The objective of this work was the optimization of the conditions of in vitro culture for callus production of Silybum marianum (L.) Gaertn. (Asteraceae). Sections of cotyledons, previously disinfected by washing successively with ethanol 70º, NaClO (10% w/v) and Tween 20 (0.05% v/v) and rinsing with sterile distilled water, were used as explants. For its initial culture, B5 medium supplemented with BA and 2,4-D solidified with phytagel was used, and a 63% survival was achieved. To obtain callus, two solid media were assayed (S1 and S2) using B5 medium supplemented with growth regulators (BA and 2,4-D or NAA and BA, respectively). The calli were grown at 25ºC during 45 days in darkness. Growth kinetics was studied using S1 medium obtaining a typical growth curve with an exponential phase after 14 days of incubation (rate of growth 0.005 g dry weight/ day) and stationary phase after 35 days. The rate of growth in S2 medium was slower, and rhizogenesis was observed starting on the fifth week of incubation. From these results, the best culture medium for callus production of Silybum marianum was S1 medium.Facultad de Ciencias Exacta

Cimino, Cecilia Verónica

Natalucci, Claudia Luisa

Priolo de Lufrano, Nora Silvia

Spina, Francisco

Vairo Cavalli, Sandra Elizabeth

Electronic Journal of Biotechnology

English

SEDICI - Repositorio de la UNLP

Electronic Journal of Biotechnology ISSN: 0717-3458                                                                                         Vol.9 No.3, Special Issue, 2006 
© 2006 by Pontificia Universidad Católica de Valparaíso -- Chile                                       
This paper is available on line at http://www.ejbiotechnology.info/content/vol9/issue3/full/14/ 
DOI: 10.2225/vol9-issue3-fulltext-14                                                                                                      RESEARCH ARTICLE 
 
 
Callus culture for biomass production of milk thistle as a potential source 
of milk clotting peptidases 
Cecilia Cimino 
Laboratorio de Investigación de Proteínas Vegetales 
Universidad Nacional de La Plata 
La Plata 47 y 115, CC 711, 1900 
La Plata. Argentina 
Tel: 54 221 4235333 ext. 57 
Fax: 54 221 422 4067 
E-mail: cvcimino@biol.unlp.edu.ar 
Sandra Vairo Cavalli 
Laboratorio de Investigación de Proteínas Vegetales 
Universidad Nacional de La Plata 
La Plata 47 y 115, CC 711, 1900 
La Plata. Argentina 
Tel: 54 221 4235333 ext. 57 
Fax: 54 221 422 4067 
E-mail: svairo@biol.unlp.edu.ar  
Francisco Spina 
Laboratorio de Investigación de Proteínas Vegetales 
Universidad Nacional de La Plata 
La Plata 47 y 115, CC 711, 1900 
La Plata. Argentina 
Tel: 54 221 4235333 ext. 57 
Fax: 54 221 422 4067 
E-mail: frankspina1@hotmail.com  
Claudia Natalucci 
Laboratorio de Investigación de Proteínas Vegetales 
Universidad Nacional de La Plata 
La Plata 47 y 115, CC 711, 1900 
La Plata. Argentina 
Tel: 54 221 4235333 ext. 57 
Fax: 54 221 422 4067 
E-mail: natalucci@biol.unlp.edu.ar 
Nora Priolo* 
Laboratorio de Investigación de Proteínas Vegetales 
Universidad Nacional de La Plata 
La Plata 47 y 115, CC 711, 1900 
La Plata. Argentina 
Tel: 54 221 4235333 ext. 57 
Fax: 54 221 422 4067 
E-mail: priolo@biol.unlp.edu.ar 
Financial support: The present work was supported by grants from ANPCyT, CIC, CONICET, CYTED, and UNLP.  
Keywords: Asteraceae, callus, rhizogenesis, Silybum marianum. 
Abbreviations: 2,4-D: dichlorophenoxy acetic acid 
BA: benzyladenine 
NAA: naphtalenacetic acid 
 
The objective of this work was the optimization of the 
conditions of in vitro culture for callus production of 
Silybum marianum (L.) Gaertn. (Asteraceae). Sections of 
cotyledons,     previously     disinfected      by      washing  
*Corresponding author 
successively with ethanol 70º, NaClO (10% w/v) and 
Tween 20 (0.05% v/v) and rinsing with sterile distilled 
water, were used as explants. For its initial culture, B5 
medium supplemented with BA and 2,4-D solidified 
 
