Synchrotron-Based Techniques Shed Light on Mechanisms of Plant Sensitivity and Tolerance to High Manganese in the Root Environment

Plant species differ in response to high available manganese (Mn), but the mechanisms of sensitivity and tolerance are poorly understood. In solution culture, greater than or equal to 30 µm Mn decreased the growth of soybean (Glycine max), but white lupin (Lupinus albus), narrow-leafed lupin (Lupin angustifolius), and sunflower (Helianthus annuus) grew well at 100 µm Mn. Differences in species’ tolerance to high Mn could not be explained simply by differences in root, stem, or leaf Mn status, being 8.6, 17.1, 6.8, and 9.5 mmol kg^–1 leaf fresh mass at 100 µm Mn. Furthermore, x-ray absorption near edge structure analyses identified the predominance of Mn(II), bound mostly to malate or citrate, in roots and stems of all four species. Rather, differences in tolerance were due to variations in Mn distribution and speciation within leaves. In Mn-sensitive soybean, in situ analysis of fresh leaves using x-ray fluorescence microscopy combined with x-ray absorption near edge structure showed high Mn in the veins, and manganite [Mn(III)] accumulated in necrotic lesions apparently through low Mn sequestration in vacuoles or other vesicles. In the two lupin species, most Mn accumulated in vacuoles as either soluble Mn(II) malate or citrate. In sunflower, Mn was sequestered as manganite at the base of nonglandular trichomes. Hence, tolerance to high Mn was ascribed to effective sinks for Mn in leaves, as Mn(II) within vacuoles or through oxidation of Mn(II) to Mn(III) in trichomes. These two mechanisms prevented Mn accumulation in the cytoplasm and apoplast, thereby ensuring tolerance to high Mn in the root environment.Manganese (Mn) is an essential element for plant growth, but its availability differs greatly in space and time, depending largely on the nature and amount of Mn minerals present and on the soil’s pH and redox potential. With an elaborate chemistry, Mn forms complexes with many organic and inorganic ligands. In soils, Mn has three common oxidation states, Mn(II), Mn(III), and Mn(IV), which form hydrated oxides of mixed valency; Mn is present also as numerous carbonates, silicates, sulfates, and phosphates (Lindsay, 1979). Cationic Mn²⁺ is the most common form readily absorbed by plant roots (Clarkson, 1988). The toxicity of Mn occurs in acid or waterlogged soils high in Mn minerals.Many plants have mechanisms to accommodate the large differences in Mn²⁺ in soils. At low available Mn, uptake is increased in some Poaceae by excretion of phytosiderophores of the mugineic acid family (Takahashi et al., 2003), with root phytase exudation also potentially important for acquisition of Mn when Mn availability is limited (George et al., 2014). Mechanisms in other plants include the ability of roots to decrease rhizosphere pH or excrete organic ligands (Neumann and Romheld, 2012; Lambers et al., 2015). However, the relative importance of the many complexes on Mn uptake remains unclear. Toxicity results from high Mn in leaf cell walls (Wissemeier et al., 1992; Wissemeier and Horst, 1992) and through adverse effects on symplastic proteins (Führs et al., 2008). Many plants have mechanisms that limit the adverse effects of high Mn²⁺ in soils, with numerous ligands involved in its translocation and that of other essential cations (Haydon and Cobbett, 2007). Edwards and Asher (1982) classified a range of crop and pasture species based on their ability to deal with high Mn as those that (1) limit Mn from entering the roots, (2) retain Mn in the roots, or (3) tolerate high Mn in the shoots. At the extreme are plants that hyperaccumulate more than 10,000 mg Mn kg^–1 on a dry mass (DM) basis in foliar tissues without metabolic damage (Fernando et al., 2013; van der Ent et al., 2013). Based on 15% DM of leaves, this equates to 12.1 mmol kg^–1 on a fresh mass (FM) basis. Celosia argentia, a species adapted to growth on Mn-contaminated mine tailings, accumulated more than 20,000 mg kg^–1 Mn in leaves (Liu et al., 2014). Tolerance of high Mn in shoots of some Mn