Sequence analysis revealed phospholipase A2 (PLA2) motifs in capsid proteins of parvoviruses. Although PLA2 activity is not known to exist in viruses, putative PLA2s from divergent parvoviruses, human B19, porcine parvovirus, and insect GmDNV (densovirus from Galleria mellonella), can emulate catalytic properties of secreted PLA2. Mutations of critical amino acids strongly reduce both PLA2 activity and, proportionally, viral infectivity, but cell surface attachment, entry, and endocytosis by PLA2-deficient virions are not affected. PLA2 activity is critical for efficient transfer of the viral genome from late endosomes/lysosomes to the nucleus to initiate replication. These findings offer the prospect of developing PLA2 inhibitors as a new class of antiviral drugs against parvovirus infections and associated diseases.
Nitric oxide (NO) is a signaling and defense molecule of major importance in living organisms. In the model legume Medicago truncatula, NO production has been detected in the nitrogen fixation zone of the nodule, but the systems responsible for its synthesis are yet unknown and its role in symbiosis is far from being elucidated. In this work, using pharmacological and genetic approaches, we explored the enzymatic source of NO production in M. truncatula-Sinorhizobium meliloti nodules under normoxic and hypoxic conditions. When transferred from normoxia to hypoxia, nodule NO production was rapidly increased, indicating that NO production capacity is present in functioning nodules and may be promptly up-regulated in response to decreased oxygen availability. Contrary to roots and leaves, nodule NO production was stimulated by nitrate and nitrite and inhibited by tungstate, a nitrate reductase inhibitor. Nodules obtained with either plant nitrate reductase RNA interference double knockdown (MtNR1/2) or bacterial nitrate reductase-deficient (napA) and nitrite reductase-deficient (nirK) mutants, or both, exhibited reduced nitrate or nitrite reductase activities and NO production levels. Moreover, NO production in nodules was found to be inhibited by electron transfer chain inhibitors, and nodule energy state (ATP-ADP ratio) was significantly reduced when nodules were incubated in the presence of tungstate. Our data indicate that both plant and bacterial nitrate reductase and electron transfer chains are involved in NO synthesis. We propose the existence of a nitrate-NO respiration process in nodules that could play a role in the maintenance of the energy status required for nitrogen fixation under oxygen-limiting conditions.
Following fruit set, the early development of tomato (Lycopersicon esculentum Mill.) fruit comprises two distinct phases: a cell division phase and a consecutive phase of cell expansion until the onset of ripening. In this study, we analyzed cytological and molecular changes characterizing these early phases of tomato fruit development. First we investigated the spatial and temporal regulation of the mitotic activity during fruit development. The DNA content of isolated nuclei from the different fruit tissues was determined by flow cytometry analysis. The results confirm the data of mitotic activity measurements and show that cell differentiation, leading to expanded cells, is characterized by endoreduplication. Second, we isolated two cDNAs, named Lyces;CDKA1 (accession no. Y17225) and Lyces;CDKA2 (accession no. Y17226), encoding tomato homologs of the cyclin-dependent kinase (CDK) p34 cdc2 . Tomato CDKA gene expression was followed at both the transcriptional and translational levels during fruit development. The transcripts for Lyces;CDKA1 and Lyces;CDKA2 and the corresponding CDKA proteins are predominantly accumulated during the phase of cell division between anthesis and 5 d post anthesis (DPA). In whole fruits, the maximum CDK activity was obtained between 5 and 10 DPA. The determination of the kinase activity using protein extracts from the different fruit tissues was in agreement with mitotic activity analysis. It showed the particular disappearance of the activity in the gel tissue as early as 15 DPA. The overall data of CDK activity measurements suggest a strong post-translational regulation of CDK at the temporal and spatial levels during early tomato fruit development.
