Polymorphism of transferrin and esterase in Alaskan wolves: evidence of close molecular homology with the dog

By the use of isoelectric focusing in polyacrylamide gels serum samples from 146 Alaskan wolves were studied with regard to transferrin (Tf) and esterase (ArE) polymorphism, comparing the phenotypic band patterns with those of selected Norwegian dogs. The study revealed Tf and ArE polymorphisms in the wolf with phenotypic band patterns being indistinguishable from the corresponding ones in dogs. This suggests the occurrence of the same two common Tf alleles in the wolf as in the dog. In the ArE system the results are consistent with the occurrence of three alleles which also occur in dogs whereas a fourth allele, so far not seen in dogs, is seen in Alaskan wolves.     

5-(4-Acetoxy-1-butinyl)-2,2′-bithiophene:acetate esterase from Tagetes patula

From the aerial parts of Tagetes patula, an enzyme with high substrate specificity, namely 5-(4-acetoxy-1-butinyl)-2,2′-bithiophene:acetate esterase, was partly purified. The enzyme has a MW of 67000 (±5000), pH optimum of 7.5 and its activity is affected considerably in the presence of bovine serum albumin (BSA). BSA at a concentration of 5 mg/ml in the reaction mixture prevents substrate polymerization.     

Genetics of esterases in Drosophila. VII. Genetic control of the activity level of juvenile hormone (JH)-esterase and heat resistance in D. virilis at high temperatures

The heat-resistant subline 147S was obtained in Drosophila virilis by selecting for viability individuals of heat-sensitive stock 147. It was shown that in the heat-treated 147S pupae the activity of juvenile hormone (JH)-esterase is decreased and, consequently, the titer of juvenile hormone is increased compared with those in the control pupae. These changes are consistent with those observed earlier for resistant stock 101. Heat-resistant stocks 101 and 147S were crossed with heat-sensitive stock 147, whose heat-treated larvae show earlier activation and higher activity of JH-esterase than control larvae. The viability and electrophoretic esterase patterns were analyzed in the F₁ and F₂ hybrids at different temperatures. It was found that the F₁ hybrid is resistant to the effect of high temperature and its activity level of JH-esterase is lower compared with controls. In the F₂ hybrid, there was a 3:1 segregation of viability and a 1:2:1 segregation of the activity level of JH-esterase at high temperatures. It is concluded that the activity level of JH-esterase and heat resistance in D. virilis are monogenically controlled at high temperatures.     

Molecular-genetic mechanisms regulating tissue-specific expression of the drosophilaestS gene

A study was made of theDrosophila melanogaster est6 andD. virilis estS genes for tissue-specific esterase, and their expression at various stages of development was characterized. The former has one promoter and is expressed in the seminal ducts, whereas the latter has two promoters and is expressed in the seminal bulbs. In transgenicD. melanogaster, estS was expressed in the seminal bulbs, as observed in the donor. A region adjacent to the structural gene proved responsible for its expression in the seminal bulbs. TransgenicD. melanogaster lines were also obtained with constructs containing various fragments of theestS regulatory region and thelacZ reporter gene. Histochemical analysis with X-Gal staining allowed identification of a region that inhibitsestS expression in all organs other than seminal bulbs. An esterase S homolog was found in a marine mollusk.     

Investigation of kinetics of immobilized liver esterase by flow calorimetry

Flow calorimetry (FC) was shown to be a powerful tool for investigation of the kinetics of phenyl acetate hydrolysis catalyzed by pig liver carboxyl esterase. The enzyme was immobilized in alginate gel particles that were placed in a calorimetric flow column and the heat effect of enzyme reaction was followed in single flow and total recirculation conditions. It was shown that the registered temperature change was proportional to molar amount of substrate transformed in the column. A mathematical model describing the enzyme reaction, mass transfer, and heat effects in the calorimetric system was developed and used for the kinetic data evaluation. By combining data from single flow and recirculation modes true kinetic parameters were evaluated by the proposed mathematical procedure based on the model solution and successive approximations.

The kinetic data for carboxyl esterase showed a slide substrate inhibition by phenyl acetate. The obtained kinetic parameters were as follows: Michaelis constant K_m=2 mmol dm⁻³ and substrate inhibition constant K_i=42 mmol dm⁻³. The method can be applied to kinetic study of immobilized enzymes directly in the flow calorimeter without any requirement of an independent analytical technique.     

Genetics of four plasma protein loci in Equus przewalskii: new alleles at the prealbumin, postalbumin and transferrin loci

This paper reports genetic variation at the prealbumin ( Pr ), postalbumin ( Pa ) and transferrin ( Tf ) loci in Equus przewalskii found using thin layer isoelectric focusing and an amphoteric separator. The method resolves all three loci plus serum esterase ( Es ) on a single gel, and typing of all four loci is readily achieved. In addition to the esterase alleles previously reported by Fisher & Scott (1979), five alleles were found at the Pr locus. three at the Pa locus and six at the Tf locus. Analysis of several mating types confirms inheritance is autosomal and codominant for all four loci.     

