Peroxides, test for

Peroxides, test for, 41, 92 Peroxy acids from carboxylic acids and 70% hydrogen peroxide, 43, 96 Peroxybenzoic acid, 43,93 iodometric analysis of, 43, 94 Peroxystearic acid, 43,96 Phenacylamine hydrochloride, 41, 82... 

This test must not be confused with the familiar guaiacum-peroxide test for blood (p. 403), which will not work in an acid solution. Many... 

The colour sequence already described, for the reduction of van-adium(V) to vanadium(II) by zinc and acid, gives a very characteristic test for vanadium. Addition of a few drops of hydrogen peroxide to a vanadate V) gives a red colour (formation of a peroxo-complex) (cf. titanium, which gives an orange-yellow colour). 

Addition of hydrogen peroxide to a solution of a dichromate yields the blue colour of "peroxochromic acid. This is a test for soluble chromates and dichromates. 

The purple colour of this ion alone is a sufficient test for its presence addition of sulphuric acid and hydrogen peroxide discharges ihe colour. 

Di-n-butyl ether. Technical n-butyl ether does not usually contain appreciable quantities of peroxides, unless it has been stored for a prolonged period. It should, however, be tested for peroxides, and, if the test is positive, the ether should be shaken with an acidified solution of a ferrous salt or with a solution of sodium sulphite (see under Diethyl ether). The ether is dried with anhydrous calcium chloride, and distilled through a fractionating column the portion, b.p. 140-141°, is collected. If a fraction of low boiling point is obtained, the presence of n-butyl... 

It is recommended that the tsopropanol be tested for peroxides and, if present, removed by refluxing with solid stannous chloride (for details, see concluding paragraph of Section VI,12)... 

Recovery of the wopropyl alcohol. It is not usually economical to recover the isopropyl alcohol because of its lo v cost. However, if the alcohol is to be recovered, great care must be exercised particularly if it has been allowed to stand for several days peroxides are readily formed in the impure acetone - isopropyl alcohol mixtures. Test first for peroxides by adding 0-6 ml. of the isopropyl alcohol to 1 ml. of 10 per cent, potassium iodide solution acidified with 0-6 ml. of dilute (1 5) hydrochloric acid and mixed with a few drops of starch solution if a blue (or blue-black) coloration appears in one minute, the test is positive. One convenient method of removing the peroxides is to reflux each one litre of recovered isopropyl alcohol with 10-15 g. of solid stannous chloride for half an hour. Test for peroxides with a portion of the cooled solution if iodine is liberated, add further 5 g. portions of stannous chloride followed by refluxing for half-hour periods until the test is negative. Then add about 200 g. of quicklime, reflux for 4 hours, and distil (Fig. II, 47, 2) discard the first portion of the distillate until the test for acetone is negative (Crotyl Alcohol, Note 1). Peroxides generally redevelop in tliis purified isopropyl alcohol in several days. 

It is recommended that the eompound be fused with a mixture of sodium carbonate (2 parts) and sodium peroxide (1 part) as in the test for Plvoaphoms. Extract the fused mass with water, filter, and acidify with dilute hydrochloric acid. Pass hydrogen sulphide through the hot solution arsenic is precipitated as yellow arsenic sulphide. If antimony is present, it will be precipitated as orange antimony trisulphide. 

Detecting the presence of small, even invisible, amounts of blood is routine. Physical characteristics of dried stains give minimal information, however, as dried blood can take on many hues. Many of the chemical tests for the presence of blood rely on the catalytic peroxidase activity of heme (56,57). Minute quantities of blood catalyze oxidation reactions between colorless materials, eg, phenolphthalein, luco malachite green, luminol, etc, to colored or luminescent ones. The oxidant is typically hydrogen peroxide or sodium perborate (see Automated instrumentation,hematology). 

Low molecular weight ether hydroperoxides are similarly dangerous and therefore ethers should be tested for peroxides and any peroxidic products removed from them before ethers are distilled or evaporated to dryness. Many ethers autoxidize so readily that peroxidic compounds form at dangerous levels when stored in containers that are not airtight (133). Used ether containers should be handled cautiously and if they are found to contain hazardous soHd ether peroxides, bomb-squad assisted disposal may be required (134). ZeoHtes have been used for removal of peroxide impurities from ethers (135). 

Peroxide Formation. Except for the methyl alkyl ethers, most ethers tend to absorb and react with oxygen from the air to form unstable peroxides that may detonate with extreme violence when concentrated by evaporation or distillation, when combined with other compounds that give a detonable mixture, or when disturbed by heat, shock, or friction. Appreciable quantities of crystalline soHds have been observed as gross evidence for the formation of peroxides, and peroxides may form a viscous Hquid in the bottom of ether-fiHed containers. If viscous Hquids or crystalline soHds are observed in ethers, no further tests for the detection of peroxides are recommended. Several chemical and physical methods for detecting and estimating peroxide concentrations have been described. Most of the quaHtative tests for peroxides are readily performed and strongly recommended when any doubt is present (20). 

