Nitroaniline,production

Compound 27 or one of the above-mentioned derivatives can also be reacted with a 2-hydroxyethylsulfonylaniline instead of with a diamine. After reduction of the 4-nitroaniline product 34 followed by condensation with chloranil, the cyclization takes place in oleum where, besides ring closure, the 2-hydroxyethyl-sulfonyl groups are also esterified to 3-sulfooxyethylsulfonyl groups [vinylsulfone (VS) groups]. Thus, the reactive anchor is formed concurrently during the cyclization reaction [64,65] (Scheme 3.2) ... 

Fig. 28. Hydration dependence of chymotrypsin acylation. Dependence on relative humidity ( plp,) of the extent of conversion of the amide substrate, iV-succinyl-L-phenylalanine-p-nitroaniline (SPN), to the nitroaniline product and acyl enzyme, for a 1 1 SPN-o-chymotrypsin powder of nominal pH 7.5. Reaction time was 5-7 days. The weight percentages of sodium acetate present in the powder were curve 1, 0% curve 2, 6.4% curve 3, 12% curve 4, 17% and curve 5,56.5%. The ordinate, A = D416/DJ57, is a measure of the nitroaniline product. (From Khurgin etal., 1977.)...

A mixed self-assembled monolayer was used for the aptamer immobilization on the gold electrode. The aptamer-modified electrodes were then incubated for 1 h at 37°C with thrombin (18 ag/mL). Electrochemical measurements were recorded in the thin-layer cell configured to contain a total volume of 20 [xL. Thrombin chromogenic substrate (/3-Ala-Gly-Arg-p-nitroaniline) was injected into the cell and differential pulse voltammetry (DPV) measurements between -0.2 and -1V with a pulse height of—0.05 V and pulse duration of 70 ms were carried out. The DPV measurements showed that /3-Ala-Gly-Arg-p-nitroaniline substrate and the p-nitroaniline product have different redox potentials. Moreover, the DPV experiments showed a current peak at -0.45 V in the presence of the thrombin substrate. After 5 min, the peak at —0.45 V decreased and a new peak was detected at -0.70 V, indicating the formation of p-nitroaniline. The same measurements carried out on a control electrode in order to test the specificity of the assay in this experiment bovine serum albumin (BSA) substituted thrombin and in this case only the peak at 0.45 V was measured. 

Amino-5-methylthiazole does not react with diazotized p-nitroaniline in solutions acidified with acetic or hydrochloric acid (391). 2-Amino-4,5-dimethylthiazole with the diazonium salts of para-substituted anilines, however, gives product 193, involving reactivity of the exocyclic nitrogen (Scheme 122) (399). 

The procedure of simultaneous extracting-spectrophotometric determination of nitrophenols in wastewater is proposed on the example of the analysis of mixtures of mono-, di-, and trinitrophenols. The procedure consists of extraction concentrating in an acid medium, and sequential back-extractions under various pH. Such procedures give possibility for isolation o-, m-, p-nitrophenols, a-, P-, y-dinitrophenols and trinitrophenol in separate groups. Simultaneous determination is carried out by summary light-absorption of nitrophenol-ions. The error of determination concentrations on maximum contaminant level in natural waters doesn t exceed 10%. The peculiarities of application of the sequential extractions under fixed pH were studied on the example of mixture of simplest phenols (phenol, o-, m-, />-cresols). The procedure of their determination is based on the extraction to carbon tetrachloride, subsequent back-extraction and spectrophotometric measurement of interaction products with diazo-p-nitroaniline. 

Diaminoazobenzene was reported by Nietzki to have been prepared by diazotizing -nitroaniline and coupling the product with aniline. The resulting 4-nitrodiazoaminobenzene is rearranged and the nitro group reduced. The submitters tried several times to carry out this procedure but were unsuccessful. 4,4 -Diaminoazobenzene has been prepared by the oxidation of -nitroaniline with potassium persulfate followed by the reduction of the nitro groups. ... 

Ho, the acidity function introduced by Hammett, is a measure of the ability of the solvent to transfer a proton to a base of neutral charge. In dilute aqueous solution ho becomes equal to t d Hq is equal to pH, but in strongly acid solutions Hq will differ from both pH and — log ch+. The determination of Ho is accomplished with the aid of Eq. (8-89) and a series of neutral indicator bases (the nitroanilines in Table 8-18) whose pA bh+ values have been measured by the overlap method. Table 8-19 lists Ho values for some aqueous solutions of common mineral acids. Analogous acidity functions have been defined for bases of other structural and charge types, such as // for amides and Hf for bases that ionize with the production of a carbocation ... 

The corresponding reaction with 2-methylamino-5-nitroaniline affords an unambiguous synthesis of l-methyl-6-nitroquinoxaIin-2-one, the A -mcthyl derivative of (6) this product is also obtained by treatment of (6) with methyl iodide and methanolic sodium methoxided ... 

A methanolic solution of a V-alkyl-2-nitroaniline (13.3 mmol) was hydrogenated at 20 C and atmospheric pressure in the presence of Raney nickel, filtered and treated with coned HCI (1.32 mL, 13.3 mmol), followed by sodium dicyanimide (1.17 g, 13.1 mmol) in H20 (5 mL). The mixture was heated in an open vessel on a steam bath for 1 h, by which time most of the McOH had evaporated. The resulting suspension of a black oil was treated with a solution of picric acid (6.0 g, 26.2 mmol) in MeOH, whereupon the dipicrate of the product separated as yellow crystals. 