Cimino, C. et al. 
 238
with phytagel was used, and a 63% survival was 
achieved. To obtain callus, two solid media were assayed 
(S1 and S2) using B5 medium supplemented with 
growth regulators (BA and 2,4-D or NAA and BA, 
respectively). The calli were grown at 25ºC during 45 
days in darkness. Growth kinetics was studied using S1 
medium obtaining a typical growth curve with an 
exponential phase after 14 days of incubation (rate of 
growth 0.005 g dry weight/ day) and stationary phase 
after 35 days. The rate of growth in S2 medium was 
slower, and rhizogenesis was observed starting on the 
fifth week of incubation. From these results, the best 
culture medium for callus production of Silybum 
marianum was S1 medium. 
Enzyme preparations, from extracts of plants or animal 
tissue, were used well before much was known about the 
nature and properties of enzymes. The great majority of 
commercial enzymes have been obtained mainly from 
microbial sources. Plant enzymes, such as papain, 
bromelain and ficin (cysteine peptidases) are employed in 
different industrial processes and medicine (Uhlig, 1998). 
All enzymes employed in milk coagulation are aspartic 
peptidases, with acidic optima pH, and possess high levels 
of homology between their primary structures and  
similarity between their catalytic mechanisms (Silva and 
Malcata, 1999). 
The flowers of different species of cardoon (Asteraceae) 
have been characterized because they are a rich source of 
aspartic peptidases with milk clotting activity (Veríssimo et 
al. 1996; Cordeiro et al. 1998; Llorente et al. 2004). Since 
Roman times, aqueous extracts of Cynara cardunculus 
flowers have been used as a milk coagulant in the 
manufacture of various types of the Iberian Peninsula 
traditional cheeses such as Serra da Estrela cheese, Serpa, 
Azeitão, Los Pedroches, La Serena and Flor de Guía (Silva 
and Malcata, 1999; Silva et al. 2002). 
The presence of aspartic peptidases with milk clotting 
activity has been detected in crude aqueous extracts of 
flowers of milk thistle, Silybum marianum (L.) Gaertn. 
(Asteraceae), (Vairo Cavalli et al. 2005) and the use of its 
flowers and leaves for the production of small-scale Serpa 
cheese has been reported (Cabral et al. 1984). 
One of the reasons for research on various plant cell, tissue 
or organ cultures is the ability of these cultures to 
synthesize in vitro some of the metabolites that are found in 
the whole plants (Tamer and Mavituna, 1996). Thus, this 
becomes an alternative for obtaining products that are 
difficult to obtain by conventional methods or whose 
production is not economically viable. Furthermore, plant 
enzyme supply tends to be erratic and influenced by climate 
and season which determinates its uselessness in a full-
scale cheese industry. 
Cabral et al. (1984) have immobilized cells and protoplasts 
obtained from S. marianum cell suspension cultures with 
milk clotting activity, but the peptidases responsible for the 
activity have not been characterized. 
The aim of the present work is the optimization of callus 
culture of Silybum marianum (Asteraceae), milk thistle, for 
biomass production as a potential source of milk clotting 
peptidases. The media chosen were selected due to its 
usefulness for the in vitro production of peptidases with 
milk clotting activity in different species of Asteraceae. 
(Fevereiro et al. 1986). 
MATERIALS AND METHODS 
Explants 
Achenes of Silybum marianum (L.) Gaertn. (Marzocca, 
1957) were washed under tap water for 24 hrs and began to 
germinate in seedbeds for 2 weeks and kept at an 8 hrs light 
/ 8 hrs dark photoperiod. The seedbeds remained during this 
time in trays with provision of water. The plantlets were 
scrupulously washed and its cotyledons were chopped in 
two parts that were used as explants for callus production. 
Plant material disinfection 
For disinfection of plant material destined to in vitro 
cultures, assays were done varying the times of exposition 
and the concentrations of the agents used (ethanol and 
sodium hypochlorite). The method selected consisted in 
disinfecting the plant material successively washing it with 
ethanol 70o for 5 min, NaClO 10% for 10 min and Tween 
20 (0.05% v/v) for 15 min. They were finally washed 
thoroughly three times with sterile distilled water in a 
laminar flux chamber. 
 
