Comparative esterase electrophoretic polymorphism of Escherichia coli isolates obtained from animal and human sources

To determine whether enzyme electrophoretic polymorphism in Escherichia coli populations was influenced by environmental background, the mobilities of four electrophoretically variable esterases (A, B, C and I) were examined. The distinction between isolates was established by significant differences in the electrophoretic distribution and the genetic diversity coefficient of individual esterases. Principal components analysis on each population and on all strains revealed three groups of allozymes. The first, characterized by slow electrophoretic mobilities of esterase B, was frequently observed in strains obtained from human extra-intestinal infections and rarely in commensal organisms. The second, characterized by fast mobilities of esterases A and B, was frequently found in animal isolates. The third, characterized by prominence of the most common mobilities of esterases B and A, was recovered in all populations. These results were confirmed by discriminant analysis. Among the 610 strains investigated, 316 electrophoretic types (distinctive combinations of allozymes of the four varieties of esterases) were distinguished, illustrating high esterase polymorphism.     

Shigella endotoxin protein--its electrophoretic and serological properties

The electrophoretic analysis of lipid A-associated protein (LAP), obtained from S. sonnei, in polyacrylamide gel in the presence of sodium dodecyl sulfate and urea has revealed the heterogeneity of the preparation; it has found to contain three main components with molecular weights of 43, 38 and 18 KD and some minor components with molecular weights of 49, 45 35, 30, 29, 27, 5, 21 and 14 KD. The electrophoretic mobility of the main protein components in the isolated preparation of LAP coincides with that of endotoxin components. The dissociation of proteins and lipopolysaccharide in the process of boiling the endotoxin in 2% sodium dodecyl sulfate is indicative of the noncovalent binding of these components. LAP contained in the endotoxin, in contrast to isolated LAP, is resistant to trypsin and proteinase K. The enzyme immunoassay (EIA) system with the use of LAP as a component of its solid phase has been developed, which makes it possible to carry out the quantitative determination of antibodies to this protein. The EIA system shows high sensitivity in the determination of anti-LAP IgG antibodies: in hyperimmune rabbit sera their titer is 1:250,000-1:800,000. As shown by the method of competitive EIA, the antigenic affinity of LAP of different origin corresponds to the degree of taxonomic propinquity of microorganisms: the maximal degree of cross reactions is observed between LAP obtained from S. sonnei, S. flexneri and Escherichia coli, while their affinity to Salmonella typhi is considerably less; remote microbial species (Bacterium bifidum and Sarcina marcescens) give practically no cross reactions.     

Coordinate induction of electrophoretic variants of juvenile hormone esterase

Major and minor electrophoretic variants of juvenile hormone esterase (JHE) were found in the hemolymph of last instar larvae of Trichoplusia ni, both before and after metamorphic commitment. The average ratios of activity of the two major forms were similar during both last stadium peaks in activity. Immunological analysis showed that the hemolymph concentration of JHE during this stadium paralleled the level of enzymatic activity, and no putative higher molecular weight, inactive forms were detected. Immunological analysis provided the first evidence of relatedness of major and minor forms. After hormonal stimulation, the concentration of the two major forms increased concomitantly and by a similar proportion, suggesting that charge variation, at least for these two major forms, is not a point of hormonal or developmental regulation of JHE.     

Molecular analysis of esterase D polymorphism

We have analyzed the esterase D (EsD) polymorphism at the nucleic acid level. Two common alleles, EsD¹ and EsD², are characterized by the substitution of one amino acid (Gly-to-Glu), which is caused by the point mutation of one nucleotide (G-to-A). Individuals exhibiting the EsD1 and EsD 2 phenotypes are homozygotes for EsD 1 and EsD 2 cDNAs, respectively. Individuals showing the EsD 2-1 phenotype have two kinds of cDNAs, viz., EsD 1 and EsD 2. The point mutation difference between the cDNAs of the EsD¹ and EsD² alleles results in a different SspI digestion site. A restriction fragment length polymorphism caused by this difference with respect to the SspI digestion site makes it possible to determine the EsD phenotype using DNA samples extracted from forensic materials with no EsD enzymatic activity.     

The electrophoretic polymorphism of bacterial esterases

Abstract: The specific activities of esterases and certain other molecular properties including immunospecificity indicate that the electrophoretic variations of these enzymes in bacterial populations are the result of allelic variations at specific gene loci. The esterase polymorphism of Enterobacteriaceae and some other species isolated from man or animals demonstrates that esterases can distinguish between bacteria at the species or subspecies level, both by their biochemical properties and by their electrophoretic differences. The esterase data complement DNA hybridization studies and agree with ribosomal DNA polymorphism, especially for delineating a phylogenetically distinct group of highly pathogenic strains in Escherichia coli . A two-dimensional electrophoretic profile obtained by establishing a direct correspondence between homologous esterase bands resolved by independent runs of isoelectric focusing and standard electrophoresis considerably improves the detection of allelic variations, whereas protein titration curves (electrophoresis in pH gradient) can be used to demonstrate the real electrophoretic homogeneity of allozymes or evalue their molecular relationship in terms of apparent amino acid substitutions. This overview establishes that esterases, by their significant electrophoretic polymorphism, are reliable molecular markers for systematics and epidemiology, and are suitable enzyme systems for studying population genetics and phylogeny.     

