Silicon confers cucumber resistance to salinity stress through regulation of proline and cytokinins.

Salt stress is a continuous threat to global crop production. Here, we studied the alleviation role of exogenous silicon (Si) in NaCl-stressed cucumber, with special emphasis on plant growth, proline (Pro) and hormone metabolisms. The results showed that Si supplementation ameliorated the adverse effects of NaCl on plants growth, biomass, and oxidative stress. Salt stress greatly increased the content of Pro throughout the experiment, while Si regulated Pro content in two distinct ways. Si promoted the salt-induced Pro levels after 3 and 6 days of treatment, but decreased it after 9 and 12 days of treatment. Moreover, P5CS and ProDH activities and P5CS gene play important roles in Si and salt-regulated Pro levels in different stress phase. Under stress condition, Si addition tend to revert the content of ABA, IAA, cytokinin and SA to the control levels in most cases. Further correlation analysis revealed a negative correlation between the root cytokinin and Pro content after 3 days of treatment, suggesting the interaction between cytokinin and Pro metabolism. Exogenous application of Pro and ProDH competitive inhibitor D-Lactate confirmed the possible interplay between Pro and cytokinin metabolism. Further study identified several CKX (Csa4G647490 and Csa1G589070) and IPT (Csa7G392940 and Csa3G150100) genes that may be responsible for the regulation of cytokinin accumulation by Si and/or Pro after short-term of treatment. The results suggested that Pro is a key factor in Si-induced salt tolerance, and Si-increased Pro content may participate in the regulation of cytokinin metabolism under short-term of salt stress.

Effects of maternal L-proline supplementation on inflammatory cytokines at the placenta and fetus interface of mice.

Dietary L-proline (proline) supplementation during gestation enhances fetal survival and placental development in mice. The objective of the present study was to test the hypothesis that this beneficial effect of proline was associated with alterations in inflammatory response at the placenta and fetus interface. Populations of immune cells present in peripheral blood mononuclear cells (PBMC) were determined by flow cytometry analysis. The concentrations of immunoglobulins in plasma, and the concentrations of cytokines in plasma, uterus, placenta, and amniotic fluid were measured using a bead-based immunoassay. The data showed that proline supplementation led to higher (P < 0.05) populations of B lymphocytes (CD3-CD19+), natural killer (NK) cells (CD3-NK1.1+), and dendritic cells (DCs, CD11c+MHCII+) in peripheral blood, as compared with the controls. Conversely, mice fed a proline-supplemented diet had a lower population of neutrophils (CD11b+F4/80-). Further study showed that proline supplementation decreased (P < 0.05) the concentrations of (1) interleukin (IL)-23, IL-1α, and IL-6 in plasma; (2) IL-6 in the uterus; and (3) tumor necrosis factor alpha (TNF-α), monocyte chemotactic protein (MCP)-1, and IL-17 in the placenta; and (4) interferon (IFN)-γ in amniotic fluid, compared with controls. Conversely, proline supplementation resulted in higher (P < 0.05) concentrations of (1) IL-10, IL-17 and granulocyte-macrophage colony-stimulating factor (GM-CSF) in plasma; (2) IL-10 and IL-1α in the uterus; and (3) IL-1α, IL-1ß, IL-10, IL-27, and IFN-ß in amniotic fluid, compared with controls. Moreover, concentrations of immunoglobulin (Ig) G2b and IgM were enhanced (P < 0.05) by proline administration. Taken together, our results reveal a regulatory effect of proline in the immunological response at the maternal-fetal interface, which is critical for embryonic development and fetal survival.

Validación de un método por CLAR para la cuantificación de L-prolina en la tintura al 20 por ciento de Murraya paniculata L Jack / Validation of a high performance liquid chromatography method for quantitation of L-proline in 20 percent tincture from Murraya paniculata L Jack

