棉铃虫蜕皮时期同工酶表达模式

同工酶广泛存在于不同种属生物的组织细胞中,在生物发育的不同阶段有着特定的表达模式和重要的生理功能。昆虫蜕皮是在促前胸腺激素（PTTH）、蜕皮激素和保幼激素共同控制下由一系列基因表达和调控的级联反应。阐明蜕皮发育过程中同工酶的表达模式,可以为研究蜕皮的分子机理提供新的分子靶标,为研制生长调节剂类杀虫剂提供检测的分子标记。该研究分析了棉铃虫Helicoverpa armigera蜕皮时期不同组织中过氧化物酶、乙醇脱氢酶和酯酶的表达模式,找到了3种蜕皮差异表达的过氧化物酶, 2种蜕皮或变态差异表达的乙醇脱氢酶,3种蜕皮差异表达的酯酶。生长调节剂类化学杀虫剂非甾醇类蜕皮激素竞争物RH24-85可以诱导3种酯酶表达上调,可能与蜕皮有关。这些结果为进一步研究棉铃虫蜕皮的分子机理和检测促蜕皮生长调节剂类化学杀虫剂提供了新的分子靶标。     

Characterization of the esterase isozymes of Ips typographus (coleoptera,scolytidae)

Four esterase isozymes hydrolyzing α-naphthyl acetate (α-NA) were detected screening whole body homogenates of larvae and adults of Ips typographus by electrophoresis. Two of the four isozymes (isozymes 3 and 4) were not detected by α-NA staining in the pupal stage, but topical application of juvenile hormone III (JH III) on the pupa induced these isozymes. The JH esterase (JHE) activity on the gel was associated with the proteins of isozyme 2. The compounds OTFP, PTFP, and DFP inhibited this catalytic activity of isozyme 2 on the gel at low concentrations, whereas the proteins of isozyme 3 and 4 were affected only at higher concentrations. A quantitative developmental study was performed to characterize which of the esterases hydrolyzed JH III, using a putative surrogate substrate for JH (HEXTAT) and α-NA. The I₅₀ of several esterase inhibitors and the JH metabolites were also defined. All findings supported the results that a protein associated with isozyme 2 is catabolizing JH and that isozymes 3 and 4 are the main contributors to the general esterase activity on α-NA. The JHE from Tenebrio molitor was purified by affinity chromatography. Although the recovery was low, an analytical isoelectric focusing gel showed that the JHE activity of the purified enzyme. T. molitor cochromatographed at the same pl as the JHE activity of I. typographus. Arch. Insect Biochem. Physiol. 34:203–221, 1997. © 1997 Wiley-Liss, Inc.     

Developmental genetics of the esterase isozymes of Fundulus heteroclitus

The ontogeny of the esterase isozymes of the teleost, Fundulus heteroclitus, has been investigated. One group of esterase isozymes is present at all stages of development, whereas other esterase isozymes only very gradually appear at later stages of development, or abruptly appear at such dramatic developmental events as hatching. The ontogeny of these isozyme patterns is interpreted as the expression of differential regulation of separate esterase genes. The general pattern of teleost esterase gene activation is similar to that reported for birds and mammals. Allelic variation was detected at two of the esterase loci. On the basis of electrophoretic mobility, substrate specificity, inhibitor specificity, genetic variation, and ontogeny of esterases, there appear to be at least 15 different esterase isozymes, which constitute 6–8 groups, each of which is probably encoded in one or more genetic loci.This study was supported by NSF Grant GB 544OX to Professor C. L. Markert and an NSF Graduate Fellowship to G. S. Whitt.     

