Stress and defense responses in plant secondary metabolites production

In the growth condition(s) of plants, numerous secondary metabolites (SMs) are produced by them to serve variety of cellular functions essential for physiological processes, and recent increasing evidences have implicated stress and defense response signaling in their production. The type and concentration(s) of secondary molecule(s) produced by a plant are determined by the species, genotype, physiology, developmental stage and environmental factors during growth. This suggests the physiological adaptive responses employed by various plant taxonomic groups in coping with the stress and defensive stimuli. The past recent decades had witnessed renewed interest to study abiotic factors that influence secondary metabolism during in vitro and in vivo growth of plants. Application of molecular biology tools and techniques are facilitating understanding the signaling processes and pathways involved in the SMs production at subcellular, cellular, organ and whole plant systems during in vivo and in vitro growth, with application in metabolic engineering of biosynthetic pathways intermediates.

Efeito do herbicida glifosato sobre o crescimento e produção de metabólitos secundários em Microcystis aeruginosa e Cylindrospermopsis raciborskii / The effect of herbicide glyphosate on the growth and of secondary metabolites production in Microcystis aeruginosa and Cylindrospermopsis raciborskii

ianobactérias, conhecidas por sua habilidade de sintetizar metabólitos com ação tóxica, podem se tornar dominantes em águas com altas concentrações de nitrogênio e fósforo. Embora a toxicidade do glifosato, o herbicida mais usado no mundo, em alguns organismos aquáticos seja conhecida, poucos estudos abordam o efeito desse composto sobre a produção de metabólitos secundários por cianobactérias. O objetivo deste trabalho foi avaliar a influência de diferentes concentrações de glifosato (produto técnico) sobre o crescimento e produção de cianotoxinas e microgininas pelas cepas brasileiras Microcystis aeruginosa LTPNA 08 e Cylindrospermopsis raciborskii CENA 302. Na presença de 15 mg/L de glifosato, o crescimento e a produção de toxinas pela M. aeruginosa foram reduzidos e de microgininas significativamente aumentada. Já a C. raciborskii, quando exposta à 20 mg/L de glifosato teve seu crescimento e síntese de clorofila-a, carotenoides e saxitoxinas aumentados. Concentrações superiores a 20 e 30 mg/L impediram o crescimento celular das cepas LTPNA 08 e CENA 302, respectivamente. A análise de ácidos graxos mostrou perfis bastante distintos entre as cepas. Na cepa LTPNA 08, enquanto que na presença de 10 mg/L de glifosato ocorreu diminuição do teor do ácido linoleico, o ácido estearidônico foi aumentado. Nenhuma das concentrações testadas promoveu alteração sobre o perfil de ácidos graxos da cepa CENA 302. A toxicidade de 5 produtos formulados a base de glifosato foi comparada ao produto técnico em ambas as linhagens-teste. Observou-se uma resistência distinta entre as cepas e toxicidade também variável entre as formulações comerciais. Sendo assim, diante da elevada resistência das cianobactérias M. aeruginosa e C. raciborskii ao glifosato, e considerando-se a elevada interferência antrópica através das práticas agrícolas, pode-se inferir que o uso excessivo e frequente desse herbicida é capaz de estimular o crescimento e dominância desses organismos, podendo modificar a estrutura e funcionalidade de ecossistemas aquáticos