Introducción: la búsqueda de técnicas analíticas para el control de la calidad de los medicamentos constituye un aspecto de gran interés en el campo farmacéutico, más si van dirigidas al estudio del o los marcadores químicos de las plantas medicinales, sus extractos y fitomedicamentos. Objetivo: validar un método de cromatografía líquida de alta resolución (CLAR) para la determinación cuantitativa del aminoácido L-prolina como sustancia marcador en la tintura de Murraya paniculata L. Jack. Métodos: en el método por CLAR, la separación se realizó en una columna C-18 (UP5ODB-150/046), se utilizó como fase móvil una mezcla de solución buffer fosfato, pH ajustado a 2,4 y acetonitrilo (70:30 v/v), con una velocidad de flujo de 0,6 mL/min, modo isocrático, con detección ultravioleta a 440 nm. El volumen de inyección de la muestra fue de 20 µL. El método fue validado según la categoría I, siguiendo las exigencias internacionales. Resultados: la curva de calibración fue lineal en el rango de concentraciones ensayadas (30 a 375 µg/mL), se observó una buena precisión con coeficientes de variación menores del 2 por ciento. Los valores de recobrado estuvieron dentro de los límites establecidos para los métodos cromatográficos (98-102 por ciento). Se demostró la especificidad del método, al no presentarse interferencias de picos adicionales en la zona de elusión del compuesto de interés (L-prolina). Conclusiones: el método analítico por CLAR, validado para la cuantificación del aminoácido L-prolina en la tintura de M. paniculata, demostró ser lineal, preciso, exacto y específico bajo las condiciones de estudio(AU)

Introduction: the search for analytical methods that may monitor the quality of drugs is an issue of great interest in the pharmaceutical field, even more if they are directed to studying chemical markers of medicinal plants, their extracts and phytomedicines. Objective: to validate a high-resolution liquid chromatography (HPLC) method for the quantitative determination of the L-proline amino acid as a marker substance in Murraya paniculata L. Jack tincture. Methods: in the HPLC, the separation was performed on a C-18 (UP5ODB-150/046) column, with a mixture of phosphate buffer solution, pH adjusted to 2.4 and acetonitrile (70:30 v/v) used as mobile phase, the flow rate was 0.6 mL/min, isocratic mode with UV detection set at 440 nm. The injection volume of the sample was 20 ÁL. The method was validated according to category I, following international requirements. Results: the calibration curve was linear over the concentration range tested (30-375 mg/mL), good precision was observed with a variation coefficient less than 2 percent. Recovery values were within the limits for chromatographic methods (98-102 percent). The method was specific since there was no-interference by additional peaks in the elution zone of the compound in question (L-proline). Conclusions: the HPLC analytical method, validated for the quantification of L-proline amino acid in M. paniculata tincture, proved to be linear, precise, accurate and specific under the study conditions(AU)

Validación de un método por CLAR para la cuantificación de L-prolina en la tintura al 20 por ciento de Murraya paniculata L. Jack / Validation of a high performance liquid chromatography method for quantitation of L-proline in 20 percent tincture from Murraya paniculata L. Jack

INTRODUCCIÓN: la búsqueda de técnicas analíticas para el control de la calidad de los medicamentos constituye un aspecto de gran interés en el campo farmacéutico, más si van dirigidas al estudio del o los marcadores químicos de las plantas medicinales, sus extractos y fitomedicamentos. OBJETIVO: validar un método de cromatografía líquida de alta resolución (CLAR) para la determinación cuantitativa del aminoácido L-prolina como sustancia marcador en la tintura de Murraya paniculata L. Jack. MÉTODOS: en el método por CLAR, la separación se realizó en una columna C-18 (UP5ODB-150/046), se utilizó como fase móvil una mezcla de solución buffer fosfato, pH ajustado a 2,4 y acetonitrilo (70:30 v/v), con una velocidad de flujo de 0,6 mL/min, modo isocrático, con detección ultravioleta a 440 nm. El volumen de inyección de la muestra fue de 20 µL. El método fue validado según la categoría I, siguiendo las exigencias internacionales. RESULTADOS: la curva de calibración fue lineal en el rango de concentraciones ensayadas (30 a 375 µg/mL), se observó una buena precisión con coeficientes de variación menores del 2 por ciento. Los valores de recobrado estuvieron dentro de los límites establecidos para los métodos cromatográficos (98-102 por ciento). Se demostró la especificidad del método, al no presentarse interferencias de picos adicionales en la zona de elusión del compuesto de interés (L-prolina). CONCLUSIONES: el método analítico por CLAR, validado para la cuantificación del aminoácido L-prolina en la tintura de M. paniculata, demostró ser lineal, preciso, exacto y específico bajo las condiciones de estudio(AU)