Spectrophotometric assay and electrophoretic detection of trans-feruloyl esterase activity.

Wheat bran cell walls were subjected to mild acid hydrolysis and the major phenolic product was purified and identified as 5-O-(trans-feruloyl)-arabinofuranose. Sensitive continuous and stopped, microtiter plate-based spectrophotometric assays for trans-feruloyl esterase activity were developed using this compound as substrate. Procedures were also developed for the detection of trans-feruloyl esterase activities on gels following electrophoresis using this compound. These procedures are applicable to other natural feruloyl esters derived from plant cell walls by enzymatic hydrolysis. The extracellular trans-feruloyl esterases of Aspergillus niger 814 grown on 1% wheat bran were fractionated by anion-exchange chromatography and isoelectric focusing. These studies indicate that there are multiple forms of trans-feruloyl esterase but that most activity is associated with a major isozyme with a pI of 3.2.     

An analysis of molecular polymorphism of esterase M produced by motileAeromonas strains

The high levels of electrophoretic polymorphism of esterase M detected in eight distinct hybridization groups of motileAeromonas raise questions of genetic homogeneity of the electromorphs. The 40 electromorphs detected fall in fourM _r classes—75, 80, 90, and 110 kD—and one typical variant belonging to each of these classes was purified. The four purified esterases exhibited the same resistance to heat, topH and to diisopropyl fluorophosphate, the sameK _m values for 1-naphthyl acetate and 1-naphthyl propionate (1mm), and immunological cross-reactions. Within each class, the electromorphs appeared to be related in term of single amino acid substitutions as estimated from their comparative titration patterns. The titration curves of the four purified esterases were strictly parallel suggesting close structural similarities. Thus, despite considerable variation in theirpI,M _F,andM _r values, it seems likely that the variants of esterase M are the products of closely related loci originating from a common ancestral gene.This work was supported by a grant from the Conseil Scientifique de la Faculté Xavier Bichat (Université Paris VII).     

Differentiation of Citrobacter strains using electrophoretic protein patterns

The aim of this study was checking of the usefulness of electrophoretic protein patterns in differentiation of Citrobacter strains. For analysis of whole-cell proteins 181 Citrobacter strains were prepared. Electrophoresis was performed in Mini Protean Duall Slab Cell (Bio-Rad) apparatus. Electrophoresis was carried out in 10% polyacrylamide gel according to the SDS-PAGE method of Laemmli. Whole-cell proteins of all tested Citrobacter strains gave after electrophoresis 12 to 20 bands. Patterns consisting of 12 to 20 fragments ranging in size from 70,000 to 14,000 and smaller, were not distinguishable. There were no significant differences between electrophorograms of Citrobacter strains belonging to the different species, useful for species differentiation. Identical protein band patterns were observed in the case of selected strains e.g. strains C. sedlakii studied in this study, coming from an outbreak, having the some phenotype.     

Relation between electrophoretic esterase patterns and organophosphate resistance in Musca domestica

An Italian OP-resistant strain C turned out to be heterogeneous for a gene on the 5th chromosome causing a difference in the mobility of an esterase in electrophoresis. Individuals containing only band 1 or 2 are homozygous for either allele, individuals containing esterase 1 and 2 are heterozygous. Two substrains were derived, E₁ and E₂, homozygous for the allele for 1 and 2 respectively. These strains were found to be remarkably different in OP-resistance. E₁ is approximately equally resistant as strain C, and contains the breakdown enzyme degrading paraoxon and diazoxon. E₂ has a lower resistance and does not contain the breakdown enzyme. The presence of the breakdown enzyme and the 1 esterase are controlled by the same gene allele, but they are certainly not identical. For instance the 1 band is quite stable, and is in solution in normal homogenates, whereas the breakdown enzyme is very labile and particulate. Therefore one allele, a _C1, controls both band 1 and the breakdown enzyme, the other, a _C2, seems to control only band 2. A similar situation was found in a susceptible strain, bwb; ocra, which had previously been shown to be heterogeneous for the ali-esterase a. Two alleles of the a gene are present here: the a ⁺allele controls the presence of band 1 and ali-esterase a; the a ₂allele seems to control band 2 only. The electrophoretic speed of the breakdown enzyme was found to be approximately equal to that of esterase 2.

