On the influence of aggressive driving behavior on the dynamics of traffic flow

The car following model under discussion is a system of ordinary differential equations describing N cars moving around a circular road. We extend the stability analysis of the model in two directions: variable reaction time (depending on the headway) and an additional part describing the aggressive driving tendency. We study the global bifurcation dynamics and in particular its dependence on these two new ingredients. (© 2005 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim)     

The decay of 161Gd to 161Tb

The level scheme of ¹⁶¹Tb populated by the β-decay of 3.7 min ¹⁶¹Gd has been studied using Ge(Li) detectors as singles and coincidence γ-ray spectrometers. A total of 130 transitions has been observed. An investigation of the Coriolis coupling between the $\text{5}\text{2}{}^{\mathrm{?}}\text{[532↑]}\text{and}\text{7}\text{2}{}^{\mathrm{?}}\text{[523↑]}$ bands is presented. Rotational bands previously only observed in charged particle transfer work are discussed. Several additional levels are suggested.     

Mutation scanning analysis of sequence heterogeneity in the second internal transcribed spacer (rDNA) within some members of the Hypodontus macropi (Nematoda: Strongyloidea) complex

Single-strand conformation polymorphism analysis was employed to investigate sequence variation in the second internal transcribed spacer (ITS-2) of nuclear ribosomal DNA within and among individuals representing three operational taxonomic units (OTUs) of Hypodontus macropi from different species of Australian macropodid marsupials. Of the 96 nematodes analysed, totals of 3 (OTU1 from Petrogale persephone), 10 (OTU2 from Macropus robustus) and 7 (OTU9 from Macropus rufus) representative individuals were selected for DNA sequencing to characterise and estimate the magnitude of nucleotide variation in the ITS-2. While no unequivocal nucleotide difference in the ITS-2 was detectable within OTU1, most sequence variation (3/44.7%) detected within OTU2 and OTU9 was related chiefly to dinucleotide (CA, TA, or a combination of both) differences. This microsatellite variability in some H. macropi OTUs suggests that the ITS-2 rDNA may be subjected to slippage events during DNA replication, resulting in short dinucleotide repeat tracts being dispersed throughout the ITS-2 lineages, or possibly transposition and/or crossing-over events. Nucleotide variation in the ITS-2 of individual OTUs was related to the proposed secondary structure for the precursor ribosomal RNAs. Most of the sequence heterogeneity or polymorphism within OTU2 and OTU9 occurred in loops or bulges of the predicted secondary structure, which appear not to be under functional constraint. The findings of this study have implications for investigating speciation events and population differentiation in nematodes at the molecular level.     

Nonisotopic single-strand conformation polymorphism analysis of sequence variability in ribosomal DNA expansion segments within the genus Trichinella (Nematoda: Adenophorea)

A nonisotopic single-strand conformation polymorphism (SSCP) approach was employed to 'fingerprint' sequence variability in the expansion segment 5 (ES5) of domain IV and the D3 domain of nuclear ribosomal DNA within and/or among isolates and individual muscle (first-stage) larvae representing all currently recognized species/genotypes of Trichinella. In addition, phylogenetic analyses of the D3 sequence data set, employing three different tree-building algorithms, examined the relationships among all of them. These analyses showed strong support that the encapsulated species T. spiralis and T. nelsoni formed a group to the exclusion of the other encapsulated species T. britovi and its related genotypes Trichinella T8 and T9 and T. murrelli, and T. nativa and Trichinella T6, and strong support that T. nativa and Trichinella T6 grouped together. Also, these eight encapsulated members grouped to the exclusion of the nonencapsulated species T. papuae and T. zimbabwensis and the three representatives of T. pseudospiralis investigated. The findings showed that nonencapsulated species constitute a complex group which is distinct from the encapsulated species and supported the current hypothesis that encapsulated Trichinella group external to the nonencapsulated forms, in accordance with independent biological and biochemical data sets.     

Single-strand conformation polymorphism analysis of genetic variation in Labiostrongylus longispicularis from kangaroos

Single-strand conformation polymorphism (SSCP) analysis was employed to screen for sequence heterogeneity in the second internal transcribed spacer (ITS-2) of ribosomal (r) DNA of Labiostrongylus longispicularis, a parasitic strongylid nematode occuring in some species of kangaroo in different geographical regions of Australia. The results showed that most of the nematodes screened had different SSCP profiles, which were subsequently shown to correspond to polymorphisms and/or an indel in the ITS-2 sequence. These variable sites related mainly to unpaired regions of the predicted secondary structure of the precursor rRNA molecule. SSCP profiles could be used to distinguish L. longispicularis in Macropus robustus robustus (New South Wales) from L. longispicularis in Macropus robustus erubescens and Macropus rufus (South Australia). This difference corresponded to a transversional change in the ITS-2 sequence at alignment position 82. The study demonstrated clearly the effectiveness of SSCP analysis for future large-scale population genetic studies of L. longispicularis in order to test the hypothesis that L. longispicularis from different geographical regions represents multiple sibling species.     