PSS-SG composite film was tested for sorption of heme proteins hemoglobin (Hb) and myoglobin (Mb). The peroxidaze activity of adsorbed proteins were studied and evaluated by optical and voltammetric methods. Mb-PSS-SG film on PG electrode was shown to be perspective for detection of dissolved oxygen and hydrogen peroxide by voltammetry with linear calibration in the range 2-30 p.M, and detection limit -1.5 p.M. Obtained composite films can be modified by different types of biological active compounds which is important for the development of sensitive elements of biosensors. 

Chemical tests for particular types of impurities, e.g. for peroxides in aliphatic ethers (with acidified KI), or for water in solvents (quantitatively by the Karl Fischer method, see Fieser and Fieser, Reagents for Organic Synthesis J. Wiley Sons, NY, Vol 1 pp. 353, 528, 1967, Library of Congress Catalog Card No 66-27894). 

Peroxides. These are formed by aerial oxidation or by autoxidation of a wide range of organic compounds, including diethyl ether, allyl ethyl ether, allyl phenyl ether, dibenzyl ether, benzyl butyl ether, n-butyl ether, iso-butyl ether, r-butyl ether, dioxane, tetrahydrofuran, olefins, and aromatic and saturated aliphatic hydrocarbons. They accumulate during distillation and can detonate violently on evaporation or distillation when their concentration becomes high. If peroxides are likely to be present materials should be tested for peroxides before distillation (for tests see entry under "Ethers", in Chapter 2). Also, distillation should be discontinued when at least one quarter of the residue is left in the distilling flask. 

A simple test for ether peroxides is to add lOmL of the ether to a stoppered cylinder containing ImL of freshly prepared 10% solution of potassium iodide containing a drop of starch indicator. No colour should develop during one minute if free from peroxides. Alternatively, a 1% solution of ferrous ammonium sulfate, O.IM in sulfuric acid and O.OIM in potassium thiocyanate should not increase appreciably in red colour when shaken with two volumes of the ether. 

Quantitative tests for catalase activity find their greatest usefulness in examination of finished product. For this purpose gasometric methods (36) or chemical methods based upon measurement of residual hydrogen peroxide (2) may be used. In the use of these quantitative methods it might be well to observe the precaution of removing the skins. 

A common method for determining the stability of pastry, potato chips, and the like is to place a number of broken pieces of the product in 4-ounce mayonnaise jars with screw tops and store them at room temperature or in the Schaal oven in the absence of light. At regular intervals samples are removed and tested for peroxide content and organoleptic rancidity. 

Pollard s Test for Stability of Propellants. This test, proposed in 1924—25, is based upon the action of nitric peroxide on colloidal Ag oxide Procedure. A current of air is passed over a sample of proplnt in storage into a colloidal soln of Ag oxide. If free nitrogen peroxide is present, it reacts with the colloid and decreases the amt of light diffused by it. The larger the decrease, the higher the amt of N02 present, and the more decompd is the proplnt Ref Reilly (1938), 80... 

The checkers used 3-methyl-2-butanone purchased from Eastman Organic Chemicals. One sample that gave a positive test for peroxides was purified by passage through a column of alumina before distillation. The material was distilled routinely before use. 

Analyses for the Saxitoxins. Early methods for analysis of the saxitoxins evolved from those used for toxin isolation and purification. The principal landmarks in the development of preparative separation techniques for the saxitoxins were 1) the employment of carboxylate cation exchange resins by Schantz et al. (82) 2) the use of the polyacrylamide gel Bio-Gel P2 by Buckley and by Shimizu (5,78) and 3) the development by Buckley of an effective TLC system, including a new solvent mixture and a new visualization technique (83). The solvent mixture, designated by Buckley as "E", remains the best for general resolution of the saxitoxins. The visualization method, oxidation of the saxitoxins on silica gel TLC plates to fluorescent degradation products with hydrogen peroxide and heat, is an adaptation of the Bates and Rapoport fluorescence assay for saxitoxin in solution. Curiously, while peroxide oxidation in solution provides little or no response for the N-l-hydroxy saxitoxins, peroxide spray on TLC plates is a sensitive test for all saxitoxin derivatives with the C-12 gemdiol intact. 

Antioxidant capacities of common individual curcuminoids were determined in vitro by phosphomolybdenum and linoleic acid peroxidation methods. Antioxidant capacities expressed as ascorbic acid equivalents (pmol/g) were 3099 for curcumin, 2833 for demethoxycurcumin, and 2677 for bisdemethoxycurcumin at concentrations of 50 ppm. The same order of antioxidant activity (curcumin > demethoxycurcumin > bisdemethoxycurcumin) was observed when compared with BHT (buty-lated hydroxyl toluene) in linoleic peroxidation tests. The antioxidant activity of curcumin in the presence of ethyl linoleate was demonstrated and six reaction products were identified and structurally characterized. The mechanism proposed for this activity consisted of an oxidative coupling reaction at the 3 position of the curcumin with the lipid and a subsequent intramolecular Diels-Alder reaction. ... 

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