hyperaccumulators has been found to occur through binding to ligands (such as malate or citrate) or sequestration in the vacuole (Fernando et al., 2010).Characteristic symptoms of Mn toxicity include chlorotic and distorted leaves with small necrotic lesions. These lesions have been shown in cowpea (Vigna unguiculata) to contain oxidized Mn and callose (Wissemeier et al., 1992), which forms as a reaction to high intracellular Ca (Kartusch, 2003). The necrotic lesions result mainly from oxidized phenolics (Wissemeier and Horst, 1992) and increased peroxidase activity in the apoplast (Horst et al., 1999). With a critical solution concentration for toxicity (10% growth reduction) of no more than 9 µm Mn, Edwards and Asher (1982) found that cotton (Gossypium hirsutum), bean (Phaseolus vulgaris), cowpea, and soybean (Glycine max) were the most sensitive species of 13 crop and pasture plants grown for 18 to 31 d at constant Mn in solution culture. By contrast, the critical concentration for sunflower (Helianthus annuus) was 7 times higher at 65 µm Mn. Sunflower was the first species found to tolerate high Mn through its sequestration in the trichomes on stems, petioles, and leaves (Blamey et al., 1986). The suspected accumulation of Mn was confirmed using wavelength dispersive x-ray spectroscopy with darkening inferred as due to insoluble higher oxides of Mn. Similarly, high Mn results in darkened trichomes of cucumber (Cucumis sativus) leaves due to oxidized Mn, as shown by the colorimetric benzidine test (Horiguchi, 1987). Watermelon (Citrullus lanatus; Elamin and Wilcox, 1986b), but not muskmelon (Citrullus melo; Elamin and Wilcox, 1986a), grown at high Mn also develops small dark spots around the leaf trichomes. Other species that sequester Mn in the trichomes include common nettle (Urtica dioica; Hughes and Williams, 1988) and Alyssum murale, a Ni hyperaccumulator (Broadhurst et al., 2009; McNear and Küpper, 2014). Thus, some plants in four families, Asteraceae, Cucurbitaceae, Urticaceae, and Brassicaceae, tolerate high Mn in shoots through Mn sequestration in or around the trichomes. The mechanisms may differ, however, because the high Mn present during development of common nettle stinging hairs decreases as plants mature (Hughes and Williams, 1988).Recently developed techniques, including those based on synchrotron radiation, allow investigations of the distribution and speciation of Mn in planta, with most research to date focused on Mn hyperaccumulators (Fernando et al., 2013). For example, Fernando et al. (2010) used x-ray absorption near-edge spectroscopy (XANES) to confirm the widely accepted view that Mn(II) predominates in seven Mn hyperaccumulators. Synchrotron-based x-ray fluorescence microspectroscopy (µ-XRF) was used by McNear and Küpper (2014) to show that the basal region of trichomes of A. murale plants grown at no more than 10 µm Mn contained Mn(II) complexed with phosphate. At 50 µm Mn in solution, however, the increased amount of Mn that had accumulated around the trichomes was present as Mn(III). Few studies, however, have used synchrotron-based techniques to investigate the mechanisms of Mn toxicity and tolerance in agronomic species despite their importance for food production in regions where soils are acidic or intermittently waterlogged. One study on cowpea, with a critical toxicity concentration of only 2 µm Mn (Edwards and Asher, 1982), has shown an accumulation of Mn-citrate in the root cap and associated mucigel within 5 min of exposure to 150 µm Mn (Kopittke et al., 2013).This study aimed to determine the distribution and speciation of Mn in fresh roots, stems, and leaves of four crop species, soybean, white lupin (Lupinus albus), narrow-leafed lupin (Lupinus angustifolius), and sunflower, which differ in tolerance to high Mn. It was hypothesized that Mn distribution and speciation would differ between Mn-sensitive soybean and the three other species. Furthermore, we considered it likely that the Mn tolerance mechanism of sunflower would differ from those of the two lupin species, which do not have darkened trichomes when grown at high Mn.     

