua propagação necessitam de maiores estudos, uma vez que a espécie passa por um contínuo processo de domesticação. Objetivou-se obter um protocolo de organogênese indireta e de enraizamento in vitro, com posterior aclimatização das plantas de H. speciosa. Para a obtenção de organogênese indireta, segmentos internodais foram inoculados em meio de cultivo WPM gelificado com ágar 7 g L-1, acrescido de 30 g L-1 de sacarose, 0,4 g L-1 de PVP e suplementado com diferentes concentrações de 2,4-D (0,0; 2,46; 7,38; 12,30 e 17,22 µM), BAP (0,0; 4,92; 9,84; 14,76 e 19,68 µM) e TDZ (0,0; 4,92; 9,84; 14,76 e 19,68 µM). Para o enraizamento in vitro, foram utilizadas brotações com aproximadamente 6,0 cm de comprimento, mantidas por 15 dias em meio WPM isento de fitorreguladores e, em seguida, submetidas a tratamentos com diferentes auxinas (Controle; 9,84 µM de AIB; 9,84 µM de ANA e 9,84 µM de AIA), bem como as combinações entre estes reguladores (4,92 µM AIA + 4,92 µM AIB; 4,92 µM ANA + 4,92 µM AIB; 4,92 µM ANA + 4,92 µM AIA). Foi observada formação de calos em todos os explantes submetidos às concentrações dos reguladores testados. A maior regeneração de brotação ocorreu com 7,38 µM de 2,4-D (73%). Maior porcentagem de enraizamento das brotações (80%) e raízes com maior comprimento (1,3 cm) foi verificada em meio de cultivo contendo a combinação de 4,92 µM de ANA e 4,92 µM de AIB. É possível a regeneração in vitro de H. speciosa. A aclimatização foi realizada com sucesso, com 100% de sobrevivência das plantas.

Induction of in vitro shoots of Billbergia euphemiae E. Morren (Bromeliaceae) from leaf explants / Indução in vitro de brotos de Billbergia euphemiae E. Morren (Bromeliaceae) a partir de explantes foliares

Bromeliads are an important group for the maintenance of the Atlantic Forest, with many threatened species due to exacerbated extraction and destruction of their natural habitats. Considering the need of developing protocols for the conservation of these species, the aim of this work was to evaluate the effect of different growth regulators in the in vitro induction of shoots of Billbergia euphemiae. Leaf explants were excised from seedlings derived from in vitro germination and grown on MS medium supplemented with NAA (0, 1 or 2 µM) and BA (0, 2, 4 or 6 µ M) combinations. The evaluation of the number of shoots per explant, shoot length, number of leaves per shoot and longest leaf length average was carried out after 30 and 60 days of culture. The best in vitro responses were observed in the presence of 1 µM NAA after 60 days of culture, which induced the best production of shoots per explant (16.39), as well as the highest rates of shoot length (1.08 cm), number of leaves per shoot (5.00) and the longest leaf length (0.56 cm). This work determined the best conditions for shoot production from leaf explants of B. euphemiae, being the first report on micropropagation of this species.

As bromélias constituem um importante grupo para a manutenção da Floresta Atlântica, com várias espécies ameaçadas de extinção pelo extrativismo exacerbado e a destruição dos habitats naturais. Considerando a necessidade do desenvolvimento de protocolos para a conservação destas espécies, este trabalho teve como objetivo avaliar o efeito de diferentes reguladores de crescimento na indução de brotos de Billbergia euphemiae. Explantes foliares foram excisados de plântulas derivadas da germinação in vitro e inoculados em meio MS suplementado com combinações de ANA (0, 1 ou 2 µM) e BA (0, 2, 4 ou 6 µM). O número de brotos por explantes, comprimento dos brotos, número médio de folhas por broto e comprimento médio da maior folha foram avaliados após 30 e 60 dias de cultura. As melhores respostas foram observadas na presença de ANA a 1 µM, após 60 dias de cultura, que induziu a maior produção de brotos por explante (16,39), assim como as maiores taxas de comprimento dos brotos (1,08 cm), número médio de folhas por broto (5,00) e comprimento da maior folha (0,56 cm). Este trabalho determinou as melhores condições para produção de brotos de B. euphemiae a partir de explantes foliares, representando o primeiro relato de micropropagação desta espécie.

