Neuronal response in nucleus reticularis thalami and neighboring thalamic structures to natural stimulation during chronic experiments on cats

Spike response was investigated in 104 neurons of the nucleus reticularis thalami (R) and adjoining thalamic nuclei to acoustic, tactile, and visual stimuli during chronic experiments on cats. Of the test neurons, 29% responded to acoustic stimulation and 11% showed no preference in relation to different acoustic stimuli. Minimum latencies of response to sounds measured 12–37 msec in excitatory and 18–27 msec in inhibitory cells. Duration of excitation produced by acoustic stimuli reached 50–250 msec; inhibition lasted 27–190 msec. Most cells belonging to this nucleus were excited by different stimuli; the proportion of inhibitory neurons did not exceed 4–10%.A. A. Bogomolets Institute of Physiology, Academy of Sciences of the Ukrainian SSR, Kiev. Translated from Neirofiziologiya, Vol. 21, No. 4, pp. 451–461, July–August, 1989.     

Macrobenthic community structure before, during, and after implementation of the Clean Water Act in the Neches River estuary (Texas)

Community structure of macrobenthos in the industrialized, tidal Neches River was studied 12 years after implementation of phase III of the Clean Water Act (CWA). Result were compared with a 1971–72 study conducted before implementation of the CWA and a 1984–85 study conducted after implementation of phases I & II of the CWA. The permitted BOD waste load decreased 93% between the 1971–72 and 1984–85 studies, then increased 19% between 1984–85 and the current study. A total of 50 taxa were collected during the 1971–72 study, 104 during the 1984–85 study, and 110 during the current study. Numbers of taxa per collection at each station increased by a factor of at least two between the 1971–72 and 1984–85 studies and were significantly different at the 0.0001 level. Numbers of taxa per collection at each station were not significantly different between the 1984–85 and the current study (p=0.286). Minimum collection densities in 1984–85 were higher than maximum densities in 1971–72 and were significantly different at the 0.0001 level. Collection densities were not significantly different between the 1984–85 study and the current study (p=0.374). Shannon's annual and station collection diversity values significantly increased (p=<0.05) between the 1971–72 and 1984–85 studies, but not between the 1984–85 and the current study (p=>0.05). Dendrograms of Sorenson's similarity index between all pairs of stations were more alike between the 1971–72 and the current study than between the 1984–85 and the current study. Evidence of some organic enrichment at the upper stations was indicated by the dominance of Limnodrilus hoffmeisteri and depressed oxygen concentrations. Environmental quality in the river has greatly improved since implementation of the CWA in 1972. Most of the improvments were due to phases I & II of the CWA, with little apparent change since implementation of phase III.     

Control of the production of individual fusicoccins at different dissolved oxygen concentrations

The regulatory effect of different concentrations of dissolved oxygen on the production of fusicoccins by the fungus Fusicoccum amygdali Del. was studied. The maximum output of total fusicoccins was obtained by using a profiled dissolved oxygen tension (DOT) regime, in which the DOT was maintained at 15–20% during the biomass growth phase and at 5–8% during the fusicoccins production phase. In comparison with the profiled regime, the maintenance of DOT at 15–20% during the whole fermentation shortened the fusicoccins production phase. The fermentation performance at a low DOT (5–8%) inhibited both the accumulation of biomass and the production of fusicoccins. At high DOT (40–50%), an accelerated accumulation of the biomass with an expressed autolysis of mycelia took place, and the production of fusicoccins was lowered. The qualitative composition of individual fusicoccins varied substantially at different DOTs. Fusicoccins, A, C, D, J, H, 16-O-demethyl-J, detretpentenylfusicoccin and some minor fusicoccin metabolites were found in the fermentation broth using the method of liquid secondary ion mass spectrometry. It was established that the profiled DOT regime (15–20% to 5–8%) provided both the maximum concentration of fusicoccins and an enhanced accumulation of the main metabolite – fusicoccin A (FC A). The performance of the fermentation at a DOT of 15–20% decreased the content of FC A by 2–6% in comparison with the profiled DOT regime, and increased the content of fusicoccin C to 14–20% of the total fusicoccins. Fermentation at DOT of 5–8% was characterized by the highest content of the precursors of FC A, the less oxidized fusicoccins H and J, the contents of which were in range 7–12% and 16–17% of total fusicoccins, respectively.     