Excised maize (Zea mays) root tips were used to follow the effects of a prolonged glucose starvation. Respiration rate began to decrease immediately after excision, reaching 30 to 40% of its initial value after 20 hours, and then declined more slowly until death of the tissues, which occurred after 200 hours of starvation. During the whole process, respiration could be uncoupled by 2,4-dinitrophenol and the energy charge remained high. These results suggest that in excised maize root tips, respiration rate is essentially limited by the rate of biosyntheses (ATP-utilizing processes) rather than mitochondrial number. Carbohydrates are the main respiratory substrates for plants, furnishing the malate and the acetyl-CoA necessary for the functioning of the Krebs cycle. Fifteen years ago it was still considered that, during the day, photosynthesis allowed starch synthesis in such amounts that the plant, particularly the root system, was never deprived of sugars. However, it is now known that carbohydrate starvation is common in most higher plants. Indeed, microbial, insect, or herbivore attacks or reduction in light intensity or temperature may cause a substantial decrease in photosynthesis, and thus lead to starvation.Since the end of the seventies, carbohydrate starvation has been studied in a number of plant species: wheat (28, 29), maize (14, 18), barley (8), pearl millet (1), pea (20,26,27), soybean (13, 25), sycamore (7, 10, 12, 17), etc. These studies have shown that in most cases, sugar starvation triggers the following sequence in plant cells: (a) the depletion of intracellular carbohydrate content and the subsequent decrease of respiration (1,12,18,20,25); (b) the breakdown of lipids and proteins (1,7,12,28) and a decline in the respiratory quotient from 1 to 0.75 (18); (c) an increase in inorganic phosphate ( 12,17), phosphorylcholine (7, 17), and free amino acids (10), and a concomitant decline in nucleotides (17, 18) and glycolytic enzymatic activities (12); and (d) the more or less marked disappearance of some cell ultrastructures (1, 29).The origin of the respiratory decrease during starvation was first attributed to carbohydrate depletion, by way of limitation of the substrate either for respiration or for biosynthetic processes; however, some experiments showed that root respiration rate was not a simple function ofcarbohydrate supply (8). Journet and co-workers (12) reported that during starvation the decrease in uncoupled respiration of sycamore cells was attributable to a progressive decrease in the number of mitochondria per cell; these authors concluded that the availability of respiratory substrates for the mitochondria does not determine the respiration rate of starved cells.In the present work, we investigated changes in 02 consumption, different organic compounds (sugars, fatty acids, proteins, adenine nucleotides), enzyme activities, and physical parameters (fresh and dry weight, osmolarity) in excised maize (Zea mays) root tips from the beginning of glucose starvation to tissue dea...
Metabolic pathways of the intermediate metabolism of maize root tips were identified and quantified after labeling to isotopic and metabolic steady state using glucose labeled on carbon-1, -2, or -6 with 14C or 13C. The specific radioactivity of amino acids and the 13C-specific enrichment of specific carbons of free glucose, sucrose, alanine and glutamate were measured and used to calculate metabolic fluxes. The non-triose pathways, including synthesis of polysaccharides, accumulation of free hexoses, and to a lesser extent starch synthesis, were found to consume 75% of the glucose entering the root tips. The cycle of synthesis and hydrolysis of sucrose was found to consume about 70% of the ATP produced by respiration. The comparison of the specific radioactivities of amino acids and phospholipid glycerol phosphate after labeling with [1-(14)C] or [6-(14)C]glucose revealed the operation of the pentose phosphate pathway. The transfer of label from [2-(14)C]glucose to carbon-1 of starch glucosyl units confirmed the operation of this pathway and indicated that it is located in plastids. It was found to consume 32% of the hexose phosphates entering the triose pathways. The remaining 68% were consumed by glycolysis. The determination of the specific enrichment of carbohydrate carbons -1 and -6 after labeling with [1-(13)C]glucose indicated that both the conversion of triose phosphates back to hexose phosphates and the transaldolase exchange contributed to this randomization. Of the triose phosphates produced by glycolysis and the pentose phosphate pathway, about 60% were found to be recycled to hexose phosphates, and 28% were directed to the tricarboxylic acid cycle. Of this 28%, two-thirds were found to be directed through the pyruvate kinase branch and one-third through the phosphoenolpyruvate branch. The latter essentially has an anaplerotic function since little malate was found to be converted to pyruvate (malic enzyme reaction).