INTRODUCTION: the search for analytical methods that may monitor the quality of drugs is an issue of great interest in the pharmaceutical field, even more if they are directed to studying chemical markers of medicinal plants, their extracts and phytomedicines. OBJECTIVE: to validate a high-resolution liquid chromatography (HPLC) method for the quantitative determination of the L-proline amino acid as a marker substance in Murraya paniculata L. Jack tincture. METHODS: in the HPLC, the separation was performed on a C-18 (UP5ODB-150/046) column, with a mixture of phosphate buffer solution, pH adjusted to 2.4 and acetonitrile (70:30 v/v) used as mobile phase, the flow rate was 0.6 mL/min, isocratic mode with UV detection set at 440 nm. The injection volume of the sample was 20 µL. The method was validated according to category I, following international requirements. RESULTS: the calibration curve was linear over the concentration range tested (30-375 mg/mL), good precision was observed with a variation coefficient less than 2 percent. Recovery values were within the limits for chromatographic methods (98-102 percent). The method was specific since there was no-interference by additional peaks in the elution zone of the compound in question (L-proline). CONCLUSIONS: the HPLC analytical method, validated for the quantification of L-proline amino acid in M. paniculata tincture, proved to be linear, precise, accurate and specific under the study conditions(AU)

Inhibition of ribonuclease and protease activities in arsenic exposed rice seedlings: role of proline as enzyme protectant.

When seedlings of two rice (Oryza sativa L.) cvs. Malviya-36 and Pant-12 were raised under 25 and 50 microM As2O3 in the medium an increase in the level of RNA, proteins and proline accompanied with a decline in the level of free amino acid pool was observed under arsenic supplementation compared to controls. In situ As3+ treatment caused a marked inhibition in activities of ribonuclease (RNase, EC 3.1.27.1), protease and leucine aminopeptidase (LAP, EC 3.4.11.1) whereas the activity level of carboxypeptidase (EC 3.4.16.5) was enhanced. In vitro supply of As2O3 in the enzyme assay medium beyond 400 microM resulted in gradual inhibition of RNase and beyond 5 microM inhibition of LAP activities. Addition of 1M proline in the assay medium significantly restored the loss in RNase activity due to in vitro arsenic treatment or due to osmotic stress created by incorporation of polyethylene glycol (PEG). Isoform pattern of RNase extracted from As3+ -exposed seedlings showed a significant alteration compared to its pattern in unexposed seedlings. Results suggest that arsenic exposure impairs hydrolysis of RNA and proteins in rice seedlings due to inhibition of RNase and proteases activities and that proline accumulating under As3+ toxicity appears to serve as enzyme protectant.

Copper-induced oxidative stress in the chlorophycean microalga Chlorella vulgaris: response of the antioxidant system.

A concentration dependent increase in lipid peroxidation, carotenoid content and activity of superoxide dismutase was observed in the green microalga Chlorella vulgaris following copper exposure. In contrast, activities of catalase, ascorbate peroxidase and glutathione reductase, and the cellular GSH, ascorbate and K+ pool depicted a reverse trend. However, a significant rise in intracellular proline content was also evident in copper supplemented cultures. Though this study depicted the malfunction of the major antioxidant system of C. vulgaris under copper stress the test organism was found to survive and grow even at 3.0 microg mL(-1) of Cu treatment (32% growth). Further study is needed to establish the role of proline in metal toxicity regulation.

Functional analysis of homologs of translation initiation factor 2gamma in yeast.

The gamma subunit of eukaryotic translation initiation factor 2 is an EF-Tu-like protein that plays an essential role in protein synthesis. We have isolated an eIF-2gamma homolog from the fission yeast Schizosaccharomyces pombe that complements a gcd11 null allele in Saccharomyces cerevisiae. GCD11 is an essential gene that encodes S. cerevisiae eIF-2gamma. Comparison among three eIF-2gamma homologs from humans, S. cerevisiae, and S. pombe, and a putative Drosophila homolog, reveals the presence of a domain N-terminal to the GTP-binding (G) domain that varies in length (relative to EF-Tu) from 12 residues in S. pombe to 89 residues in S. cerevisiae. In S. cerevisiae, these sequences are not essential for function. However, unlike a deletion, a missense mutation in this domain confers a slow growth phenotype and constitutively derepresses expression of the GCN4 transcriptional activator. The eIF-2gamma homologs also contain a partially conserved 35-37 amino acid insertion in the G domain that is absent from EF-Tu and other G proteins. Unlike the variable N-terminal domain, these residues are required for the essential function of eIF-2gamma.