Unit responses in the anterior zone of the suprasylvian gyrus to peripheral stimuli of different modalities

Unit responses in the anterior zone of the suprasylvian gyrus to visual, electrodermal, and acoustic stimulation were investigated in experiments on unanesthetized cats immobilized with tubocurarine. Electrical activity was recorded from 131 units, 121 of which were spontaneously active. In 65.5% of cells responses consisted of a short or long increase or a decrease in intensity of spike activity. Most cells (58.2%) were monosensory. Responses to visual stimulation were given by 72% of neurons, to electrodermal by 61.6%, and to acoustic by 9.3%. The corresponding latent periods were 20–40, 20–30, and 15–20 msec. Responses of the same neurons to different peripheral stimuli were uniform or they differed in their dynamics. Intracellular recording gave responses in the form of EPSPs (amplitude 4–5 mV, duration 60–80 msec) or, rarely, IPSPs (amplitude 2–3 mV, duration 160–200 msec). The functional organization of the associative cortex and mechanisms of analysis of incoming afferent information are discussed.A. A. Bogomolets Institute of Physiology, Academy of Sciences of the Ukrainian SSR, Kiev. Translated from Neirofiziologiya, Vol. 4, No. 4, pp. 368–374, July–August, 1972.     

Growth and age structure of the swan mussel Anodonta cygnea (L.) at different depths in lake Mattsee (Salzburg, Austria)

Unionid clams were collected at 1–2 m, 3–4 m and 6–7 m depth in lake Mattsee, a moderately mesotrophic lake, to investigate the effect of depth on clam growth and age structure. No significant differences in age structure of Anodonta cygnea were found (p=0.65). Three and ten years old clams were present at all depths, but in different percentages. Whereas at 1–2 m 13.3% of the collected clams were <4 years old, this percentage was 4.4% at 6–7 m and 7.1% at 3–4 m. A greater percentage (6.7%) of older mussels (9, 10 years) were collected at 6–7 m than at 1–2 m (2.2%). Growth declined with depth. Total length at a given age of clams at 1–2 m and 3–4 m did not differ (p=0.54), whereas differences were significant between clams at 1–2 m and 6–7 m (p<0.05) as well as between 3–4 m and 6–7 m (p<0.05). The Growth constant k was highest at 1–2 m depth.     

Determination of zearalenone and its metabolites α- and β-zearalenol in beer samples by high-performance liquid chromatography–tandem mass spectrometry

A fast, robust and sensitive LC–MS–MS method for the determination of zearalenone (ZON) and its metabolites α-zearalenol (α-ZOL) and β-zearalenol (β-ZOL) in beer samples is described. Sample preparation was performed by direct RP-18 solid-phase extraction of undiluted beer samples followed by selective determination of analytes by LC–MS–MS applying an atmospheric pressure chemical ionization (APCI) interface. Using the negative ion mode limits of determination of 0.03–0.06 μg l⁻¹ beer and limits of quantification of 0.07–0.15 μg l⁻¹ beer were achieved, which was distinctly more sensitive than in the positive ion mode. Twenty-three beer samples from different countries, produced from different grains and under different brewing conditions, were investigated by this method, but only in one sample could β-ZOL and ZON be detected. Independently of the type of beer, relative standard deviations between 2.1% and 3.3%, a linear working range of 0.15 μg l⁻¹ to 500 μg l⁻¹ beer and recovery rates around 100% could be achieved when zearalanone (ZAN) was used as internal standard.     