Intersyngenic variations in the esterases of axenic stocks of Paramecium aurelia

The esterase isozymes were surveyed in axenic stocks of syngens 1, 2, 4, 5, 6, and 8 of Paramecium aurelia by starch gel electrophoresis. In paramecia there appear to be four types of esterases which are clearer in axenic than in bacterized stocks. Each type differs in its substrate specificity and/or its response to the inhibitor eserine sulfate. Minor variations in type D esterases sometimes occur in different extracts of the same stock and may result from changes in the temperature of growth of the cells or growth cycle differences. Differences in the mobility of the A, B, or C (cathodal) types of esterases may occur in different syngens. They also occur for the A and B types among stocks within a syngen, but the frequency is low, except in the case of syngen 2. Since each of the types of esterases varies independently, at least four and possibly more genes appear to specify the esterases in the species complex. Some pairs of syngens vary in their electrophoretic positions for all types of esterases. Other pairs have identical zymograms. This observation suggests that some syngens may differ from each other by as many as four esterase genes, while others may not differ at all. The difference between P. aurelia and Tetrahymena pyriformis in the degree of intrasyngenic variation observed for enzymes is discussed in relation to other types of characters, the organization of the genetic material in the macronucleus, the presence of symbionts, and their breeding systems. It is suggested that enzyme variation is achieved by the action of different selective forces in these two groups of ciliated protozoa.Supported by research grants from the National Institute of General Medical Sciences (GM-15879), U.S. Public Health Service, and from the British Medical Research Council.     

Biochemical properties of amylase isozymes from Gammarus palustris. A comparative study

Two major α-amylase isozymes from Gammarus palustris were purified and characterized. These isozymes, Amy I^w and Amy I^c, exhibit a seasonal pattern of expression. In this article we investigate whether the seasonal variation has an adaptive significance. In addition, the species-specific properties of amylases were studied. Purification of the isozymes was achieved by sequential glycogen-ethanol precipitation, Sephadex G-200 and ion exchange chromatography. Characterization in terms of K_m, activity patterns at different temperatures, pH values and salt concentrations was done for both isozymes. In addition, the distribution of enzymatic products was analyzed in a high-performance liquid chromatography system. In all conditions tested, the two isozymes gave similar results. This observation suggests that the seasonal change in amylase expression pattern does not result in enzymes differentially suited for seasonal variation in conditions. A comparative analysis showed that G. palustris amylases are apparently distinct from other amylases. These distinctions were seen as an unusually low K_m value, an activity peak at low NaCl concentration, a relatively high pH optimum and the predominant formation of maltotriose.     

Geographic Variation of Esterase Isozymes in Populations of Alternaria mali on Apple Leaves

The 500 monoconidial isolates of Alternaria mali occurring in different locations, Suweon, Cheongju, Kochang, Daegu and Jinju, Korea, in 1983 were used to examine geographic variation of esterase isozymes. The electrophoretic patterns of esterases were qualitatively and quantitatively different between isolates. The 14 different bands were detected on the basis of the decreasing electrophoretical mobility, although all bands were not present in any of the isolates. A comparison of the frequency of esterase isozymes at different bands showed marked variations among the geographic locations. The geographic distance between A. mali populations did not correlate strongly with divergence in esterase isozymes, whereas A. mali populations within a geographic feature were more closely related than populations separated by a mountain range.     

Genetic variability of leaf esterases in Triticum aestivum L. 2n=6x=42

Summary Starch gel electrophoresis with two different buffer systems and several substrates and inhibitors have been used to study the electrophoretic variability of esterases in leaves of cultivars of Triticum aestivum. Each one of the buffer systems showed different levels of variability, according to the electrophoretic patterns. At the same time green and etiolated leaves showed different patterns in each buffer system. The variability was dependent upon the developmental stage of the leaves. According to the results from chromosomal location, the genes controlling esterases in green leaves were located in homoeology group 3, while the genes controlling esterases in etiolated leaves were in homoeology group 6. But both esterase isozymes showed a similar electrophoretic migration and a similar reponse to substrates and inhibitors. The possible origin of both sets of genes due to an interchromosomal duplication is discussed.     

Esterase isozymes in a solitary bee,Megachile rotundata (fab.): Characterization,developmental multiplicity,and adult variability

This study describes the biochemical characterization and genetic variation of cytosolic esterases in the alfalfa leafcutting bee,Megachile rotundata (Fab.). Esterase isozymes were separated by nondenaturing polyacrylamide gel electrophoresis and isoelectric focusing and characterized by inhibition with eserine sulfate, EDTA, paraoxon, andp-hydroxymercuribenzoate. Based on inhibition patterns and substrate specificity, there are major differences between adults and immature forms and more subtle differences between male and female adults. M. rotundata esterases are largely organophosphate sensitive and the two major adult allozymes were highly variable within the population examined. Differences in esterase expression between life stages with respect to niche and the occurrence of diploid males are discussed.     

