Holistic protocol for callus culture optimization using statistical modelling

Fidemann, Tiago; Pereira, Gabriela Aparecida de Araujo; Nascimento, Lia Bossard; Moraes, Milena Cristina; Bertão, Mônica Rosa; Silva, Regildo Márcio Gonçalves da; Núñez, Eutímio Gustavo Fernández

doi:10.1080/14786419.2017.1380026

Cited by 2 publications

(3 citation statements)

References 18 publications

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“…1b) within the experimental domain under consideration. Besides, the antioxidant activities herein (suspension cell culture) were lower than those previously obtained for our group in callus culture with homologous basal culture medium and hormone supplementation, as well as, explant origin (7.58 ± 4.07%) (Fidemann et al 2017).…”

Section: Antioxidant Activitycontrasting

confidence: 71%

“…The detailed procedures for the culture initiation were previously reported (Fidemann et al 2016). With the aid of sterilized tweezers and scissors, explants were cut and inoculated in Petri dishes (15 × 100 mm) (five explants per dish) containing 35 mL Murashige and Skoog culture medium (MS) (pH 5.75) (Murashige and Skoog 1962) solidified with Phytagel (Sigma Chemical Co., St. Louis, MO) 4 g L −1 , supplemented with 3% sucrose and 2,4-d/BAP (5:1 ratio) at 1.138 mg L −1 (these conditions were optimized in previous work of our team) (Fidemann et al 2017). The culture media were previously autoclaved at 121 °C, 1 atm for 20 min.…”

Section: Callus Culturementioning

confidence: 99%

“…However, equivalent studies including C. baccatum species are scarce. Our group has been recently focused on the initial in vitro culture steps (in vitro germination and callus culture) for obtaining antioxidant compounds from C. baccatum species (Fidemann et al 2016(Fidemann et al , 2017.…”

Section: Introductionmentioning

confidence: 99%

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Handling culture medium composition for optimizing plant cell suspension culture in shake flasks

Fidemann

Pereira

Heluy

et al. 2017

Plant Cell Tiss Organ Cult

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This work aimed to optimize statistically the culture medium composition for cell plant suspension culture using as a model Capsicum baccatum L. var. pendulum cells. The cell growth was maximized as well as the secondary metabolite yields with antioxidant activity, which could find applications in pharmaceutical and food industries. A Box-Behnken statistical design was utilized to optimize the basal Murashige and Skoog medium, which is widely used in plant cell culture. Three relevant ingredients, saccharose (A, 15-45 g L −1), KH 2 PO 4 (B, 0.085-0.255 g L −1) and KNO 3 (C, 0.95-2.85 g L −1) were considered. The cell growth index as well as antioxidant activity, total phenolic compounds and flavonoids from dry extracts (DE) derived of cell cultures, were determined. Growth index (GI) and flavonoids content (F) were sensitive to the changes in nutrient composition in culture medium, and they were modeled statistically according to modified quadratic (GI = 1.76 + 0.59A − 0.32B − 0.42AC) and two-factor interaction (F(mg of rutin∕g DE) = 0.88 + 0.35AC − 0.29BC) models, respectively. Antioxidant activity and total polyphenols were independent of the nutrient concentrations within the range under study. The optimized culture medium composition was defined for two approaches: maximization of the cell growth (45 g L −1 saccharose, 0.09 g L −1 KH 2 PO 4 , 0.95 g L −1 KNO 3) and maximization of flavonoids production (45 g L −1 saccharose, 0.09 g L −1 KH 2 PO 4 , 2.85 g L −1 KNO 3). According to the current results, other elicitation strategies should be assessed to make this bioprocess more efficient for manufacturing secondary metabolites with antioxidant activity from suspension culture of Capsicum baccatum L. var. pendulum cells.

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Section: Antioxidant Activitycontrasting

confidence: 71%

Section: Callus Culturementioning

confidence: 99%

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Handling culture medium composition for optimizing plant cell suspension culture in shake flasks

Fidemann

Pereira

Heluy

et al. 2017

Plant Cell Tiss Organ Cult

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Plant Tissue Culture: A Potential Tool for the Production of Secondary Metabolites

Garg,

Datta,

Ahmad

2024

In Vitro Propagation and Secondary Metabolite Production From Medicinal Plants: Current Trends (Part 2)

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Plants are an immense source of phytochemicals with therapeutic effects and are widely used as life-saving drugs, and other products of varied applications. Plant tissue culture is a unique technique employed under aseptic conditions from different plant parts called explants (leaves, stems, roots, meristems, etc.) for in vitro regeneration and multiplication of plants and synthesis of secondary metabolites (SMs). Selection of elite germplasm, high-producing cell lines, strain enhancements, and optimization of media and plant growth regulators may lead to increased in vitro biosynthesis of SMs. Interventions in plant biotechnology, like the synthesis of natural and recombinant bioactive molecules of commercial importance, have attracted attention over the past few decades; and the rate of SMs biosynthesis has increased manifold than the supply of intact plants, leading to a quick acceleration in its production through novel plant cultures. Over the years, the production of SMs in vitro has been enhanced by standardising cultural conditions, selection of high-yielding varieties, application of transformation methods, precursor feeding, and various immobilization techniques; however, most often, SM production is the result of abiotic or biotic stresses, triggered by elicitor molecules like natural polysaccharides (pectin and chitosan) that are used to immobilize and cause permeabilization of plant cells. In vitro synthesis of SMs is especially promising in plant species with poor root systems, difficulty in harvesting, unavailability of elite quality planting material, poor seed set and germination, and difficult to propagate species. Thus, the present article reviews various biotechnological interventions to enhance commercially precious SMs production in vitro.

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Holistic protocol for callus culture optimization using statistical modelling

Cited by 2 publications

References 18 publications

Handling culture medium composition for optimizing plant cell suspension culture in shake flasks

Handling culture medium composition for optimizing plant cell suspension culture in shake flasks

Plant Tissue Culture: A Potential Tool for the Production of Secondary Metabolites

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