Development of genetic markers in cyanobacteria and stability of genetically marked strains in soil

Reporter marker GUS (-glucuronidase gene from Escherichia coli) and luc operon from the American firefly were introduced into cyanobacteria and the stability of these markers in soil was examined. To transfer the integrational vector into cyanobacteria, the genomic DNA library of Synechocystis sp. or Anabaena cylindrica maintained in pBR 322, pCY 100 and pCY 101 were transformed with HB 101 containing pRL 528 and selected for Cm^r and Amp^r. These clones of HB 101 containing pRL 528 and the vectors carrying different cyanobacterial chromosomal DNA fragments were used for triparental mating with HB 101 [pRK 2013/pRK 2073] and cyanobacteria. The frequency of transconjugants for integrational vectors was between 2.1 × 10^–5 and 4.0 × 10^–4. The transfer frequency of RSF 1010 based vectors (pDSK 519 and pCY 106) was 1.0–4.5 × 10^–4 in Synechocystis sp. whereas A. cylindrica failed to maintain these vectors. Low frequency transfer (2.0–2.3 × 10^–6) of RK 2 based vectors pVK 100 and pCY 104 was observed in A. cylindrica but these were unable to replicate in Synechocystis sp. The vectors in general were stable at least by 74.9% for 60 days of incubation in BG-11 medium. The markers were less stable in A. cylindrica (74.9–84.2%) compared to Synechocystis sp. (80.1–88.8%) at 60 days of incubation. Integrational vectors were almost 85% stable in both the strains. The RK 2 derivative of pCY 104 was less stable in A. cylindrica (74.9–77.3%) than the RSF 1010-based vector pCY 106 in Synechocystis sp. (80.1–81.0%). A maximum of 64.7% of the markers were lost in soil. The chromosomal markers through integrational vectors were found to be highly stable and 68.2–72.7% of these markers were retained in cyanobacteria at 60 days of incubation. Plasmid markers were less stable, with a loss of 64.7–48.7% at the end of the experiment. In A. cylindrica 58–65% of the RK 2 vector was lost whereas in Synechocystis sp. 49–61% of RSF 1010 was lost at 60 days of incubation.     

Neuronal composition and interneuronal connection of area 5 in the cat parietal association cortex

Area 5 of the cat cortex was studied by Nissl's method and by Golgi's chromate-silver impregnation method. Its typical six-layered structure with well-developed layers of pyramidal cells was revealed. The characteristic features of area 5 are: predominance of pyramidal cells in layers II–III and the presence of large forms (40×26 µ) among them (in layer III); giant pyramidal neurons (70×23 µ) arranged singly or nidally in layer V; large (diameter 25–30 µ) and giant (diameter 40–45 µ) stellate cells with radial dendrites, arranged singly or in groups in layers V–VI; infrequent efferent fusiform neurons (40×20 µ) in layers V–VI. Stellate cells connecting pyramidal neurons in the same or in different layers were found in layers II–VI. Some stellate cells in layers II–III form long horizontal connections within area 5. Interneuronal connections are effected by axosomatic and axodendritic terminals, the latter being more numerous; Dendrodendritic and axoaxonal synapses are less common.A. A. Bogomolets Institute of Physiology, Academy of Sciences of the Ukrainian SSR, Kiev. Translated from Neirofiziologiya, Vol. 11, No. 1, pp. 35–42, January–February, 1979.     

Tetraploid-octoploid relationships and karyological evolution in the order Acipenseriformes (Pisces) karyotypes,nucleoli, and nucleolus-organizer regions in four acipenserid species

The karyotypes of four Acipenseriformes species, Acipenser gueldenstaedti, 2n=250±8, A. ruthenus, A. stellatus and Huso huso, 2n=118±2, are described. In all four karyotypes the majority of chromosomes are meta- and submetacentric macrochromosomes, and microchromosomes of different morphology make up about one third of the set. In A. ruthenus the NORs are located in the telomeric region of a pair of microchromosomes and at least in one pair of middle-size acrocentrics, and in A. stellatus and Huso huso also in the telomeric regions of at least one pair of microchromosomes. The modal number of active nucleoli in A. gueldenstaedti nuclei amounts to 6–8 (range 2–12), in A. ruthenus, A. stellatus and H. huso nuclei to 2–3 (range 1–6). The data obtained point to the tetraploid origin of Acipenseriformes species with 120 chromosomes and to the octoploid origin of species with 240–260 chromosomes.     

