The effect of copper on osmoregulation in the freshwater amphipod Gammarus pulex

The influence of copper on osmoregulation in the freshwater amphipod Gammarus pulex was determined from the analysis of water permeability, haemolymph sodium concentration, sodium influx and gill Na(+)/K(+) ATPase and Mg(2+) ATPase activity. Exposure to nominal copper concentrations of 100 microg l(-1) or greater caused a significant reduction in both haemolymph sodium concentration and sodium influx within 4 h. Measurements of water permeability, expressed as the half-time of exchange of body water (t(1/2)), excluded structural gill damage as the cause of this fall in haemolymph sodium. Copper at 10 microg l(-1) or above in the assay solution significantly reduced gill Na(+)/K(+) ATPase activity. In contrast gill Mg(2+) ATPase activity was markedly less affected by copper. These differences in enzyme sensitivity were considered with respect to the potential mechanisms of copper toxicity.     

Function and solution structure of hainantoxin-I, a novel insect sodium channel inhibitor from the Chinese bird spider Selenocosmia hainana

Hainantoxin-I is a novel peptide toxin, purified from the venom of the Chinese bird spider Selenocosmia hainana (=Ornithoctonus hainana). It includes 33 amino acid residues with a disulfide linkage of I-IV, II-V and III-VI, assigned by partial reduction and sequence analysis. Under two-electrode voltage-clamp conditions, hainantoxin-I can block rNa(v)1.2/beta(1) and the insect sodium channel para/tipE expressed in Xenopus laevis oocytes with IC(50) values of 68+/-6 microM and 4.3+/-0.3 microM respectively. The three-dimensional solution structure of hainantoxin-I belongs to the inhibitor cystine knot structural family determined by two-dimensional (1)H nuclear magnetic resonance techniques. Structural comparison of hainantoxin-I with those of other toxins suggests that the combination of the charged residues and a vicinal hydrophobic patch should be responsible for ligand binding. This is the first report of an insect sodium channel blocker from spider venom and it provides useful information for the structure-function relationship studies of insect sodium channels.     

Activity and NMR structure of synthetic peptides of the bovine ATPase inhibitor protein,IF1

The protein IF₁ is a natural inhibitor of the mitochondrial F_oF₁-ATPase. Many investigators have been prompted to identify the shortest segment of IF₁, retaining its native activity, for use in biomedical applications. Here, the activity of the synthetic peptides IF₁-(42–58) and IF₁-(22–46) is correlated to their structure and conformational plasticity determined by CD and [¹H]-NMR spectroscopy. Among all the IF₁ segments tested, IF₁-(42–58) exerts the most potent, pH and temperature dependent activity on the F_oF₁ complex. The results suggest that, due to its flexible structure, it can fold in helical and/or β-spiral arrangements that favor the binding to the F_oF₁ complex, where the native IF₁ binds. IF₁-(22–46), instead, as it adopts a rigid -helical conformation, it inhibits ATP hydrolysis only in the soluble F₁ moiety.     

Synthesis of sodium 2,6-dimesitylphenyl phosphanide and X-ray crystal structure determination of its 15-crown-5 adduct

The synthesis of the first terphenyl-based sodium phosphanide, namely DmpP(H)Na (1) (Dmp=2,6-dimesitylphenyl) as well as the X-ray crystal structure determination of a crown ether adduct of the sodium salt, namely DmpP(H)Na(15-crown-5) (2) are reported. Compound 2 crystallizes in the triclinic space group P1?. Crystal data for 2 at 198 K: a=10.5342(4) Å; b=12.0538(5) Å; c=14.4023(6) Å; α=79.9474(9)°; β=72.2234(10)°; γ=70.0716(10)°; V=1632.1(2) ų; Z=2; D_calc=1.198 g cm⁻³; R_F=7.91%. The molecular structure of 2 features a monomeric arrangement in the solid state and a bent NaPC(ipso) moiety [Na(1)P(1)C(16)=116.3(2)°].     

Fluorescent proteins in animal cells for process development: optimization of sodium butyrate treatment as an example.

Fluorescent proteins expressed in mammalian cells can be quantified quickly and noninvasively with a standard fluorescence plate reader. We have previously exploited this quality in cell growth assessment (Hunt et al., 1999b). In this work, different CHO cell lines constitutively expressing fluorescent proteins were evaluated as model systems for process development and optimization. Our results demonstrate that the fluorescence of these cell lines quickly reveals conditions that might improve the overall productivity. Sodium butyrate, a well-known yet unpredictable enhancer of production, was chosen for this study. Due to the competing effects of sodium butyrate ("butyrate") on expression and cell number, the maximal overall productivity represents a compromise between enhancement of production and toxicity. Based on fluorescence only, it is possible to separate effects on cell number and specific production by combining microplate fluorescence measurements with data obtained by flow cytometry. This allows for rapid screening of different clones without counting cells or quantifying the recombinant protein, a highly attractive feature if the expression of green fluorescent protein (GFP) was correlated to that of a protein of interest. For all clones tested, negative effects of butyrate on proliferation were similar, while net enhancement of expression was characteristic for each clone. Therefore, it is necessary to optimize treatment for each individual clone. This work demonstrates that, based on the fluorescence of GFP-expresssing cell lines, it is possible to examine noninvasively three critical, generic parameters of butyrate treatment: butyrate concentration, exposure time, and culture phase at the time of addition.     