Nonspecific esterase isozymes that focus at identical isoelectric points are kinetically analogous

Isoelectric focusing (IEF) of soluble nonspecific esterases of rat kidney and testis exhibits an identical array of organophosphate-resistant cathodal isozymes. To ascertain whether such isozymes that focus at the same pI are also kinetically analogous, two isozymes, both focused at pI 7.2, were isolated, one from each organ, by elution from cut-out, unstained gel segments. Although the esterases of the whole soluble fraction of kidney and testis exhibited different kinetic properties and organophosphate susceptibility, no differences were observed with regard to the isozymes. Therefore, because of similar electrophoretic and kinetic behavior, the two isozymes can be regarded as phenotypic expressions of similar genetic products.     

Intersyngenic variations in the esterases of bacterized Paramecium aurelia

The esterase isozymes were surveyed in bacterized stocks representative of all 14 syngens of Paramecium aurelia by starch gel electrophoresis. The properties of substrate specificity and independent variation of particular isozymes permit the ordering of the differences observed among stocks. Differences can arise from several sources: bacterial variation, intrasyngenic variation, and intersyngenic variation. Bacterial esterases tend to be found in certain zonal areas (see Rowe et al., 1971) and produce minor stock differences, which are erratic in their distribution. Unlike the situation found in Tetrahymena pyriformis, major intrasyngenic variations are rare in P. aurelia except in syngen 2. This lack of intrasyngenic variation is significant in view of the wide differences in geographic origin and micronuclear chromosome numbers among stocks within a syngen. It suggests that certain esterase genotypes must be under stringent selection within a syngen. The lack of intrasyngenic variation permits assessment of intersyngenic relationships. Syngens differ in a complex way from each other, suggesting that several gene differences may be involved. The syngens can be classified on the basis of their esterases. Syngens which have been shown to be more closely related in terms of cross-mating, breeding systems, and other criteria tend to be more similar in their esterase isozymes. The isozyme technique confirms relationships previously suggested among syngens and offers the promise of eventual assessment of evolutionary distances among syngens. However, establishment of these relationships will be clearer in the absence of bacteria.Supported by a Research Grant, GM-15879, from the National Institute of General Medical Sciences, U.S. Public Health Service     

Intersyngenic variations in the esterases and acid phosphatases of Tetrahymena pyriformis

The esterase and acid phosphatase isozymes were surveyed in strains of syngens 2–12 under conditions found to be optimal for syngen 1. Both intersyngenic and intrasyngenic variations were found. Comparisons of the esterases suggest that homologous enzymes are present in certain syngens and that some ordering of the variations with respect to syngen differences is possible. The acid phosphatases are highly polymorphic in different strains even within a syngen, and the variations cannot be ordered with respect to syngen differences. These results are discussed in terms of other types of studies directed at assessing syngen relationships and in terms of the sources of variation. It was concluded that only characters less vulnerable to intraclonal variation will be capable of revealing syngen relationships.Supported by a Research Grant, GM-15879, from the National Institute of General Medical Sciences, U.S. Public Health Service.     

Two δ1-pyrroline-5-carboxylate dehydrogenase isoforms are expressed in cultured Nicotiana plumbaginifolia cells and are differentially modulated during the culture growth cycle

δ¹-Pyrroline-5-carboxylate (P5C) dehydrogenase (EC 1.5.1.12) activity was measured in extracts from cultured tobacco (Nicotiana plumbaginifolia Viviani) cells. Two putative isozymes were resolved by anion-exchange fast protein liquid chromatography. These enzyme forms showed different patterns of expression during the culture growth cycle: activity-I increased in exponentially growing cells and declined rapidly in late logarithmic phase, while activity-II was found at substantial level only in cells which were entering the stationary phase. Both P5C dehydrogenases were partially purified and characterized with respect to kinetic and biochemical properties. They showed similar molecular masses as judged from retention patterns upon gel-filtration chromatography. The in vitro activity of both enzymes had a broad maximum around pH 7.4, and was progressively inhibited by Cl⁻ at concentrations ranging from 0.1 to 1 M. A pronounced difference was found between their apparent K _m values for the two substrates, P5C and NAD⁺, the higher affinities being shown by activity-I. Regulation of P5C dehydrogenase during salt-stress-induced proline accumulation was investigated. Following the addition of 175 mM NaCl to the culture medium the level of activity-I was substantially unaffected, while the specific activity of the other isozyme failed to increase even after the onset of the stationary phase of growth. Possible roles for P5C dehydrogenase isozymes in proline and arginine metabolism are discussed. Received: 23 May 1996 / Accepted: 18 December 1996     

