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EDTA disodium

Lithium chloride [7447-41-8] M 42.4, m 600 , 723 . Crysld from water (ImL/g) or MeOH and dried for several hours at 130 . Other metal ions can be removed by preliminary crystallisation from hot aqueous 0.0 IM disodium EDTA. Has also been crystallised from cone HCl, fused in an atmosphere of dry HCl gas, cooled under dry N2 and pulverised in a dry-box. Kolthoff and Bruckenstein [J Am Chem Soc 74 2529 1952] ppted with ammonium carbonate, washed with Li2C03 five times by decantation and finally with suction, then dissolved in HCl. The LiCl solution was evaporated slowly with continuous stirring in a large evaporating dish, the dry powder being stored (while still hot) in a desiccator over CaCl2. [Pg.435]

Some strains of P. aeruginosa are resistant to benzalkonium chloride and, in fact, can be grown in solutions concentrated in this agent. This has caused great concern because of the virulent nature of this organism in ocular infections, as discussed previously. Thus, it was an important finding in 1958 that the acquired resistance could be eliminated by the presence of ethylenediaminetetracetic acid (sodium edetate) in the formulation. This action of EDTA has been correlated with its ability to chelate divalent cations, and it is commonly used as a preservative aid [125]. The use of disodium EDTA, where compatible, is recommended in concentrations up to 0.1%. [Pg.433]

Urinary lead levels have also been used to measure current exposure (Robinson 1974) but they are of questionable value as biomarkers of exposure because of the relatively low and fluctuating lead levels that are excreted in the urine (ACGIH 1986 Ibels and Pollock 1986 Jensen 1984). In contrast, the determination of urinary lead following a single injection of the chelating agent, calcium disodium EDTA, which mobilizes extracellular lead and produces increased urinary excretion of lead, is presumed to be indicative of an elevated body burden of lead (Cory-Slechta et al. 1987 Ibels and Pollock 1986 Janin et al. 1985). Children whose PbB levels are 45 pg/dL should not receive a provocative chelation... [Pg.313]

A common form of EDTA used as a preservative is calcium disodium EDTA (CaNa2EDTA). What metals will this form of the sequestrant scavenge effectively The dissolution of the solid will yield calcium ions, sodium ions, and the EDTA anion. Any metal more effectively complexed than calcium will be readily scavenged, including all ions listed in Table 9.1 except silver (Ag+) and magnesium (Mg2+). (In the absence of the calcium counterion, as in the case of the acid form of EDTA, chelation of calcium in the body can occur. In fact, EDTA administered orally is an FDA-approved treatment for calcium deposits in the bloodstream that lead to cardiovascular disease.) Citric acid (Fig. 9.3.3) is another sequestrant of metal ions in foodstuffs. [Pg.121]

In mammals, phenobarbital and phenytoin increase serum ceruloplasmin concentrations (Aaseth and Norseth 1986). Chronic copper poisoning in sheep is exacerbated when diets contain heliotrope plants (Heliotropium sp., Echium spp., Senecio sp.). Aggravated effects of the heliotrope plants include reduced survival and a twofold to threefold increase in liver and kidney copper concentrations when compared to control animals fed copper without heliotropes (Howell et al. 1991). Rats given acutely toxic doses of 2,3,7,8-tetrachlorodibenzo-para-dioxin had elevated concentrations of copper in liver and kidney because of impaired biliary excretion of copper (Elsenhans et al. 1991). Morphine increases copper concentrations in the central nervous system of rats, and dithiocarbam-ates inhibit biliary excretion (Aaseth and Norseth 1986). In human patients, urinary excretion of copper is increased after treatment with D-penicillamine, calcium disodium EDTA, or calcium trisodium diethylenetriamine penta acetic acid (Flora 1991). [Pg.139]

For the same purpose, Kelly and Bryske used paper impregnated with 0.1N disodium ethylenediaminetetraacetate (EDTA) and two mobile solvents the organic phase from a mixture of n-butanol, ammonia, water (4 1 5) and the organic phase from a mixture of n-butanol, acetic acid, water (4 1 5). Disodium EDTA (0.1N) works as well as Mcllvaine s buffer when it is used to treat the paper in the method of Walton et al. (49). A circular paper chromatographic method also using paper dampened with Mcllvaine s buffer (pH 4.5) was reported by Urx et al. (50). They used a mixture of chloroform and n-butanol (4 1) as the mobile solvent. [Pg.125]