Vascular expression of the grp1.8 promoter is controlled by three specific regulatory elements and one unspecific activating sequence

The bean grp1.8 full-length promoter is specifically active in vascular tissue during normal development of tobacco. Deletion of a negative regulatory element resulted in ectopic activity of the promoter in cortical cells of hypocotyls, roots and stems. A 169 bp fragment (–205 to –36) of the grp1.8 promoter conferred vascular-specific expression to CaMV 35S minimal promoters whereas a 141 bp fragment (–205 to –64) strongly activated these minimal promoters both in vascular and cortical cells. These experiments defined a new regulatory element (VSE) that is essential for vascular-specific expression and is located between –64 and –36. The 141 bp grp1.8 promoter sequence had enhancer-like properties as it was active in both orientations. A 24 bp sequence (bp –119 to –96, corresponding to the SE1 regulatory element) enhanced expression from several minimal promoters strongly but unspecifically, whereas a 26 bp sequence (–98 to –73, corresponding to the RSE regulatory element) induced vascular-specific expression. Thus, the grp1.8 promoter is regulated by a combinatorial mechanism that can integrate the action of different, non-additively acting regulatory elements into vascular-specific expression.     

Widespread occurrence of ATP:citrate lyase and carnitine acetyltransferase in filamentous fungi

Ten filamentous fungi, belonging to five different genera of both higher and lower fungi, including oleaginous fungi and fungi known to produce secondary metabolites, all possessed both ATP:citrate lyase (17–84nmol min–1 (mg protein)–1) and carnitine acetyltransferase activity (9–62nmol min–1 (mg protein)–1). The possession of these two enzymes appears to be a common feature in filamentous fungi.     

Genetic Analysis of the Epidermal Differentiation Complex (EDC) on Human Chromosome 1q21: Chromosomal Orientation, New Markers, and a 6-Mb YAC Contig

The epidermal differentiation complex (EDC) unites a remarkable number of structurally, functionally, and evolutionarily related genes that play an important role in terminal differentiation of the human epidermis. It is localized within 2.05 Mb of region q21 on human chromosome 1. We have identified and characterized 24 yeast artificial chromosome (YAC) clones by mapping individual EDC genes, sequence-tagged site (STS) markers (D1S305, D1S442, D1S498, D1S1664), and 10 new region-specific probes (D1S3619–D1S3628). Here we present a contig that covers about 6 Mb of 1q21 including the entire EDC. Fluorescencein situhybridization on metaphase chromosomes with two YACs flanking the EDC determined its chromosomal orientation and established, in conjunction with physical mapping results, the following order of genes and STSs: 1cen–D1S442–D1S498–S100A10–THH–FLG–D1S1664–IVL–SPRR3–SPRR1–SPRR2–LOR–S100A9–S100A8–S100A7–S100A6–S100A5–S100A4–S100A3–S100A2–S100A1–D1S305–1qtel. These integrated physical, cytogenetic, and genetic mapping data will be useful for linkage analyses of diseases associated with region 1q21 and for the identification of novel genes and regulatory elements in the EDC.     

Effects of experimentally induced deficiency of catecholaminergic transmission on neuronal activity in the ventrolateral thalamic nucleus

Background activity was investigated in 272 neurons of the ventrolateral thalamic nucleus (VLTN) before and after systemic administration of neuroleptics (haloperidol and droperidol) at cataleptic doses by means of extracellular techniques during chronic experiments on cats. Autocorrelation and spectral analysis revealed regularly-occurring changes in the background activity rate of VLTN neurons, the periodicity of which changed by fractions of seconds (0.2–0.8 sec), seconds (1.5–10 sec), or tens of seconds (12–30 sec). While numbers of neurons with individual types of periodic activity did not exceed 6–8% in intact animals, it did increase to 18–30% after administering neuroleptics. Raised numbers of neurons with two types of regularly occurring processes within a single spike train were also noted. Experimentally-produced data were compared with findings from clinical observations. Quantities of neurons with different variations in the periodicity of their firing activity reached 19–46% in patients with parkinsonism but did not exceed 4–8% in those with torsion dystonia. The genesis of raised rhythmic firing in thalamic neurons occurring with parkinsonism is thought to be associated with impaired catecholaminergic (both dopaminergic and -adrenergic) transmission.A. A. Bogomolets Institute of Physiology, Academy of Sciences of the Ukrainian SSR, Kiev. Translated from Neirofiziologiya, Vol. 22, No. 3, pp. 359–368, May–June, 1990.     