Cyanobacteria, known for their ability to synthesize toxic metabolites, can become dominant in water bodies with high concentrations of nitrogen and phosphorus. Although the toxicity of glyphosate, the most widely used herbicide in the world, in some aquatic organisms is well known, few studies address the effect of this compound on the production of secondary metabolites by cyanobacteria. The aim of this study was to evaluate the influence of different concentrations the herbicide glyphosate (technical grade) on growth and production of cyanotoxins and microginins by Brazilian strains of Microcystis aeruginosa LTPNA 08 and Cylindrospermopsis raciborskii CENA 302. In the presence of 15 mg/L of glyphosate, growth and toxin production by M. aeruginosa were reduced and microginins cell quota significantly increased. The C. raciborskii strain, when exposed to 20 mg/L of glyphosate, had the growth, and chlorophyll-a, carotenoids and saxitoxins production increased. Concentrations above 20 and 30 mg/L prevented cell growth of LTPNA 08 and CENA 302 strains, respectively. Fatty acid analysis showed distinct profiles among the strains. When exposed to 10 mg/L of glyphosate, a decrease in the linoleic acid and increase in stearidonic acid content were observed in M. aeruginosa LTPNA 08 strain. None of the tested concentrations of glyphosate promoted change on the fatty acid profile of CENA 302 strain. The toxicity of 5 glyphosate formulated products was compared to technical product to both strains. There was a distinct resistance among strains and also a variable toxicity among formulated products. Thus, given the high glyphosate resistance of M. aeruginosa and C. raciborskii cyanobacteria, and considering the high anthropogenic interference through agri cultural practices, it can be inferred that excessive and frequent use of this herbicide is able to stimulate growth and dominance of these organisms, which may modify the structure and function of aquatic ecosystems

In vitro antioxidant capacity and free radical scavenging evaluation of active metabolite constituents of Newbouldia laevis ethanolic leaf extract

BACKGROUND: The aim of the present study was to evaluate the in vitro antioxidant and free radical scavenging capacity of bioactive metabolites present in Newbouldia laevis leaf extract. RESULTS: Chromatographic and spectrophotometric methods were used in the study and modified where necessary in the study. Bioactivity of the extract was determined at 10 µg/ml, 50 µg/ml, 100 µg/ml, 200 µg/ml and 400 µg/ml concentrations expressed in % inhibition. The yield of the ethanolic leaf extract of N.laevis was 30.3 g (9.93%). Evaluation of bioactive metabolic constituents gave high levels of ascorbic acid (515.53 ± 12 IU/100 g [25.7 mg/100 g]), vitamin E (26.46 ± 1.08 IU/100 g), saponins (6.2 ± 0.10), alkaloids (2.20 ± 0.03), cardiac glycosides(1.48 ± 0.22), amino acids and steroids (8.01 ± 0.04) measured in mg/100 g dry weight; moderate levels of vitamin A (188.28 ± 6.19 IU/100 g), tannins (0.09 ± 0.30), terpenoids (3.42 ± 0.67); low level of flavonoids (1.01 ± 0.34 mg/100 g) and absence of cyanogenic glycosides, carboxylic acids and aldehydes/ketones. The extracts percentage inhibition of DPPH, hydroxyl radical (OH.), superoxide anion (O2 .-), iron chelating, nitric oxide radical (NO), peroxynitrite (ONOO-), singlet oxygen (1O2), hypochlorous acid (HOCl), lipid peroxidation (LPO) and FRAP showed a concentration-dependent antioxidant activity with no significant difference with the controls. Though, IC50 of the extract showed significant difference only in singlet oxygen (1O2) and iron chelating activity when compared with the controls. CONCLUSIONS: The extract is a potential source of antioxidants/free radical scavengers having important metabolites which maybe linked to its ethno-medicinal use.

Induction of secondary metabolite production by UV-C radiation in Vitis vinifera L. Öküzgözü callus cultures

