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Sulfonation enzymatic

The enzymatic oxygenation process is of particular value as there is a significant difference in the formation rates of sulfoxides and sulfones. The initial conversion of sulfide to the optically active sulfoxide by an MO is usually very fast compared to the subsequent oxidation step to sulfone, upon which chirality is lost (Scheme 9.26). In many cases, over-oxidation to sulfone is not observed at all when employing MOs. [Pg.253]

The method is not restricted to secondary aryl alcohols and very good results were also obtained for secondary diols [39], a- and S-hydroxyalkylphosphonates [40], 2-hydroxyalkyl sulfones [41], allylic alcohols [42], S-halo alcohols [43], aromatic chlorohydrins [44], functionalized y-hydroxy amides [45], 1,2-diarylethanols [46], and primary amines [47]. Recently, the synthetic potential of this method was expanded by application of an air-stable and recyclable racemization catalyst that is applicable to alcohol DKR at room temperature [48]. The catalyst type is not limited to organometallic ruthenium compounds. Recent report indicates that the in situ racemization of amines with thiyl radicals can also be combined with enzymatic acylation of amines [49]. It is clear that, in the future, other types of catalytic racemization processes will be used together with enzymatic processes. [Pg.105]

Oxime carbamates are not directly amenable to gas chromatography (GC) because of their high thermal instability, which often leads to their breakdown at the injection port or in the column during analysis. Analysis of oxime carbamates by GC with sulfur detection or flame photometric detection involves oxidation of the intact insecticides or alkaline hydrolysis to form the more volatile but stable oxime compound. Enzymatic techniques have been reported for the analysis of these compounds. Enzyme-linked immunosorbent assay (ELISA) has been used to determine aldicarb and its sulfone and sulfoxide metabolites and methomyl in water, soil, and sediment samples. [Pg.1144]

Despite the higher selectivity of enzymatic methyl transfer over chemical methylation, where toxic or hazardous reagents are often employed, such as methyl sulfonate and diazomethane, the synthetic applications of these enzymes have been largely ignored primarily as a result of high costs associated with the cofactor SAM. Recent efforts have been directed to in vivo methylation, where SAM may be regenerated inside cells. For example, methyl benzoate production was engineered in recombinant Saccharomyces cerevisiae and in vivo... [Pg.308]

Desulfurization using purified enzymes Investigations into enzymatic desulfurization as an alternative to microbial desulfurization has revealed several enzymes capable of the initial oxidation of sulfur. A study reported use of laccase with azino-bis-(3-ethylbenzothiazoline-6-sulfonic acid) (ABTS) as a mediator for oxidation of DBT [181]. The rate of this reaction was compared to hydrogen peroxide-based phosphotungstic acid-catalyzed oxidation and the latter was found to be about two orders of magnitude higher. The authors also oxidized diesel oil sulfur to no detectable levels via extraction of the oxidized sulfur compounds from diesel. In Table 9, the enzymes used in oxidation of DBT to DBTO are reported. [Pg.102]

Rhin(bpy)3]3+ and its derivatives are able to reduce selectively NAD+ to 1,4-NADH in aqueous buffer.48-50 It is likely that a rhodium-hydride intermediate, e.g., [Rhni(bpy)2(H20)(H)]2+, acts as a hydride transfer agent in this catalytic process. This system has been coupled internally to the enzymatic reduction of carbonyl compounds using an alcohol dehydrogenase (HLADH) as an NADH-dependent enzyme (Scheme 4). The [Rhin(bpy)3]3+ derivative containing 2,2 -bipyridine-5-sulfonic acid as ligand gave the best results in terms of turnover number (46 turnovers for the metal catalyst, 101 for the cofactor), but was handicapped by slow reaction kinetics, with a maximum of five turnovers per day.50... [Pg.477]