Histology of the regeneration of Paulownia tomentosa (Paulowniaceae) by organogenesis / Histología de la regeneración por organogénesis en Paulownia tomentosa (Paulowniaceae)

Paulownia tomentosa is a fast-growing tree species with a considerable economic potential because of its value for wood as well as its high biomass production, and elevated stress tolerance. The objective of the present study was to evaluate the development of adventitious buds in leaves obtained from four-week-old shoots of P. tomentosa, in order to identify the cells involved in in vitro adventitious bud development. Leaves (proximal halves with the petiole) from the first node were excised from four-week-old micropropagated shoots, and cultured on Murashige and Skoog medium, supplemented with 3% (w/v) sucrose, 0.6% (w/v) Sigma agar, 22.7µM thidiazuron (TDZ) and 2.9µM indole-3-acetic acid for two weeks, explants were then transferred to the same medium with 0.44µM N6-benzyladenine for another four weeks. Five explants were collected daily during the two first weeks in TDZ treatment. A total of 140 samples were processed. Most of the buds developed indirectly from the callus formed in the petiole stub, and they became visible after eight-ten days of culture, although some buds were also observed in the area of the laminar cut at the level of the veins. The first histological changes could be observed after two-three days of culture, with the dedifferentiation of some subepidermal and inner parenchyma cells, which exhibited a large, prominent nucleus, densely-stained cytoplasm and a high nucleusto-cell area ratio. Proliferation of these cells gives rise to meristemoid formation after seven-ten days of culture. Organized cell division in meristemoids allows the formation of bud primordia that emerged from the explants surface. The progressive structural differentiation of the apical meristem, leaf primordia, and procambium strands, led to formation of complete buds that were observed in the exterior of the explants after 10-15 days of culture. Direct development of buds from cells in the subepidermic and/or epidermic layers were observed ...

Paulownia tomentosa es un árbol de rápido crecimiento y con un gran potencial económico por su madera, su utilización para la producción de biocombustible, así como su alto rendimiento en la producción de biomasa y su elevada tolerancia al estrés. El objetivo del presente trabajo ha sido evaluar el desarrollo a nivel histológico de yemas adventicias en hojas de Paulownia tomentosa. Hojas del primer entrenudo de brotes de cuatro semanas cultivados in vitro, fueron cultivadas en medio de Murashige y Skoog complementado con 22.7µM tidiazuron y 2.9µM ácido indol acético durante dos semanas. Los explantos fueron posteriormente transferidos a igual medio con 0.44µM N6 -benciladenina durante otras cuatro semanas. Se recogieron cinco muestras diarias durante las dos primeras semanas de tratamiento en medio con TDZ, procesando un total de 140 muestras. La mayoría de las yemas se desarrollan indirectamente a partir del callo formado en la superficie de corte del pecíolo. Después de dos-tres días de cultivo se observan los primeros cambios histológicos, con la desdiferenciación de algunas células de las capas subepidérmicas y del parénquima interno. La posterior proliferación de estas células da lugar a la formación de los meristemoides después de siete-diez días de cultivo. La progresiva diferenciación de estos meristemoides da lugar a la formación de las yemas que son visibles al exterior a partir de los 10-15 días. En la superficie adaxial del pecíolo se observó la formación de yemas adventicias de forma directa. Este protocolo puede ser de gran utilidad para la determinación de las células más adecuadas para los procesos de transformación genética.

Comparison of haploid and doubled haploid sugar beet clones in their ability to micropropagate and regenerate

Background: Haploid plant material is considered as recalcitrant to organogenesis, propagation, and maintenance in vitro. However, sugar beet (Beta vulgaris L.) breeders utilizing doubled haploid (DH) technology in their breeding programs indicate that sugar beet haploids may be cultured in vitro as well as diploids. Thus in this paper the in vitro performance of haploid and the doubled haploid sugar beet of various origin was evaluated. The DHs were derived from haploids by diploidization and twelve such haploid and corresponding DH clone pairs were obtained thus the comparison included haploid and DH clones that had identical allelic composition and differed only in their ploidy level. Results: The genotypes differed in shoot morphology and susceptibility to blackening during culture in vitro, but no significant differences were observed between the haploids and DHs. The micropropagation rate was, on average, higher for the haploids than DHs. Viability of the midrib and petiole explants after a 6-week culture was highly genotype dependent, but not affected by explant ploidy level. However, regeneration efficiency depended on both the genotype and ploidy level. The explants of several haploids regenerated more frequently and developed more adventitious shoots than the corresponding DHs thus overall efficiency was higher for haploids. Conclusions: The results obtained indicate that most of the haploids used in the comparison performed similar to or even better than DHs. This suggests that sugar beet haploid material can be successfully used not only for the production of DHs, but also maintained in vitro and utilized in projects requiring haploid tissues as the source material.