 
Figure 1. Variation of dry weight from S. marianum callus 
obtained in S1 medium during growth time. 
 
Callus culture for biomass production of milk thistle as a potential source of milk clotting peptidases 
 
 239
Callus initiation and production 
The basal medium used was B5 (Gamborg et al. 1968) 
supplemented with 0.05 mg/l of BA and 0.5 mg/l of 2,4-D, 
and solidified with 2.5 g/l of phytagel. The pH was adjusted 
to 5.8. Explants obtained from 60 plantlets were incubated 
at 24 ± 2ºC in darkness during 45 days. 
The calli obtained this way were inoculated in two solid 
media. The media assayed (S1 and S2) were B5 medium 
solidified with 2.5 g/l of phytagel and supplemented with 
growth regulators (BA and 2,4-D or NAA and BA 
respectively). S1 medium was supplemented with 0.05 mg/l 
of BA and 0.5 mg/l of 2,4-D; S2 medium was 
supplemented with 0.025 mg/l of BA and 0,01 mg/l of 
NAA. These hormonal supplements were selected because 
they were optimum for the production in vitro of peptidases 
with milk clotting activity in different species of Asteraceae 
(Fevereiro et al. 1986). In both cases the pH was adjusted to 
5.8. The media were sterilized in autoclave at 1 atmosphere 
of overpressure for 20 min. The callus were grown at 24 ± 
2ºC during 45 days of incubation in the darkness. 
Growth kinetics was studied by determination of dry weight 
of fresh callus at 7, 14, 21, 28, 35 and 42 days old. Dry 
weight of fresh callus was determined after drying in a 
vacuum oven at 65ºC until constant weight. 
RESULTS AND DISCUSSION  
After surface sterilization, 63% of survival was achieved 
and 25% of the samples were contaminated. Longer periods 
of contact with the NaClO produced the death of the 
explants. A good response was obtained when the explants 
were inoculated on the selected medium. 
Other authors when assaying different media for the 
obtention of calli of Cynara cardunculus supplemented 
with different combinations of kinetin and NAA, 
combinations of kinetin and 2,4-D, and combinations of BA 
and 2,4-D, have obtained the best biomass production using 
B5 medium supplemented with BA and 2,4 D in relation 
1:10 (Figueiredo et al. 1987). In the present work the best 
response in terms of biomass production was obtained 
using S1 medium. 
Growth kinetics in S1 medium showed a typical curve with 
an exponential growth phase that began after 14 days of 
incubation and stationary growth phase that began after 35 
days. The rate of growth during the exponential growth 
phase was of 0.005 g (dry weight)/day, with correlation 
coefficient of 0.99 (Figure 1). 
On the contrary, the rate of growth in S2 medium was 
slower (Figure 2), and produced rhizogenesis (Figure 3) 
starting on the fifth week of incubation. When media 
supplemented with different proportions of BA and NAA 
for obtaining of calli from Cynara scolymus L. 
(Asteraceae) were assayed, the best results were achieved 
using a ratio BA/NAA of 1:10. 
CONCLUDING REMARKS 
From the results obtained, the best culture medium for 
callus production for biomass production of milk thistle 
(Silybum marianum) as a potential source of milk clotting 
peptidases was B5 medium solidified with 2.5 g/l of 
phytagel and supplemented with 0.05 mg/l of BA and 0.5 
mg/l of 2,4-D. 
ACKNOWLEDGMENTS 
S. Vairo-Cavalli is awarded fellowship by CONICET and 
C.L. Natalucci is member of CIC Researcher Career. 
Authors also thank Tolbiac S.R.L. and Mr. José Madarnas 
for the supply of de Silybum marianum seeds. 
 
 
Figure 2. Variation of dry weight from S. marianum callus 
obtained in S2 medium during growth time 
 
 
Figure 3. Rhizogenesis from culture callus in S2 medium. 
Cimino, C. et al. 
 240
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Callus culture for biomass production of milk thistle as a potential source of milk clotting peptidases

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Callus culture for biomass production of milk thistle as a potential source of milk clotting peptidases

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