Anaerobic bio-reduction of azo dye is a nonspecific and presumably extracellular process and comprises of three different mechanisms by researchers (Fig. 1), including the direct enzymatic reduction, indirect/mediated reduction, and chemical reduction. A direct enzymatic reaction or a mediated/indirect reaction is catalyzed by biologically regenerated enzyme cofactors or other electron carriers. Moreover, azo dye chemical reduction can result from purely chemical reactions with biogenic bulk reductants like sulfide. These azo dye reduction mechanisms have been shown to be greatly accelerated by the addition of many redox-mediating compounds, such as anthraquinone-sulfonate (AQS) and anthraquinone-disulfonate (AQDS) [13-15],... [Pg.88]

Buynak et al. [53] synthesized several 6-(mercaptomethyl) penicillanates (9r and 9s, Table 1) that include both C-6 stereoisomers as well as the sulfide and sulfone oxidation states of the penam thiazolidine sulfur. Selected mercaptomethyl penicillanates inactivated both metallo- and serine /5-lactamases, and displayed synergism with piperacillin against various //-lactamase-producing strains, including metallo-/5-lactamase-producing P. aeruginosa strain. Compound 9r would be capable of bidentate chelation of zinc subsequent to enzymatic hydrolysis of the /5-lactam (Scheme 3). [Pg.239]

The esterification of acetic acid with ethanol using sulfonic ion-exchange resins as catalyst/selective sorbent was studied by Mazzotti et al. [164]. The authors developed a detailed mathematical model, which was able to predict correctly the system s behavior. They succeeded in obtaining 100% conversion of acetic acid in addition to a complete separation. Several other studies involving enzymatic reactions were also carried out and will be presented in more detail in the next section. [Pg.195]

Disulfoton causes neurological effects in humans and animals. The mechanism of action on the nervous system depends on the metabolism of disulfoton to active metabolites. The liver is the major site of metabolic oxidation of disulfoton to disulfoton sulfoxide, disulfoton sulfone, demeton S-sulfoxide and demeton S-sulfone, which inhibit acetylcholinesterase in nervous tissue. These four active metabolites are more potent inhibitors of acetylcholinesterase than disulfoton. Cytochrome P-450 monooxygenase and flavin adenine dinucleotide monooxygenase are involved in this metabolic activation. The active metabolites ultimately undergo nonenzymatic and/or enzymatic hydrolysis to more polar metabolites that are not toxic and are excreted in the urine. [Pg.90]

Kurz, L.C. and Erieden, C. (1977). Comparison of the structures of enzymatic and nonenz3fmatic transition states. Reductive desulfonation of 4-X-2,6-dinitrobenzene-sulfonates by reduced nicotinamide adenine dinucleotide. Biochemistry 16, 5207 -5216... [Pg.75]

Sulfoxidation reactions are characterized by enzymatic conversion of a divalent compound to sulfoxide (Fig. 15.7) or, in some cases, to sulfone (S SO O ). The degradation also may be catalyzed by minerals, converting organic sulfides (thioesters) and sulfites to the corresponding sulfoxides and sulfates. Because it is difficult to determine if the reaction is chemically or biologically induced, microbially mediated sulfoxidation in the subsurface environment can be established only when a biocatalyst is found. [Pg.309]

For the analytical characterization of sulfated tyrosine peptides, spectroscopic methods as well as amino acid analysis and, more recently, mass spectrometry are employed. In Table 2 the spectroscopic data of tyrosine 0-sulfate are compared to those of the related sulfonic acid derivatives as possible byproducts in the chemical sulfation of the tyrosine or tyrosine peptides.[361 In the course of the synthesis of tyrosine 0-sulfate peptides and, particularly in the final deprotection step, desulfation may occur which limits the characterization of the final compounds in terms of quantitative identification of the tyrosine 0-sulfate. This is achieved by amino acid analyses of basic hydrolysates of the sulfated tyrosine peptides or preferably by analyses of the enzymatic hydrolysates with aminopeptidase M or leucine-aminopeptidase. [Pg.429]


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See also in sourсe #XX -- [ Pg.225 , Pg.228 , Pg.229 ]




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Enzymatic Synthesis of Sulfonic Acid Derivatives

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