Indução e análise histológica de calos em explantes foliares de Jatropha curcas L. (Euphorbiaceae) / Induction and histological analysis of callus leaf explants of Jatropha curcas L. (Euphorbiaceae)

O objetivo deste trabalho foi avaliar o efeito de BAP e AIB sobre a formação de calos a partir de explantes foliares de Jatropha curcas L. (acesso JCUFS-012), descrever a curva de crescimento e realizar análise histológica dos calos. O delineamento experimental foi o inteiramente casualizado, em esquema fatorial 5x4, com cinco concentrações de BAP (0,0; 0,5; 1,0; 2,0 e 3,0 mg.L-1) e quatro de AIB (0,0; 0,5; 0,75 e 1,0 mg.L-1). Durante o experimento, a curva de crescimento dos calos foi acompanhada e mensurada aos 0, 5, 10, 15, 20, 25, 30, 35, 40, 45, 50, 55, 60 dias de cultivo. A análise histológica foi realizada a partir de calos crescidos em meio MS acrescido de 1,0 mg.L-1 de BAP e 0,5 mg.L-1 de AIB, após 60 dias de cultivo. A interação dos reguladores de crescimento BAP e AIB proporcionou a formação de calos compactos e posterior regeneração de brotações. Um maior número médio (6,2) de brotos por calo foi observado quando se adicionou ao meio de cultivo 1,65 mg.L-1 de BAP. A curva de crescimento de calos apresentou cinco fases distintas: lag, exponencial, linear, estacionária e desaceleração. Na análise histológica dos calos de J. curcas fica evidenciado a organogênese indireta pela formação de brotos adventícios, que apresentam conexão cambial com os tecidos dos calos.

The aim of this study was to evaluate the effect of IBA and BAP on callus formation from leaf explants of Jatropha curcas L. (accession JCUFS-012), describing the growth curve and histological analysis of the callus. The experimental design was completely randomized in a 5x4 factorial design with five concentrations of BAP (0.0, 0.5, 1.0, 2.0 and 3.0 mg. L-1) and four of IBA (0.0, 0.5, 0.75 and 1.0 mg.L-1). During the experiment, the growth curve of the calli was monitored and measured at 0, 5, 10, 15, 20, 25, 30, 35, 40, 45, 50, 55, 60 days of cultivation. Histological analysis was performed from calli grown on MS medium supplemented with 1.0 mg.L-1 of BAP and 0.5 mg.L-1 of IBA after 60 days of cultivation. The interaction of the growth regulators BAP and IBA provided the formation of compact calli and subsequent regeneration of shoots. A higher number (6.2) of shoots per callus was observed when 1.65 mg.L-1 of BAP was added to the culture medium. The growth curve of calli showed five distinct phases: lag, exponential, linear, stationary and deceleration. On histological analysis of callus J. curcas, indirect organogenesis was evidenced by the formation of adventitious shoots, that presented cambial connection with the callus tissue.

Rapid in vitro plant regeneration from leaf explants of Launaea sarmentosa (Willd.) Sch. Bip. ex Kuntze

An efficient protocol for organogenesis through leaves has been established for Launaea sarmentosa (Willd.) Sch. Bip. ex Kuntze, a highly valuable medicinal plant. The leaf explants produced microshoots on MS basal medium when fortified with cytokinins and auxins. A combination of 6-benzylaminopurine (BAP) at 0.5mg/l and naphthaleneacetic acid (NAA) at 0.2mg/l resulted in the induction of high frequency microshoots in 30 days. The microshoots were successfully subcultured for shoot elongation and eventually for rooting on MS medium supplemented with indole-3-butyric acid (IBA) at 0.5mg/l. The regenerated plantlets were hardened under greenhouse conditions and transferred to garden, resulting in a 90% survival rate.