EC:6.2.1.1 - FACTA Search

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Query: EC:6.2.1.1 (ACS)
78,556 document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)

The nickel(II) complex of an N2S2 ligand, derived from a diazacycle, N,N'-bis(mercaptoethyl)-1,5-diazacycloheptane, (bme-dach)Ni, Ni-1', serves as a metallodithiolate ligand to NiII, CuI, ZnII, Ag, and PbII. The binding ability of the NiN2S2 ligand to the metal ions was established through spectrochemical titrations in aqueous media and compared to classical S-donor ligands. For M = Ni, Zn, Pb, binding constants, log K = ca. 2. were computed for 1:1 Ni-1'/M(solvate) adducts; for Ag+ and Cu+, the 3:2 (Ni-1')3M2 adducts were the first formed products even in water with log beta3,2 values of 26 and >30, respectively. In all cases, the binding ability of Ni-S-R is intermediate between that of a free thiolate and a free thioether. The great specificity for copper over nickel and zinc by N2S2Ni, which serves as a reasonable structural model for the distal nickel of the acetyl CoA synthase active site, relates to biochemical studies of heterogeneity (metal content and type) in various preparations of acetyl CoA synthase enzyme.
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PMID:N2S2Ni metallodithiolate complexes as ligands: structural and aqueous solution quantitative studies of the ability of metal ions to form M-S-Ni bridges to mercapto groups coordinated to nickel(II). implications for acetyl coenzyme A synthase. 1585 64

The proteins of HL type cytoplasmic male sterility rice anther of YTA (CMS) and YTB (maintenance line) were separated by two-dimensional electrophoresis with immobilized ph (3-10 non-linear) gradients as the first dimension and SDS-PAGE as the second. The silver-stained proteins spots were analyzed using Image Master 2D software, there were about 1800 detectable spots on each 2D-gel, and about 85 spots were differential expressed. With direct MALDI-TOF mass spectrometry analysis and protein database searching, 9 protein spots out of 16 were identified. Among those proteins, there were Putative nucleic acid binding protein, glucose-1-phosphate adenylyltransferase (ADP-glucose pyrophosphorylase, AGPase) (EC: 2.7.7.27) large chain, UDP-glucuronic acid decarboxylase, putative calcium-binding protein annexin, putative acetyl-CoA synthetase and putative lipoamide dehydrogenase etc. They were closely associated with metabolism, protein biosynthesis, transcription, signal transduction and so on, all of which are cell activities that are essential to pollen development. Some of the identified proteins, i.e. AGPase, putative lipoamide dehydrogenase and putative acetyl-CoA synthetase were deeply discussed on the relationship to CMS. AGPase catalyzes a very important step in the biosynthesis of alpha 1,4-glucans (glycogen or starch) in bacteria and plants: synthesis of the activated glucosyl donor, ADP-glucose, from glucose-1-phosphate and ATP. The lack of the AGPase in male sterile line might directly result in the reduction of starch, and the synthesis of starch was the most important processes during the development of pollen. In present research, the descent or reduction of putative lipoamide dehydrogenase and putative acetyl-CoA synthetase seemed involved in pollen sterility in rice. The degeneration and formation of various tissues during pollen development may impose high demands for energy and key biosynthetic intermediates. Under such conditions, the TCA cycle needs to operate fully, because the TCA cycle is an important source for many intermediates required for biosynthetic pathways, in addition to performing an oxidative, energy-producing role. Thus, it seemed reasonable to infer that the decrease of putative lipoamide dehydrogenase and putative acetyl-CoA synthetase in anther might prevent the conversion of pyruvate into acetyl-CoA, and as a result, the TCA cycle could no longer operate at a sufficient rate to meet all requirements in anther cells, leading to pollen sterility. This study gave new insights into the mechanism of CMS in rice and demonstrated the power of the proteomic approach in plant biology studies.
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PMID:[Preliminary proteomics analysis of the total proteins of HL Type cytoplasmic male sterility rice anther]. 1655 98