Isoenzyme Polymorphism in Flowering Plants

Esterases, leucine aminopeptidases, catalases and acid phosphatases from pollen of Oenothera organensis were studied electrophoretically. A study was made using several different extraction media to see the effect it had on esterase migration and stainability. It was found that different extraction media resulted in significant changes in migration rates and stainabilities of the esterase isozymes. Anodal esterases and leucine aminopeptidases from 13 inbred lines of maize were studied and are reported. Preliminary genetic studies of two of the esterase isozymes from maize pollen are reported. A survey of anodal esterases and leucine aminopeptidases from the pollen of 11 genera of diverse angiosperms is presented.     

Radiation-induced Cleavage of Esters of Phosphoric Acid in Aqueous Solutions

Microbiological conversion of α-terpineol to borneol and terpinolene was studied with a newly isolated microorganism. Borneol is assumed to be an end-product of the degradation of α-terpineol by the organism, but with terpinolene this is not the case because of its poor reproducibility. The strain through the results of physiological tests was tentatively identified as Ps. aeruginosa.     

Malate Dehydrogenase Isozymes (MDH; EC 1.1.1.37) in Long-Term Callus Culture of Cereus peruvianus (Cactaceae) Exposed to Sugar and Temperature Stress

Malate dehydrogenase (MDH; EC 1.1.1.37) isozymes in long-term callus tissue culture of Cereus peruvianus were studied in starch gel electrophoresis to investigate the control of differential Mdh gene expression under sugar and temperature stress. While two cytosol MDH isozymes showed an unchanged phenotype when the callus tissues were transferred to medium maintained at 22 or 37°C and containing different concentrations of sucrose, glucose, and fructose, the different combinations of five mitochondrial MDH (mtMDH) and two microbody MDH (mbMDH) showed different MDH isozyme patterns in the callus populations. Differential expression of mtMDH isozymes seems to be modulated at the posttranslational level in callus tissues exposed to different concentrations and types of sugar and to high-temperature and low-temperature stress. An inductor effect on the expression of mbMDH isozymes was observed under stress conditions and in long-term callus tissue, and they may also present different responses.     

Genetic control of enzyme polymorphisms in the California vole,Microtus californicus

Inheritance of 15 polymorphic isozymes was investigated in captive Microtus californicus. Eleven of the isozymes show patterns consistent with a Mendelian model of inheritance: glycerol-3-phosphate dehydrogenase (GPD), lactate dehydrogenases A and B (LDH-A and LDH-B), malic enzyme 2 (ME-2), isocitrate dehydrogenase 1 (ICD-1), phosphogluconate dehydrogenase (PGD), glutamate-oxaloacetate transaminase 1 (GOT-1) phosphoglucomutase 2 (PGM-2), leucine aminopeptidase (LAP), glucosephosphate isomerase (GPI), and esterase 2 (ES-2, from kidney). four of the isozymes show patterns that cannot be interpreted by a simple genetic model: esterases 1 and 4 (ES-1, ES-4, from hemolysate), esterase 3 (ES-3, from plasma), and protein 1 (PT-1). The following pairs of loci are assorting independently: LAP and PGD, LAP and PGM-2, GOT-1 and PGD, GOT-1 and GPD, LAP and GPD, GPD and PGD, GPI and PGD. Data from one test cross mating indicate that GPD and PGM-2 are loosely linked with recombination about 30%. Additional data are needed to confirm this relationship.This study was conducted while the first author was the recipient of an NIH Traineeship. The Departments of Genetics and Zoology provided financial support for the maintenance of the animal colony. This work was supported in part by an NIH-Biomed grant (3-S05-RR-07006-08S1) to W. Z. Lidicker.     