Molecular epidemiological investigation of Ascaris genotypes in China based on single-strand conformation polymorphism analysis of ribosomal DNA

Using a single-strand conformation polymorphism-based approach, we investigated nucleotide variation in part of the first internal transcribed spacer (pITS-1) of nuclear ribosomal DNA within and among a large number of Ascaris individuals from humans and pigs from six endemic regions in China, and examined the frequency of the different genotypes of Ascaris in relation to host species and geographical origin. Five different SSCP genotypes (G1-G5) were recorded for human Ascaris (n = 486), of which three (genotypes G1-G3) were detected for pig Ascaris (n = 329). Of the five Ascaris genotypes detected, genotype G1 predominantly infected humans (approximately 63-74%) whereas genotype G3 infected mainly pigs (approximately 79-86%), indicating that each of these genotypes has a particular host affiliation. In contrast, the frequencies of the other three genotypes was substantially lower for each of the two host species. The findings also suggested that the rate of cross infection of Ascaris between humans and pigs is relatively low and that gene flow between the predominant genotypes is limited, consistent with previous proposals for endemic regions in other countries. While the nature and extent of nucleotide variation in the pITS-1 (and the proposal of host affiliated Ascaris populations) may relate to "introgression" or "lineage sorting and retention of ancentral polymorphism", other explanations are possible. Evidence of multiple pITS-1 sequence types in some Ascaris individuals representing particular genotypes (e.g., G2 and G5) may suggest hybridization between human- and pig-affiliated Ascaris. This aspect and the species status of Ascaris (from each host species) warrant future experimental testing, employing the pig/Ascaris model and the present electrophoretic approach.*     

Equilibrium and kinetics study of Gd(III) and U(VI) adsorption from aqueous solutions by modified Sorrel’s cement

Modified Sorrel’s cement was prepared by the addition of ferric chloride. The modified cement (MF5) was analyzed and characterized by different methods. Adsorption of Gd(III) and U(VI) ions in carbonate solution has been studied separately as a function of pH, contact time, adsorbent weight, carbonate concentration, concentration of Gd(III) and U(VI) and temperature. From equilibrium data obtained, the values of Δ H, Δ S and Δ G were found to equal −30.9 kJ ⋅ mol⁻¹, −85.4 J ⋅ mol⁻¹ ⋅,K⁻¹, and −5.4 KJ ⋅ mol⁻¹, respectively, for Gd(III) and 18.9 kJ ⋅ mol⁻¹, 67.8 J ⋅ mol⁻¹ K⁻¹ and −1.3 KJ ⋅ mol⁻¹, respectively, for U(VI). The equilibrium data obtained have been found to fit both Langmuir and Freundlich adsorption isotherms. The batch kinetic of Gd(III) and U(VI) on modified Sorrel’s cement (MF5) with the thermodynamic parameters from carbonate solution were studied to explain the mechanistic aspects of the adsorption process. Several kinetic models were used to test the experimental rate data and to examine the controlling mechanism of the adsorption process. Various parameters such as effective diffusion coefficient and activation energy of activation were evaluated. The adsorption of Gd(III) and U(VI) on the MF5 adsorbent follows first-order reversible kinetics. The forward and backward constants for adsorption, k ₁and k ₂ have been calculated at different temperatures between 10 and 60^∘C. Form kinetic study, the values of Δ H ^* and Δ S ^* were calculated for Gd(III) and U(VI) at 25^∘C. It is found that Δ H ^* equals −14.8 kJmol⁻¹ and 7.2 kJmol⁻¹ for Gd(III) and U(VI), respectively, while Δ S ^* were found equal −95.7 Jmol⁻¹K⁻¹ and −70.5 Jmol⁻¹K⁻¹ for Gd(III) and U(VI), respectively. The study showed that the pore diffusion is the rate limiting for Gd(III) and (VI).     

High-resolution electrophoretic procedures for the identification of five Eimeria species from chickens, and detection of population variation

To overcome limitations of conventional approaches for the identification of Eimeria species of chickens, we have established high resolution electrophoretic procedures using genetic markers in ribosomal DNA. The first and second internal transcribed spacer (ITS-1 and ITS-2) regions of ribosomal DNA were amplified by polymerase chain reaction (PCR) from genomic DNA samples representing five species of Eimeria (E. acervulina, E. brunetti, E. maxima, E. necatrix and E. tenella), denatured and then subjected to denaturing polyacrylamide gel electrophoresis (D-PAGE) or single-strand conformation polymorphism (SSCP) analysis. Differences in D-PAGE profiles for both the ITS-1 and ITS-2 fragments (combined with an apparent lack of variation within individual species) enabled the unequivocal identification of the five species, and SSCP allowed the detection of population variation between some isolates representing E. acervulina, which remained undetected by D-PAGE. The establishment of these approaches has important implications for controlling the purity of laboratory lines of Eimeria, for diagnosis and for studying the epidemiology of coccidiosis.