Influence of sodium dodecyl sulfate/TritonX-100 micelles on the oxidation of D-fructose by chromic acid in presence of HClO(4)

The kinetics of oxidation of D-fructose by chromic acid in aqueous and aqueous surfactant (sodium dodecyl sulfate, SDS, and alkylphenyl polyethylenglykol, TX-100) media have been investigated in the presence of HClO(4). The reaction is acid catalyzed and is associated with an induction period which is dependent on [H(+)], [surfactant] and temperature. The order of oxidation during induction under [D-fructose]>[chromic acid] conditions is fractional in each reagent in both media. The rate constant was found to increase with [Mn(II)]. A mechanism has been proposed for the reaction. The micelles produce a catalytic effect in the range of SDS and TX-100 concentrations used, and the effect is explained by means of the pseudo-phase mass-action model. In the presence of SDS, the reaction is inhibited by electrolytes (NH(4)Br, NaBr, LiBr), and the inhibition order Na(+)>Li(+)>NH(4)(+) is explained on the basis of electrostatic considerations. The rate constant (k(m)), binding constants (K(S) and K(F)), and corresponding activation parameters (E(a), delta H( not equal ) and delta S( not equal )) have been evaluated and discussed. The order of reactivities of different sugars is found as: D-fructose>D-arabinose>D-xylose approximately D-glucose.     

Conformational equilibria and dynamics of cytochrome<Emphasis Type="Italic"> c</Emphasis> induced by binding of sodium dodecyl sulfate monomers and micelles

Circular dichroism, nuclear magnetic resonance, electron paramagnetic resonance, UV-vis absorption, and resonance Raman (RR) spectroscopic techniques were employed to study protein and heme structural changes of cytochrome c (Cyt-c) induced by sodium dodecyl sulfate (SDS) monomers and micelles via hydrophobic and electrostatic interactions, respectively. Both modes of interactions cause the transition to the conformational state B2, which is implicated to be involved in the physiological processes of Cyt-c. At sub-micellar concentrations of SDS, specific binding of only ca. three SDS monomers, which is likely to occur at the hydrophobic peptide segment 81–85, is sufficient for a complete conversion to a B2 state in which Met80 is replaced by His33 (His26). These heme pocket structural changes are not linked to secondary structure changes of the protein brought about by nonspecific binding of SDS monomers in different regions of the protein. Upon binding of micelles, B2 high-spin species can also be stabilized by electrostatic interactions. In addition, the micelle interaction domain is located on the front surface of Cyt-c, which includes a ring-like arrangement of lysine residues appropriate for binding one micelle. According to freeze-quench RR and stopped-flow experiments, state B2 is formed on the long millisecond timescale and reveals a complex dependence on the SDS concentration that can be interpreted in terms of competitive binding of monomers and micelles.     

Dynamic compartmentalization of the voltage-gated sodium channels in axons

One of the major physiological roles of the neuronal voltage-gated sodium channel is to generate action potentials at the axon hillock/initial segment and to ensure propagation along myelinated or unmyelinated fibers to nerve terminal. These processes require a precise distribution of sodium channels accumulated at high density in discrete subdomains of the nerve membrane. In neurons, information relevant to ion channel trafficking and compartmentalization into sub-domains of the plasma membrane is far from being elucidated. Besides, whereas information on dendritic targeting is beginning to emerge, less is known about the mechanisms leading to the polarized distribution of proteins in axon. To obtain a better understanding of how neurons selectively target sodium channels to discrete subdomains of the nerve, we addressed the question as to whether any of the large intracellular regions of Nav1.2 contain axonal sorting and/or clustering signals. We first obtained evidence showing that addition of the cytoplasmic carboxy-terminal region of Nav1.2 restricted the distribution of a dendritic-axonal reporter protein to axons of hippocampal neurons. The analysis of mutants revealed that a di-leucine-based motif mediates chimera compartmentalization in axons and its elimination in soma and dendrites by endocytosis. The analysis of the others generated chimeras showed that the determinant conferring sodium channel clustering at the axonal initial segment is contained within the cytoplasmic loop connecting domains II-III of Nav1.2. Expression of a soluble Nav1.2 II-III linker protein led to the disorganization of endogenous sodium channels. The motif was sufficient to redirect a somatodendritic potassium channel to the axonal initial segment, a process involving association with ankyrin G. Thus, it is conceivable that concerted action of the two determinants is required for sodium channel compartmentalization in axons.