Genetic diversity and structure in a natural Elymus caninus population from Denmark based on microsatellite and isozyme analyses

 Genetic diversity in a natural Elymus caninus population from Denmark was assessed using isozyme and microsatellite markers. A total of 119 individuals from 46 maternal plants were assayed. Microsatellite loci are shown to display higher levels of variation than isozyme loci. The mean number of alleles per locus was 1.04 for isozymes and 1.38 for microsatellites. The percentage of polymorphic loci for isozymes and microsatellites was 4.7% and 23.6% across the maternal plant, respectively. The genetic diversity at population level was 0.1 for isozymes, and 0.63 for microsatellites. The mean genetic diversity at maternal plant level was 0.027 for isozyme loci and 0.117 for microsatellite loci. The average of total allozyme diversity (H_T) was 0.22. The average of total microsatellite diversity was 0.56. Isozyme and microsatellite variation showed the same pattern of differentiation between maternal plants. More than 75% total genetic diversity was found among maternal plants. About 25% total genetic diversity was detected within maternal plants. Ten (22.7%) maternal plants produced heterozygous offspring at allozyme loci, and 30 (68.2%) maternal plants gave heterozygous offspring at microsatellite loci. Both types of markers revealed a relatively high genetic diversity in this population. Received November 7, 2000 Accepted February 15, 2001     

Differential glycosylation produces heterogeneity in elevated esterases associated with insecticide resistance in the brown planthopper Nilaparvata lugens Stål

The major insecticide resistance mechanism in the brown planthopper Nilaparvata lugens involves overproduction of esterases. Esterases purified from a resistant strain appeared as a ladder of bands on isoelectric focussing (IEF) gels from pI 4.7 to 5.0. Two-dimensional electrophoresis showed that isozymes ranged in size from 66 to 68 kDa with those of lower pI being apparently smaller. All isozymes detected by two-dimensional electrophoresis were glycosylated. N-glycosidase A reduced the number of isozymes on IEF to two, with increased pI and an increased molecular weight of 69 kDa. No O-linked glycans were detected. Deglycosylation had no effect on esterase activity, hence glycosylation is not involved in active site conformation. As N-glycosidase F completely deglycosylated the esterases, none of the glycans has an alpha1,3-bound core fucose. Reactivity with the lectins GNA, MAA and DSA, combined with differential cleavage of N-linked glycans with endoglycosidases F1 and F2, indicated that terminally linked mannose is present in high mannose and/or hybrid type glycans and that terminally linked sialic acid and galactose-beta(1-4)-N-acetylglucosamine are present in biantennary complexes. Neuraminidase treatment had the same effect on pI of isozymes as complete deglycosylation. Therefore, the majority of the heterogeneity of elevated esterases on IEF is due to differential attachment of sialic acid to glycans of the two proteins.     

Linkage conservation of homologous esterase loci in fish (Cyprinodontoidei: Poeciliidae)

Homologies among esterase isozymes in fish in the poeciliid genera Poeciliopsis and Xiphophorus are proposed. Esterase homologies are based on their tissue distributions and inhibition and substrate properties. The five esterases include two carboxylesterases, one eserine sulfate-sensitive esterase, and two esterases resistant to inhibition, one of which reacts only with acetate esters. Linkage studies in Poeciliopsis monacha indicate that the loci encoding the two carboxylesterases are linked to each other and to the locus for eye-specific lactate dehydrogenase. Comparisons of the linkage reported here with earlier studies in Xiphophorus suggest that there is a large region of linkage homology in the genetic maps of Poeciliopsis and Xiphophorus.This work was supported by grants from the National Science Foundation (DEB76-19285) to R. C. Vrijenhoek and the Charles and Johanna Busch Fund to R. C. Vrijenhoek and N. H. Hart. J. F. L. and P. J. P. were supported by U.S. Public Health Service Genetics Training Grant GM07129-04.     

Possible common origin of glucosyltransferases in Oscillatoria princeps

Gel electrophoresis of the glucosyltransferases of the blue-green alga, Oscillatoria princeps, followed by immunodiffusion against anti-phosphorylase rabbit serum, showed cross-reactions of the two phosphorylase isozymes and the two synthetase isozymes of the alga. Weak cross-reactions were also obtained with the branching isozymes. Apparent extensive similarities in the structure of the phosphorylases and the synthetases were indicated. However, only partial structural similarities between the two groups of α-1,4-glucosidic bond formers and the branching isozymes exist as indicated by the weak immunological reactions obtained and the formation of “spurs” on the immunoprecipitin lines. If the synthesis of α-1,4-glucosidic linkages and the formation of α-1,6 cross linkages were at one time due to the bifunctional action of a single catalytic protein, then the separation of these two enzymatic activities took place prior to the derivation of the synthetases from the phosphorylases.