Increased incidence of choroid plexus carcinoma due to the germline TP53 R337H mutation in southern Brazil

Background

Choroid plexus carcinomas (CPC) are rare tumors predominantly found in children. Given the high frequency of the germline R337H mutation in the TP53 gene in southern Brazil, we have evaluated the frequency of the R337H mutation in families with CPC in children.

Methodology/Principal Findings

The present series included 29 patients that were admitted to the same institution from 1992 to 2010, including 22 children with CPC (0.08–13.6 years of age at diagnosis) and 7 children with papilloma of the choroid plexus (Pp; 0.5–9.8 years of age). Surgical resection was possible in 28 children. Blood and/or tumor DNA was extracted and analyzed using PCR-RFLP and results were confirmed by sequencing 240 bp of the TP53 exon 10. The patients, all parents, and some relatives submitted samples for blood DNA analysis. In addition, we have also examined the presence of the mutation in DNA from paraffin-embedded tumor samples to evaluate loss of heterozygosity. We found 63.3% (14/22) of the CPC patients positive for the germline R337H mutation; CPC samples were either heterozygous (n = 7), lost only the wild-type (n = 4), or only the R337H copy (n = 2). One CPC sample was not available. All Pp cases (7/7, 100%) were negative for R337H. Cure (>5 years survival free of disease) was observed in 18.1% of the CPC cases with the R337H mutation (2/11), 71.4% of the Pp (5/7), and 25% of CPC cases negative for the R337H mutation (2/8). Family history of cancer (with 2 or more cancer cases) was exclusively identified on the parental side segregating the R337H mutation, and 50% (7/14) of them were compatible with Li-Fraumeni-like syndrome.

Significance

Our results show for the first time that the R337H TP53 mutation is responsible for 63% of the CPC cases in children, suggesting a higher incidence of CPC in southern Brazil.     

Antiproliferative activity of N(6)-isopentenyladenosine on HCT-15 colon carcinoma cell line

N(6)-Isopentenyladenosine (iPA), a member of the cytokinin family of plant hormones, exerts remarkable inhibition on tumor cell proliferation and apoptosis in several tumor cell lines. In this study, we report that iPA is able to inhibit the proliferation and promotes apoptosis in HCT-15 human colon cancer cells in a dose-dependent manner with a concentration of 2.5?μM, which causes 50% inhibition of cell viability. The cell cycle analysis by flow cytometry showed that iPA-induced growth arrest could be associated to apoptosis. Moreover, suppression of clonogenic activity occurs after exposure to iPA at a concentration of 2.5?μM for HCT-15.     

Type-1 cannabinoid receptors reduce membrane fluidity of capacitated boar sperm by impairing their activation by bicarbonate

Background

Mammalian spermatozoa acquire their full fertilizing ability (so called capacitation) within the female genital tract, where they are progressively exposed to inverse gradients of inhibiting and stimulating molecules.

Methodology/Principal Findings

In the present research, the effect on this process of anandamide, an endocannabinoid that can either activate or inhibit cannabinoid receptors depending on its concentration, and bicarbonate, an oviductal activatory molecule, was assessed, in order to study the role exerted by the type 1 cannabinoid receptor (CB1R) in the process of lipid membrane remodeling crucial to complete capacitation. To this aim, boar sperm were incubated in vitro under capacitating conditions (stimulated by bicarbonate) in the presence or in the absence of methanandamide (Met-AEA), a non-hydrolysable analogue of anandamide. The CB1R involvement was studied by using the specific inhibitor (SR141716) or mimicking its activation by adding a permeable cAMP analogue (8Br-cAMP). By an immunocytochemistry approach it was shown that the Met-AEA inhibits the bicarbonate-dependent translocation of CB1R from the post-equatorial to equatorial region of sperm head. In addition it was found that Met-AEA is able to prevent the bicarbonate-induced increase in membrane disorder and the cholesterol extraction, both preliminary to capacitation, acting through a CB1R-cAMP mediated pathway, as indicated by MC540 and filipin staining, EPR spectroscopy and biochemical analysis on whole membranes (CB1R activity) and on membrane enriched fraction (C/P content and anisotropy).