Long-Term Effects of Elevated CO2 on Woody Tissues Respiration of Norway Spruce Studied in Open-Top Chambers

In an open-top chamber experiment located in a mountain stand of 14-years-old Norway spruce (Picea abies [L.] Karst.), trees were continuously exposed to either ambient CO₂ concentration (A), or ambient + 350 µmol mol^–1 (E) over four growing seasons. Respiration rates of different woody parts (stem, branches, coarse roots) were measured during the last growing season. The calculated increase in the respiration rate related to a 10 °C temperature change (Q₁₀) was different in stem compared to branches and roots. Differences between the E and A variants were statistically significant only for roots in the autumn. Stem maintenance respiration (R_Ms) measured in April and November (periods of no growth activity) were not different. The stem respiration values (R_s) were recalculated to a standard temperature of 15 °C to estimate the seasonal course. The obtained R_s differed significantly between used variants during July and August. At the end of the season, R_s in E decreased slower than in A, indicating some prolongation of the physiological activity under the elevated CO₂ concentration. The total stem respiration carbon losses for the investigated growing season (May – September) were higher for A (2.32 kg(C) m^–2 season^–1) compared to E (2.12 kg(C) m^–2 season^–1). The respiration rates of the whorl branches (R_b) were lower compared with the stem respiration but not significantly different between the used variants. The root respiration rate was increased in E variant.     

Determination of disulfide bond arrangement in bombyxin-IV, an insulin superfamily peptide from the silkworm,Bombyx mori, by combination of thermolysin digestion of natural peptide and selective synthesis of disulfide bond isomers

The mode of disulfide linkages in bombyxin-IV, an insulin superfamily peptide consisting of A- and B-chains, was determined as A6–A11, A7–B10, and A20–B22. An intermolecular bond of A20–B22 was identified by sequencing and mass spectrometric analysis of the fragments generated by thermolysin digestion of natural bombyxin-IV. The mode of the remaining two bridges was determined by chemical and selective synthesis of three possible disulfide bond isomers of bombyxin-IV. A- and B-chains were synthesized by solid-phase method, and three disulfide bonds were bridged stepwise and in a fully controlled manner. Retention time on reversed-phase high-performance liquid chromatography (HPLC), thermolysin digests, and biological activity of the synthetic [A6–A11, A7–B10, A20–B22-cystine]-bombyxin-IV revealed that it was identical with the natural bombyxin-IV. Two other isomers with respect to disulfide bond arrangement, [A6–A7, A11–B10, A20–B22-cystine]- and [A6–B10, A7–A11, A20–B22-cystine]-bombyxin-IVs, were distinguishable from the natural one by use of HPLC, thermolysin digestion, and bioassay.     

Pigment estimations and photosynthesis of Ruppia drepanensis Tin. ex Guss. in a hypersaline environment

We collected the ephemeral macrophyte Ruppia drepanensis Tin. ex Guss. from the athalassic shallow lake Fuente de Piedra (Málaga. Southern Spain). This lake, situated in an endorheic basin, shows great seasonal changes in depth and Total Dissolved Solids (TDS).Dissolved oxygen evolution studied in the laboratory at 17 different photon flux densities (PFD) showed a maximum rate of photosynthesis of 0.55 mg C g dry wt^–1 h^–1, a light compensation point at 86 µE m^–2 s^–1 and a saturation point at 333 µE m^–2 s^–1. A moderate photoinhibition (\ = 1.68 10^–4) was found above 695 µE m^–2 s^–1.Estimates of pigment concentrations revealed 10 times more carotenoids than chlorophyll.The adaptation of the plants to high irradiances and to the particular features of their hypersaline environment are discussed.     