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Zusammenfassung Ein italienischer OP-resistenter Musca domestica-Stamm erwies sich als heterogen für ein Gen im 5. Chromosom, das einen Unterschied in der Beweglichkeit einer Esterase bei der Elektrophorese bedingt. Individuen, die nur die Bande 1 oder 2 enthalten, sind homozygot für jeweils das eine der beiden Allele. Individuen, welche die Esterase 1 und 2 enthalten, sind heterozygot. Es wurden zwei Unterstämme E₁ und E₂ abgezweigt, die jeweils für das Allel 1 und 2 homozygot sind. Diese Stämme erwiesen sich als bemerkenswert verschieden hinsichtlich der OP-Resistenz. E₁ ist annähernd so resistent wie Stamm C und enthält das Abbau-Enzym, welches Paraoxon und Diazoxon zerstört. E₂ hat eine geringere Resistenz und enthält kein Abbau-Enzym. Die Gegenwart des Abbau-Enzyms und der 1-Esterase werden von dem gleichen Genallel kontrolliert, sind aber sicher nicht identisch. Z.B. ist Bande 1 ganz stabil und in normalen Homogenisaten in Lösung, während das Abbau-Enzym sehr labil und ungelöst ist. Deshalb kontrolliert das eine Allel, a _C1, sowohl Bande 1 und das Abbau-Enzym, das andere, a _C2, anscheinend nur Bande 2. Eine ähnliche Situation wurde in dem anfälligen Stamm, bwb; ocra, gefunden, der sich bereits früher als heterozygot für die Ali-Esterase a erwiesen hatte. Dabei sind 2 Allele des a-Gens vorhanden: das a ⁺-Allel kontrolliet die Anwesenheit von Bande 1 und Ali-Esterase a; das a ₂-Allel scheint nur Bande 2 zu kontrollieren. Die Elektrophorese-Geschwindigkeit des Abbau-Enzyms erwies sich als annähernd so groß wie die der Esterase 2.

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When the first author died in October 1964, he left the material for this publication. It is a tribute to his accuracy that it was possible for the last author to prepare this paper from his notes.     

Differentiation of Shigella strains by plasmid profile analysis, serotyping and phage typing

Ninety-one Shigella flexneri and 29 Shigella sonnei strains isolated during 1994 from sporadic cases of shigellosis and healthy carriers were analyzed for plasmid profile in order to compare the discriminating ability of this method with that of serotyping and phage typing. Our study revealed 10 plasmid profiles (PP) among S. sonnei strains. A total of 26 out of 29 (89%) S. sonnei isolates could be placed into two phage types (type 1 and 20) comprising four PP for phage type 1 and seven PP for type 20, respectively. Twenty-three different PP were identified among S. flexneri strains. Each serotype was associated with a specific predominant plasmid profile, except serotype 2a. This serotype, the most frequently isolated in Romania, was still rather homogeneous: 33 out of 39 isolates belonged to phage type 125, 27 of which could be placed into two related PP (F10 and F17). Comparison of plasmid patterns of epidemiologically independent S. flexneri serotype 2a isolates with those exhibited by 45 serotype 2a isolates associated to six independent outbreaks revealed the same homogeneity. Thirty-eight strains, representing 4 of 6 outbreaks, had F10 and F17 plasmid patterns. The discrimination indices (D) for plasmid profile analysis alone (D = 0.890) and for the combination of serotyping and phage typing (D = 0.841) indicate that both typing systems have a nearly similar ability of discriminating among S. flexneri strains. By combining the results of the three typing methods, a total of 42 types are distinguished and the D value is 0.942. Our data suggest that plasmid profile analysis can complement phenotyping methods resulting in a degree of discrimination that cannot be achieved by either system alone.     

Correlation between ribosomal DNA polymorphism and electrophoretic enzyme polymorphism in Yersinia

Ribosomal DNA (rDNA) polymorphism was compared with electrophoretic enzyme polymorphism for the intra- and interspecies differentiation of Yersinia enterocolitica, Y. pseudotuberculosis, Y. intermedia, Y. aldovae, Y. frederiksenii and Y. kristensenii. DNA from 90 strains previously classified into six zymotypes (Y. enterocolitica and Y. frederiksenii) and into distinct enzyme electrophoretic patterns (the four other species) was digested with EcoRI or HindIII and analysed by Southern blotting. The six species were clearly differentiated from each other. In Y. enterocolitica, the subclassification of biotype 1 into zymotypes 1A and 1B was also reflected in the rDNA and the four other bio-zymotypes gave four different classes of restriction pattern. In Y. frederiksenii, both EcoRI and HindIII gave five distinct riboclasses which correlated with the zymotypes. In the four other species, the phenotype polymorphism appeared to be better correlated with the restriction fragment length polymorphism data in some enzymes than others. The data demonstrate that the inter- and intraspecies classification by rDNA polymorphism using two restriction enzymes is similar to that based on electrophoretic enzyme polymorphism. The analysis could be refined for taxonomic and epidemiological purposes by using other restriction enzymes.     

The polymorphism of red cell esterase D in Italy

1,153 unrelated individuals from three different areas of Italy were tested for the red cell esterase D polymorphism. The gene frequencies found in the three groups do not differ significantly from each other. The EsD2 allele in the total sample has a frequency of 14.6% but it is difficult at the present stage to know if this figure is valid for the whole Italian population. If so, the Italian EsD2 allele frequency lies at the upper limit of the range of the European values. No variant phenotypes were observed.