Baculo-expression and enzymatic characterization of CES7 esterase

The male reproductive tracts in different species are characterized by similar patterns of male-dependent overexpression of carboxylesterases. This phenomenon indicates male sex-associated functions of these enzymes for spermatogenesis, sperm maturation, and sperm use. Recently, a novel epididymis-specific gene named Ces7 was cloned and characterized, which belongs to the carboxylesterase family. To study the functions of CES7 in sperm maturation and storage, CES7 recombinant protein was expressed in baculovirus system. The recombinant protein had carboxylesterase activity hydrolyzing cholesterol ester and choline ester. CES7 as carboxylesterase might be involved in ester hydrolysis, sperm maturation, and storage in male reproductive tract.     

Effect of fenthion treatment on larval densities of insecticide-resistant Culex quinquefasciatus in an urban area of Sri Lanka

Abstract. In Sri Lanka the national Anti-Filaria Campaign (AFC) has routinely employed fenthion since 1974 for larvicidal control of Culex quinquefasciatus , the vector of Bancroftian filariasis in urban areas, where this mosquito breeds prolifically in polluted waters. During 1994 the efficacy of AFC fenthion treatment against organophosphate-resistant Cx quinquefasciatus was investigated at Dehiwela, near Colombo.
The AFC target rate of fenthion application was 1 mg a.i./l, but the actual concentrations of fenthion in freshly treated pits ranged from 0.64 to 63.2 mg a.i./l. There was significant suppression of larval densities in treated soakage pits, the predominant breeding site of Cx quinquefasciatus , although the mosquito population was 6-fold resistant to fenthion at the LC_W level. Production of pupae was almost completely prevented in soakage pits which were sprayed weekly with fenthion, indicating that adult mosquito emergence from this source was minimal. The rapid decline in concentration of fenthion detected in the water of soakage pits indicated that a weekly treatment schedule is essential for effective control. With the rapid recolonization of treated sites, the weekly schedule must be strictly implemented in order to achieve control of resistant larvae. Fenthion activity levels detected in treated pits suggest that a 7–10 day schedule of retreatment would completely suppress susceptible Cx quinquefasciatus.     

Esterase patterns in species of the triatome bug Rhodnius

The aim of the present study was to analyse esterase patterns in three triatomine species of Rhodnius genus. Four loci, Est 1, Est 2, Est 3 and Est 4, were found. The corresponding enzymes were characterized as carboxylesterases (E.C. 3.1.1.1) or cholinesterases (E.C. 3.1.1.8) based on inhibitory experiments, using eserine sulphate, malathion, mercury chloride, p-chloromercuribenzoate (pCMB) and iodoacetamide. Low genetic variability was observed: Est 1, Est 2 and Est 3 were monomorphic in Rhodnius domesticus , Rhodnius robustus and Rhodnius neivai , whereas locus Est 4 was polymorphic in the first two species. The UPGMA analysis based on esterase genotypic frequencies indicated greater similarity between R. domesticus and R. robustus when compared with R. neivai . The present study expands our knowledge about genetic variability among triatomines and accords with the hypothesis that R. domesticus is a species derived from R. robustus .     

Asymmetric hydrolysis of dimethyl 3-phenylglutarate catalyzed by Lecitase Ultra: Effect of the immobilization protocol on its catalytic properties

The asymmetric hydrolysis of dimethyl 3-phenylglutarate (1) by different immobilized preparations of a phospholipase A₁ (Lecitase Ultra (LECI)) at pH 7 and 25 °C has been studied. Agarose beads coated with octyl, cyanogen bromide (CNBr), polyethylenimine (PEI) or glyoxyl groups were used as supports for the immobilization of LECI. The different derivatives behaved very differently in terms of activity, discrimination between 1 and methyl 3-phenylglutarate (2) resulting from the hydrolysis of 1, enantioselectivity (in the hydrolysis of 1 to produce R or S-2) and enantiospecificity in the hydrolysis of R-2 and S-2. Using 1 mM of 1, CNBr-LECI showed the highest activity (13 × 10⁻³ μmol/min mg protein) while octyl-LECI was about 20 times less active. All the enzyme preparations mainly produced (S)-2, but with different enantioselectivity. CNBr-Lecitase was the most enantioselective, producing the S-2 10 fold more rapidly than the R-2, while octyl-Lecitase gave only half of that difference.LECI adsorbed on octyl-agarose allowed to get a yield up to 99% of S-2 (ee was 66%). The reaction stopped in the monoester and no isomer of this compound was further hydrolyzed by the enzyme. However, when the reaction was catalyzed by the other immobilized LECI preparations, the enzyme was able to hydrolyze mainly the minority isomer, permitting to improve the ee of the remaining S-2. The best results were obtained using CNBr-LECI, which gave (S)-methyl-3-phenylglutarate with a yield of 80% and an ee exceeding 99%.