A scrutiny of the biochemical pathways from Ang II to Ang-(3–4) in renal basolateral membranes

In a previous paper we demonstrated that Ang-(3–4) counteracts inhibition of the Ca²⁺-ATPase by Ang II in the basolateral membranes of kidney proximal tubules cells (BLM). We have now investigated the enzymatic routs by which Ang II is converted to Ang-(3–4). Membrane-bound angiotensin converting enzyme, aminopeptidases and neprilysin were identified using fluorescent substrates. HPLC showed that Plummer's inhibitor but not Z–pro–prolinal blocks Ang II metabolism, suggesting that carboxypeptidase N catalyzes the conversion Ang II→ Ang-(1–7). Different combinations of bestatin, thiorphan, Plummer's inhibitor, Ang II and Ang-(1–5), and use of short proteolysis times, indicate that Ang-(1–7)→ Ang-(1–5)→ Ang-(1–4)→ Ang-(3–4) is a major route. When Ang III was combined with the same inhibitors, the following pathway was demonstrated: Ang III→ Ang IV→ Ang-(3–4). Ca²⁺-ATPase assays with different Ang II concentrations and different peptidase inhibitors confirm the existence of these pathways in BLM and show that a prolyl-carboxypeptidase may be an alternative catalyst for converting Ang II to Ang-(1–7). Overall, we demonstrated that BLM have all the peptidase machinery required to produce Ang-(3–4) in the vicinity of the Ca²⁺-ATPase, enabling a local RAS axis to effect rapid modulation of active Ca²⁺ fluxes.     

Inhibitory effects of GABA on synaptic excitation in isolated rat hippocampal slices

In research on -aminobutyric acid (GABA) used at different concentrations on the amplitude of EPSP within populations (PEPSP), as recorded from dentrites in isolated hippocampal slices, GABA induced a dose-dependent reversible reduction in PEPSP amplitude with no noticeable signs of desensitization. Highest sensitivity to GABA was shown by PEPSP in hippocampal zone CA1 (threshold concentration: 3×10^–5–2×10^–4 M; (concentration at which the effect equal to 1/2 of maximum occurs) IC₅₀: 5×10^–4–1×10^–3 M). The effects of GABA on PEPSP were not blocked by bicuculline, picrotoxin, or penicillin. Action of GABA on dendritic antidromic population spike (DAPS — postynaptic effects) were slightly diminished by these blockers. Baclofen inhibited PEPSP more powerfully than GABA (threshold concentration: 1×10^–6 M: IC₅₀: 3×10^–6 M), although it only produced a minor reduction in DAPS amplitude even at high concentrations. It is concluded that the inhibitory effect of GABA on PEPSP in hippocampal zone CA1 may be put down mainly to its presynaptic action mediated by GABA_B receptors on axonal terminals of Schaffer collaterals.A. A. Bogomolets Institute of Physiology, Academy of Sciences of the Ukrainian SSR, Kiev. Translated from Neirofiziologiya, Vol. 22, No. 5, pp. 627–633, September–October, 1990.     

Bioturbation experiments in the Venice Lagoon

Short experiments (14–21 days) were carried out during autumn 1998 and spring 1999 at one selected site of the Venice Lagoon to measure bioturbation activities and mixing rates, as well as to obtain quantitative information on benthos functionality. Fluorescent sediment particles (luminophores, 63–350 m) were introduced as pulse inputs at the sediment surface. The concentration–depth profiles of the tracer were simulated with a new advection–diffusion–non local model applied under non-steady state conditions. This allowed the quantification of the mixing parameters associated with different mechanisms: biodiffusion (D _b), bioadvection (W) and non-local mixing (Ke, z₁, z₂). A parameter RS (removed sediment) was also calculated to account for the flux of sediment due to non-local transport. Results show that bioturbation was dominated by biodiffusion in autumn and by bioadvection in spring. Mean mixing parameters Db, W, and RS changed from 3.09 to 0.87 cm² y^–1, from 0.93 to 15.50 y^–1 and from 5.85 to 7.79 g cm^–2 y^–1, respectively.