Ethylene biosynthesis is directed by a family of 1-aminocyclopropane-1-carboxylic acid (ACC) synthases (ACS) that convert S-adenosyl-l-methionine to the immediate precursor ACC. Members of the type-2 ACS subfamily are strongly regulated by proteolysis with various signals stabilizing the proteins to increase ethylene production. In Arabidopsis, this turnover is mediated by the ubiquitin/26 S proteasome system, using a broad complex/tramtrack/bric-a-brac (BTB) E3 assembled with the ETHYLENE OVERPRODUCER 1 (ETO1) BTB protein for target recognition. Here, we show that two Arabidopsis BTB proteins closely related to ETO1, designated ETO1-like (EOL1) and EOL2, also negatively regulate ethylene synthesis via their ability to target ACSs for breakdown. Like ETO1, EOL1 interacts with type-2 ACSs (ACS4, ACS5 and ACS9), but not with type-1 or type-3 ACSs, or with type-2 ACS mutants that stabilize the corresponding proteins in planta. Whereas single and double mutants affecting EOL1 and EOL2 do not show an ethylene-related phenotype, they exaggerate the effects caused by inactivation of ETO1, and further increase ethylene production and the accumulation of ACS5 in eto1 plants. The triple eto1 eol1 eol2 mutant phenotype can be effectively rescued by the ACS inhibitor aminoethoxyvinylglycine, and by silver, which antagonizes ethylene perception. Together with hypocotyl growth assays showing that the sensitivity and response kinetics to ethylene are normal, it appears that ethylene synthesis, but not signaling, is compromised in the triple mutant. Collectively, the data indicate that the Arabidopsis BTB E3s assembled with ETO1, EOL1 and EOL2 work together to negatively regulate ethylene synthesis by directing the degradation of type-2 ACS proteins.
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PMID:The BTB ubiquitin ligases ETO1, EOL1 and EOL2 act collectively to regulate ethylene biosynthesis in Arabidopsis by controlling type-2 ACC synthase levels. 1880 54

Donnan dialysis is an ion exchange membrane process that can be used for the purification and concentration of diluted solutions. In this work, the behaviour of gold, silver and copper in cyanide medium is examined. Flux of cyanide complexes and corresponding free cyanide are determined using five commercial anion exchanger membranes (AMV, ACS, RAI 5035, ADP and ADS). The results show that the rate transfer depends upon the nature of the anion exchanger membrane. It is observed that the species number in the feed solution influences the transfer selectivity of metal ion complex against free cyanide Thus, gold which forms only one stable species with cyanides is transferred faster through an ACS membrane than copper which forms three species. However, this result is not verified when an ADS membrane is used. A model of the complex transfer through anion exchange membranes based on Donnan dialysis is proposed. A three compartment Donnan dialysis is performed to improve the separation between the studied metals. Decyanidation is also examined and separation factors are calculated. It is shown that Donnan dialysis can be an efficient technique for the separation of cyanides complexes of copper, gold and silver when parameters such as anion exchange membrane and the number of compartments are optimised. An advantage of this technique is also the possibility of recycling all reactants with a good impact on the environment.
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PMID:Donnan dialysis of copper, gold and silver cyanides with various anion exchange membranes. 1896 59

Real-time study of the transport and biocompatibility of nanomaterials in early embryonic development at single-nanoparticle resolution can offer new knowledge about the delivery and effects of nanomaterials in vivo and provide new insights into molecular transport mechanisms in developing embryos. In this study, we directly characterized the transport of single silver nanoparticles into an in vivo model system (zebrafish embryos) and investigated their effects on early embryonic development at single-nanoparticle resolution in real time. We designed highly purified and stable (not aggregated and no photodecomposition) nanoparticles and developed single-nanoparticle optics and in vivo assays to enable the study. We found that single Ag nanoparticles (5-46 nm) are transported into and out of embryos through chorion pore canals (CPCs) and exhibit Brownian diffusion (not active transport), with the diffusion coefficient inside the chorionic space (3 x 10(-9) cm(2)/s) approximately 26 times lower than that in egg water (7.7 x 10(-8) cm(2)/s). In contrast, nanoparticles were trapped inside CPCs and the inner mass of the embryos, showing restricted diffusion. Individual Ag nanoparticles were observed inside embryos at each developmental stage and in normally developed, deformed, and dead zebrafish, showing that the biocompatibility and toxicity of Ag nanoparticles and types of abnormalities observed in zebrafish are highly dependent on the dose of Ag nanoparticles, with a critical concentration of 0.19 nM. Rates of passive diffusion and accumulation of nanoparticles in embryos are likely responsible for the dose-dependent abnormalities. Unlike other chemicals, single nanoparticles can be directly imaged inside developing embryos at nanometer spatial resolution, offering new opportunities to unravel the related pathways that lead to the abnormalities.
ACS Nano 2007 Sep
PMID:In vivo imaging of transport and biocompatibility of single silver nanoparticles in early development of zebrafish embryos. 1912 72

The potential of using nanocrystals in applications within the fields of catalysis, electronics, medicine, and others has fueled research into the preparation and assembly of these materials. For most applications, it is necessary to have nanocrystal samples in which the size, shape, composition, and structure are tightly controlled within a narrow distribution. This need has motivated researchers to explore different synthesis protocols, including a method featured in this issue of ACS Nano by Kitaev and co-workers, where decahedral silver nanoparticles were used as seed particles for the growth of faceted silver rods. In this Perspective, we describe recent advances in seeded growth as the ultimate approach to producing metal nanocrystals with precisely controlled sizes, shapes, and compositionsthe necessary first step toward their use and assembly for large-scale applications.
ACS Nano 2009 Jan 27
PMID:Pushing nanocrystal synthesis toward nanomanufacturing. 1920 42