Three-week-old maize (Zea mays L.) plants were submitted to light/dark cycles and to prolonged darkness to investigate the occurrence of sugar-limitation effects in different parts of the whole plant. Soluble sugars fluctuated with light/dark cycles and dropped sharply during extended darkness. Significant decreases in protein level were observed after prolonged darkness in mature roots, root tips, and young leaves. Glutamine and asparagine (Asn) changed in opposite ways, with Asn increasing in the dark. After prolonged darkness the increase in Asn accounted for most of the nitrogen released by protein breakdown. Using polyclonal antibodies against a vacuolar root protease previously described (F. James, R. Brouquisse, C. Suire, A. Pradet, P. Raymond [1996] Biochem J 320: 283-292) or the 20S proteasome, we showed that the increase in proteolytic activities was related to an enrichment of roots in the vacuolar protease, with no change in the amount of 20S proteasome in either roots or leaves. Our results show that no significant net proteolysis is induced in any part of the plant during normal light/ dark cycles, although changes in metabolism and growth appear soon after the beginning of the dark period, and starvation-related proteolysis probably appears in prolonged darkness earlier in sink than in mature tissues.Carbohydrate deprivation is a fact of life for most higher plants. When the emergence of young seedlings and their transition to autotrophy is delayed (Elamrani et al., 1994b), when competition occurs between sink tissues such as roots, flowers, or fruits (Dejong and Grossman, 1995;Ho, 1996), or when under environmental constraints, the photosynthesis rate or the translocation of nutrients to sink tissues decreases (Amthor and McCree, 1990;Setter, 1990) and higher plants may experience carbon starvation. Similarly, in some types of senescence (Noodén, 1988) or in postharvest situations (King et al., 1990), the degradation of some tissue or cell structures is clearly related to the appearance of carbon-starvation symptoms, such as a decrease in sugar content, net lipid and protein breakdown, degradation of plastids, or loss of membrane selective permeability. The metabolic consequences of carbohydrate starvation have been studied in a number of plant models, and the situation may be summarized as follows: to survive, plant cells have to adapt to the lack of carbohydrates by substituting protein and lipid metabolism for sugar metabolism through autophagic processes (James, 1953;Thomas, 1978;Saglio and Pradet, 1980;Journet et al., 1986;Roby et al., 1987; Baysdorfer et al., 1988;Peoples and Dalling, 1988;King et al., 1990; Brouquisse et al., 1991;Tassi et al., 1992;Elamrani et al., 1994b).There are many reports of degradation and synthesis of proteins during carbon deprivation. Thus, enzymic activities related to sugar metabolism and respiration (Journet et al., 1986; Brouquisse et al., 1991;Irving and Hurst, 1993), nitrogen reduction and assimilation (Thomas, 1978;Peeters and Van Laere, 1992; Brouquisse ...
Asparagine metabolism and nitrogen distribution during protein degradation in sugar-starved maize root tips
Excised maize (Zea mays L.) root tips were used to monitor the effects of prolonged glucose starvation on nitrogen metabolism. Following root-tip excision, sugar content was rapidly exhausted, and protein content declined to 40 and 8% of its initial value after 96 and 192 h, respectively. During starvation the contents of free amino acids changed. Amino acids that belonged to the same "synthetic family" showed a similar pattern of changes, indicating that their content, during starvation, is controlled mainly at the level of their common biosynthetic steps. Asparagine, which is a good marker of protein and amino-acid degradation under stress conditions, accumulated considerably until 45 h of starvation and accounted for 50% of the nitrogen released by protein degradation at that time. After 45 h of starvation, nitrogen ceased to be stored in asparagine and was excreted from the cell, first as ammonia until 90-100 h and then, when starvation had become irreversible, as amino acids and aminated compounds. The study of asparagine metabolism and nitrogen-assimilation pathways throughout starvation showed that: (i) asparagine synthesis occurred via asparagine synthetase (EC 6.3.1.1) rather than asparagine aminotransferase (EC 2.6.1.14) or the β-cyanoalanine pathway, and asparagine degradation occurred via asparaginase (EC 3.5.1.1); and (ii) the enzymic activities related to nitrogen reduction and assimilation and amino-acid synthesis decreased continuously, whereas glutamate dehydrogenase (EC 1.4.1.2-4) activities increased during the reversible period of starvation. Considered together, metabolite analysis and enzymic-activity measurements showed that starvation may be divided into three phases: (i) the acclimation phase (0 to 30-35 h) in which the root tips adapt to transient sugar deprivation and partly store the nitrogen released by protein degradation, (ii) the survival phase (30-35 to 90-100 h) in which the root tips expel the nitrogen released by protein degradation and starvation may be reversed by sugar addition and (iii) the cell-disorganization phase (beyond 100 h) in which all metabolites and enzymic activities decrease and the root tips die.
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