The bis amido complex [Au(bipy)(NHC6H4N02-4)2][Pp6] (43) has been similarly obtained by reaction of 40 with p-nitroaniline in acetone solution (Equation 2.14 in Scheme 2.6) [45b]. Complex 40 promotes the stoichiometric oxidation of various amines different from p-nitroaniline. Azotoluene is the main organic product of the... 

At the moment, only three in vitro studies have been performed on Bfx metabolic behavior, hi one case, it has been shown that Bfxs are able to be reduced by oxyhemoglobin to the corresponding o-nitroaniline derivatives (Scheme 5) [237]. hi the reaction between compoimd 135 and oxyhemoglobin compound 136 was generated as secondary product resulting from both nitrile hydrolysis and deoxygenation. This study indicates that blood is a possible site for metabolism of Bfxs with the consequent methemoglobinemia. 

LDPE or HDPE extracts has been determined colorimet-rically at 430 nm by oxidation with H202 in the presence of H2S04 [66]. p-Phenylenediamine derivatives such as Flexzone 3C, used as antiozonants in rubber products, have been determined colorimetrically after oxidation to the corresponding Wurster salts [67]. A wide range of amine AOs in polyolefins has been determined by the p-nitroaniline spectrophotometric procedure [68]. Monoethanolamine (MEA) in a slip agent in PE film has been determined as a salicylaldehyde derivative by spectrophotometric quantification at 385 nm [69]. Table 5.6 contains additional examples of the use of 1JV/VIS spectrophotometry for the determination of additives in polymers. 

There is a preparative hazard for this reaction product of A-methyl-p-nitroaniline... 

A method was described for the determination of niclosamide in simulated gastric and intestinal media using spectrophotometry at 386 nm [55], The method obeyed Lambert-Beer s law at 2-16 pg niclosamide/mL. Alkaline hydolysis of niclosamide gave two products, 5-chlorosalicylic acid and 2-chloro-4-nitroaniline. Niclosamide appeared to be stable in simulated gastric and intestinal media. 

The stability of niclosamide was studied in simulated gastric and intestinal juices, with and without enzymes, after incubation at 37°C. The remaining intact drug and its degradation products (2-chloro-4-nitroaniline and 5-chlorosalicylic acid) were extracted with chloroform/methanol (5 1) and determined by TLC and HPLC. The drug was stable in these media for at least 6 h [68]. 

A gas liquid chromatographic (GLC) method was described for determining residues of Bayer 73 (2-aminoethanol salt of niclosamide) in fish muscle, aquatic invertebrates, mud, and water by analyzing for 2-chloro-4-nitroaniline, a hydrolysis product of Bayer 73 [83]. Residues were extracted with acetone-formic acid (98 + 2), and partitioned from water samples with chloroform. After sample cleanup by solvent and acid base partitioning, the concentrated extract was hydrolyzed with 2N NaOH and H202 for 10 min at 95°C. The 2-chloro-4-nitroaniline was then partitioned hexane ethyl ether (7 + 3) and determined by electron capture GLC. Average recoveries were 88% for fish, 82% for invertebrates, 82% for mud, and 98% for water at 3 or more fortification levels. 

Hassan et al. [39] used a sensitive color reaction method for the determination of primaquine in pharmaceutical preparation. Primaquine was treated with diazo-p-nitroaniline in acidic medium to give an orange-yellow product with an absorbance maximum at 478 nm. When the medium was made alkaline, bathochromic, and hypochromic shifts occurred the new maximum was located at 525 nm. The mean percentage recoveries for authentic samples amounted to 100 and 100.21 by the acid and alkaline procedures, respectively (P = 0.05). Both reactions could be used to determine primaquine salts in pharmaceutical preparations. The results obtained were in good agreement with those of the official methods. Recoveries were quantitative by both methods. 

Azide 367 is prepared from 4-r -butyl-2-nitroaniline in 76% yield by its diazotization followed by treatment with sodium azide. In a 1,3-dipolar cycloaddition with cyanoacetamide, azide 367 is converted to triazole 368 that without separation is directly subjected to Dimroth rearrangement to give derivative 369 in 46% yield. Reduction of the nitro group provides ortfc-phenylenediamine 371 in 91% yield <2000EJM715>. Cyclocondensation of diamine 371 with phosgene furnishes benzimidazol-2-one 370 in 39% yield, whereas its reaction with sodium nitrite in 18% HC1 leads to benzotriazole derivative 372, which is isolated in 66% yield (Scheme 59). Products 370 and 372 exhibit potassium channel activating ability <2001FA841>. 

Two commercial disazo disperse dyes of relatively simple structure were selected for a recent study of photolytic mechanisms [180]. Both dyes were found to undergo photoisomerism in dimethyl phthalate solution and in films cast from a mixture of dye and cellulose acetate. Light-induced isomerisation did not occur in polyester film dyed with the two products, however. The prolonged irradiation of Cl Disperse Yellow 23 (3.161 X = Y = H) either in solution or in the polymer matrix yielded azobenzene and various monosubstituted azobenzenes. Under similar conditions the important derivative Orange 29 (3.161 X = N02, Y = OCH3) was degraded to a mixture of p-nitroaniline and partially reduced disubstituted azobenzenes. 

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