Mix 0.01 M dimethyltryptamine, 0.02 M phosphate buffer pH 7.2 containing 5 mM ascorbic acid, 0.02 M disodium EDTA and 0.01 M ferrous sulfate (CuCI may substitute) and add with stirring at 20-22° 0.02 M H202 (0.01 M may increase yield). Let reaction proceed to completion (2 hours or less) and extract with ethyl acetate. Dry and evaporate in vacuum to get about 30% yield of psilocin. The product, which contains the other OH-DMT s as well, can be chromatographed on silica thin layer with t-butanol-acetic acid-water (ACS 22,1210 (1968)) or on a 5% alumina-Nickel... [Pg.73]

Prepare 100 mL (500 mL if the gel is to be run under the buffer) of an electrophoresis buffer that is 20 mM tris-(hydroxymethyl)amino methane (TRIS or THAM), 6 mM sodium acetate, and 1 mM disodium EDTA. Adjust the pH of this solution to 7.9 using concentrated HC1. Also prepare small volumes of solutions of hemoglobin and cytochrome C in the buffer (the concentration is not important) and also a mixture solution of these two solutes. Add a quantity of sucrose to each. [Pg.483]

Prepare a buffer solution that is 20 mM tris-(hydroxymethyl)amino methane (TRIS or THAM), 6 mM sodium acetate, and 1 mM disodium EDTA. Adjust to pH = 7.9. [Pg.485]

E 385 Calcium disodium ethylene diamine tetra-acetate (Calcium disodium EDTA)... [Pg.36]

In actual practice, whenever the disodium EDTA solution is added to a solution of a metal ion previously buffered to augment complexation, it has been observed that initially the rate of change of concentration of metal ion is rather slow, but interestingly it picks up quite rapidly as further addition of sodium-EDTA approaches one equivalent. [Pg.164]

In direct titration, usually an appropriate buffer solution and a suitable indicator are added to the M2+ (metal-ion) solution and subsequently the resulting solution is titrated with previously standardized disodium-EDTA until the indicator just changes colour. Sometimes, a simultaneous blank determination is also recommended to have a check for the presence of traces of metallic impurities in the reagents. [Pg.166]

Table 9.2 Substances Assayed by Direct Titration with Disodium-EDTA... Table 9.2 Substances Assayed by Direct Titration with Disodium-EDTA...
Alkali reagent (disodium EDTA, 0.1 M + sodium hydroxide, 2 M) - weigh 80 g NaOH and 37.2 g disodium EDTA into a beaker and dissolve in ammonia-free water. Transfer to a 1 -I volumetric flask, and when cool make up to the mark and mix. [Pg.154]

In soil analysis, the sample pretreatment varies depending on whether a total elemental analysis or an exchangeable cation analysis is required. In the former, a silicate analysis method (see below) is appropriate. In the latter, the soil is shaken with an extractant solution, e.g. 1 M ammonium acetate, ammonium chloride or disodium EDTA. After filtration, the extractant solution is analysed. Fertilizers and crops can be treated as chemical and food samples, respectively. [Pg.13]

Venous blood (8 mL) was collected into 15-mL tubes containing 50 mmol/L disodium EDTA, and genomic DNA was extracted by the standard (phenol/chloroform) method. The genotype frequencies for GSTPl were determined by polymerase chain reaction (PCR)/RFLP-based methods using DNA extracted from peripheral lymphocytes. [Pg.149]

Dimercaprol is FDA-approved as single-agent treatment of acute poisoning by arsenic and inorganic mercury and for the treatment of severe lead poisoning when used in conjunction with edetate calcium disodium (EDTA see below). Although studies of its metabolism in humans are limited, intramuscularly administered dimercaprol appears to be readily absorbed, metabolized, and excreted by the kidney within 4-8 hours. Animal models indicate that it may also undergo biliary excretion, but the role of this excretory route in humans and other details of its biotransformation are uncertain. [Pg.1240]


See other pages where EDTA disodium is mentioned: [Pg.452]    [Pg.453]    [Pg.245]    [Pg.439]    [Pg.95]    [Pg.133]    [Pg.546]    [Pg.1193]    [Pg.126]    [Pg.126]    [Pg.314]    [Pg.324]    [Pg.511]    [Pg.483]    [Pg.451]    [Pg.258]    [Pg.273]    [Pg.274]    [Pg.170]    [Pg.72]    [Pg.250]    [Pg.254]    [Pg.258]    [Pg.142]    [Pg.298]    [Pg.104]    [Pg.451]    [Pg.112]    [Pg.164]    [Pg.164]    [Pg.167]   
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Calcium Disodium EDTA

Disodium

Disodium ethylene diamine tetraacetic acid EDTA)

EDTA

EDTA (ethylenediaminetetraacetic Edetate calcium disodium

Nickel disodium EDTA

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