Conclusions/Significance

Altogether, these data demonstrate that the endocannabinoid system strongly inhibits the process of sperm capacitation, acting as membrane stabilizing agent, thus increasing the basic knowledge on capacitation-related signaling and potentially opening new perspectives in diagnostics and therapeutics of male infertility.     

Constitutive overexpression of the OsNAS gene family reveals single-gene strategies for effective iron- and zinc-biofortification of rice endosperm

Background

Rice is the primary source of food for billions of people in developing countries, yet the commonly consumed polished grain contains insufficient levels of the key micronutrients iron (Fe), zinc (Zn) and Vitamin A to meet daily dietary requirements. Experts estimate that a rice-based diet should contain 14.5 µg g⁻¹ Fe in endosperm, the main constituent of polished grain, but breeding programs have failed to achieve even half of that value. Transgenic efforts to increase the Fe concentration of rice endosperm include expression of ferritin genes, nicotianamine synthase genes (NAS) or ferritin in conjunction with NAS genes, with results ranging from two-fold increases via single-gene approaches to six-fold increases via multi-gene approaches, yet no approach has reported 14.5 µg g⁻¹ Fe in endosperm.

Methodology/Principal Findings

Three populations of rice were generated to constitutively overexpress OsNAS1, OsNAS2 or OsNAS3, respectively. Nicotianamine, Fe and Zn concentrations were significantly increased in unpolished grain of all three of the overexpression populations, relative to controls, with the highest concentrations in the OsNAS2 and OsNAS3 overexpression populations. Selected lines from each population had at least 10 µg g⁻¹ Fe in polished grain and two OsNAS2 overexpression lines had 14 and 19 µg g⁻¹ Fe in polished grain, representing up to four-fold increases in Fe concentration. Two-fold increases of Zn concentration were also observed in the OsNAS2 population. Synchrotron X-ray fluorescence spectroscopy demonstrated that OsNAS2 overexpression leads to significant enrichment of Fe and Zn in phosphorus-free regions of rice endosperm.

Conclusions

The OsNAS genes, particularly OsNAS2, show enormous potential for Fe and Zn biofortification of rice endosperm. The results demonstrate that rice cultivars overexpressing single rice OsNAS genes could provide a sustainable and genetically simple solution to Fe and Zn deficiency disorders affecting billions of people throughout the world.     

Palmitoylation-dependent estrogen receptor alpha membrane localization: regulation by 17beta-estradiol

A fraction of the nuclear estrogen receptor alpha (ERalpha) is localized to the plasma membrane region of 17beta-estradiol (E2) target cells. We previously reported that ERalpha is a palmitoylated protein. To gain insight into the molecular mechanism of ERalpha residence at the plasma membrane, we tested both the role of palmitoylation and the impact of E2 stimulation on ERalpha membrane localization. The cancer cell lines expressing transfected or endogenous human ERalpha (HeLa and HepG2, respectively) or the ERalpha nonpalmitoylable Cys447Ala mutant transfected in HeLa cells were used as experimental models. We found that palmitoylation of ERalpha enacts ERalpha association with the plasma membrane, interaction with the membrane protein caveolin-1, and nongenomic activities, including activation of signaling pathways and cell proliferation (i.e., ERK and AKT activation, cyclin D1 promoter activity, DNA synthesis). Moreover, E2 reduces both ERalpha palmitoylation and its interaction with caveolin-1, in a time- and dose-dependent manner. These data point to the physiological role of ERalpha palmitoylation in the receptor localization to the cell membrane and in the regulation of the E2-induced cell proliferation.