Monodisperse size-controlled faceted pentagonal silver nanorods were synthesized by thermal regrowth of decahedral silver nanoparticle (AgNPs) in aqueous solution at 95 degrees C, using citrate as a reducing agent. The width of the silver nanorods was determined by the size of the starting decahedral particle, while the length was varied from 50 nm to 2 mum by the amount of new silver added to the growth solution. Controlled regrowth allowed us to produce monodisperse AgNPs with a shape of elongated pentagonal dipyramid (regular Johnson solid, J(16)). Faceted pentagonal particles exhibited remarkable optical properties with sharp plasmon resonances precisely tunable across visible and NIR. Due to the narrow size distribution, faceted pentagonal silver nanorods readily self-assembled into the 3-D arrays similar to smectic mesophases. Hexagonal arrangement in the array completely overrode five-fold symmetry of the nanorods. Overall, our findings highlight the importance of pentagonal symmetry in metal nanoparticles and offer a facile method of the preparation of monodisperse AgNPs with controlled dimensions and plasmonic properties that are promising for optical applications and functional self-assembly.
ACS Nano 2009 Jan 27
PMID:Synthesis of size-controlled faceted pentagonal silver nanorods with tunable plasmonic properties and self-assembly of these nanorods. 1920 44

We report here the use of a simple washing approach to reduce the ionic strength of the solution, which increased the thickness of the electric double layer on the surface of silver (Ag) nanoparticles and thereby enhanced their surface zeta-potential. This approach allowed us to prepare optically uniform (75-99%) and purified Ag nanoparticles (11.3 +/- 2.3 nm) that are stable (nonaggregation) in solution for months, permitting them to become robust and widely used single nanoprobes for in vivo optical imaging. These Ag nanoparticles show remarkable photostability and serve as single nanoparticle photonic probes for continuous imaging nanoenvironments of segmentation-stage zebrafish embryos for hours. Unlike other particle tracking experiments, we utilized size-dependent localized surface plasmon resonance spectra (LSPRS) (colors) of single Ag nanoparticles to determine given colored (sized) nanoparticles in situ and used the monodisperse color (size) of nanoparticles to simultaneously measure viscosities and flow patterns of multiple proximal nanoenvironments in segmentation-stage zebrafish embryos in real time. We found new interesting counterclockwise flow patterns with rates ranging from 0.06 to 1.8 microm/s and stunningly high viscosity gradients spanning two orders of magnitude in chorion space of the embryos, with the highest viscosity observed around the center of chorion space and the lower viscosity at the interfacial areas near the surface of both chorion layers and inner mass of the embryos. This study demonstrates the possibility of using individual monodisperse nanophotonics to probe the roles of embryonic fluid dynamics in embryonic development.
ACS Nano 2008 Jul
PMID:Design of stable and uniform single nanoparticle photonics for in vivo dynamics imaging of nanoenvironments of zebrafish embryonic fluids. 1920 4

Herein we report the spontaneous reduction of silver ions into nanostructures by yeast surface-displayed glutamic acid (E(6)) and aspartic acid (D(6)) peptides. Light spectroscopy and electron microscopy reveal that silver ions are photoreduced in the presence of the polycarboxylic acid-containing peptides and ambient light, with an increase in reduction capability of E(6) expressing yeast over D(6) yeast. The importance of tethering peptides to a biological scaffold was inferred by observing the reduced particle forming capacity of soluble peptides with respect to corresponding yeast-displayed peptides. This principle was further extended to the M13 virus for fabrication of crystalline silver nanowires. These insights into the spontaneous reduction of metal ions on biological scaffolds should help further the formation of novel nanomaterials in biological systems.
ACS Nano 2008 Jul
PMID:Peptide-mediated reduction of silver ions on engineered biological scaffolds. 1920 18

Silver vanadium oxide (SVO) and V2O5 nanowires have been hydrothermally synthesized. The as-made nanowires are over 30 microm long and 10-20 nm in diameter. The nanowires have a layered structure with a d-spacing of 1.07 nm. The nanowires can be fabricated into free-standing and flexible sheets by suction filtration. The electrical conductivity of the SVO nanowires is 0.5 S/cm, compared to 0.08 S/cm for the V2O5 nanowires. The Li ion diffusion coefficient in the SVO nanowires was 7 times higher than that in the V2O5 nanowires. An electrochromic device was fabricated from the SVO nanowires that displayed a color-switching time of 0.2 s from the bleached state (green) to the colored state (red-brown) and 60% transmittance contrast.
ACS Nano 2008 Feb
PMID:Fabrication of silver vanadium oxide and V2O5 nanowires for electrochromics. 1920 30

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