BACKGROUND: The aim of the present work was to examine the role of UV-C irradiation on the production of secondary metabolites (total phenolic, total flavanols, total flavonols, catechin, ferulic acid and trans-resveratrol in phenolic compounds and α-, ß-, γ- δ-tocopherols) in callus cultures. Studies on the effects of UV-C treatment on callus culture are seldom and generally focused on UV-B. However UV-C radiation play an important role in accumule secondary metabolites. RESULTS: In this study, callus cultures from Öküzgözü grape cultivar were initiated from leaf petiole explants. Calli formed after 6 weeks on the medium supplemented with 0.5 mg L-1 benzylaminopurine (BA), 0.5 mg L-1 indole acetic acid (IAA) on B5 media. Callus tissues were exposed to UV-C irradiation at 10, 20 and 30 cm distances from the UV source for 5 and 10 minutes and samples were collected at hours 0, 24 and 48. CONCLUSIONS: The greatest total phenolic content (155.14 mg 100 g-1) was detected in calli exposed to UV-C for 5 min from 30 cm distance and sampled after 24 h. 24 h and 48 h incubation times, 30 cm and 5 min were the most appropriate combination of UV-C application in total flavanol content. Maximum total flavonol content (7.12 mg 100 g-1) was obtained on 0 h, 5 min and 20 cm combination. The highest (+)- catechin accumulation (8.89 mg g-1) was found in calli with 10 min UV-C application from 30 cm distance and sampled after 48 h. Ferulic acid content increased 6 fold in Öküzgözü callus cultures (31.37 µg g-1) compared to the control group. The greatest trans-resveratrol content (8.43 µg g-1) was detected in calli exposed to UV-C for 5 min from 30 cm distance and sampled after 24 h. The highest α-tocopherol concentration was found in calli exposed to UV-C for 10 min from 30 cm distance and sampled after 24 h. As a conclusion, it was showed that UV-C radiation had remarkable promoting effects on the accumulation of secondary metabolites in the calli of Öküzgözü grape cultivar.

Efeito de dinamizações de Arnica montana L. no metabolismo de chambá (Justicia pectoralis Jacq. ) / Effect of dynamizations of Arnica montana in metabolism of chambá (Justicia pectoralis Jacq. )

Este estudo objetivou avaliar a resposta do crescimento e do metabolismo secundário de Justicia pectoralis, expresso em produção de cumarina, a crescentes dinamizações de A. montana. O experimento foi conduzido na Universidade Federal de Viçosa. O delineamento estatístico foi inteiramente casualizado, com seis repetições e cinco tratamentos, totalizando 30 parcelas experimentais, sendo cada parcela constituída de uma planta por vaso. Os tratamentos foram as dinamizações 3CH, 30CH, 60CH, 100CH e 200CH do preparado homeopático A. montana. Os tratamentos foram aplicados às plantas via pulverização, em intervalos semanais, iniciando logo após o plantio. Após quatro meses do plantio as plantas foram colhidas. As características de crescimento avaliadas foram matérias fresca e seca de folhas e caules, matérias fresca e seca de inflorescências e matérias fresca e seca total. No estudo fitoquímico foi avaliada a produção da cumarina (1-2 benzopirona). Não houve resposta nas variáveis de crescimento aos tratamentos. As dinamizações de A. montana causaram alterações no metabolismo secundário das plantas. Os conteúdos de cumarina das plantas com A. montana 3CH e 30CH foram próximos e mais baixos, aumentando progressivamente a partir de 60CH, chegando ao máximo em 100CH, seguido de redução em 200CH. A preparação homeopática A. montana causa alterações no metabolismo secundário de chambá, sendo as repostas dependentes da dinamização.

Were evaluated the responses to dynamizations of Arnica montana in the growth and in the secondary metabolism of Justicia pectoralis expressed as coumarin production. The studies were carried out at the Universidade Federal de Viçosa. The statistical design was completely randomized, with six replicates and five treatments, 30 experimental plots, one plant per pot. The treatments were dynamizations 3CH, 30CH, 60CH, 100CH and 200CH homeopathic preparation of A. montana. The application the treatments begun are planting seedlings, the aerial part being sprayed, at weekly intervals. After four months of planting, the plants were harvested. The evaluated growth characteristics were: fresh and dry matter of leaves and stems, fresh and dry matter of inflorecenses, and fresh and dry matter total. In the phytochemistry study, the production of the coumarin 1,2-benzopyrone was evaluated. Were no responses of growth characteristics. The dynamizations of A. montana caused changes in secondary metabolism of plants. The coumarin production with A. montana plants 3CH and 30CH were lower, increasing progressively from 60CH, and coming to increased in 100CH, followed by a large reduction in the 200CH. The homeopathic preparation A. montana cause change in secondary metabolism of chambá, and the responses depend on dynamizations.