Rapid,sensitive and specific electron capture—gas chromatographic method for the quantitation of 6-chloro-2-(1-piperazinyl)pyrazine in biological fluids

A highly specific and sensitive gas chromatographic method for the determination of 6-chloro-2-(1-piperazinyl)pyrazine (MK-212), a central serotonin-like agent, in biological fluids is described. MK-212 and a related internal standard are extracted into benzene from an alkaline solution, back-extracted into acid and then re-extracted into benzene at an alkaline pH. The amines are converted to the trifluoroacetyl derivatives (characterized by gas—liquid chromatography—mass spectrometry), chromatographed and detected with a ⁶³Ni electron capture detector. The sensitivity of the method is such that 10 ng of drug can be measured per aliquot of biological fluid. The precision and accuracy of the method are well within acceptable limits. Specificity of analysis was established by gas—liquid chromatography—mass spectrometry techniques.     

New insights into the membrane-binding and activation mechanism of pyruvate oxidase from Escherichia coli

Pyruvate oxidase from Escherichia coli (EcPOX) is a thiamin diphosphate- (ThDP) and FAD-dependent peripheral membrane protein that carries out the irreversible oxidative decarboxylation of pyruvate to acetate and carbon dioxide. Concomitant two-electron reduction of the flavin cofactor was suggested to induce a structural rearrangement of the C-terminus triggering recruitment of the protein from the cytosol to the cell membrane, where the electrons are eventually transferred to final electron acceptor ubiquinone 8. Binding to the membrane, or alternatively, mild proteolytic digestion leads to a multifold enhancement of both the catalytic activity and substrate affinity. Recent X-ray crystallographic studies on EcPOX in the resting state and on a C-terminal truncation variant mimicking the membrane-bound activated form have fueled our understanding of the membrane-binding mechanism and concomitant catalytic activation. In the resting state, the auto-inhibitory C-terminal membrane anchor adopts a half-barrel/helix fold that occludes the active site. Upon activation, the C-terminus is expelled and becomes structurally flexible thereby freeing the active site. Circular dichroism spectroscopic analysis revealed the isolated C-terminus to be disordered, however, formation of a helical structure was observed in the presence of micelles. Limited proteolysis experiments indicate that activation of EcPOX involves at least two sequential structural transitions: the first occurring after binding of pyruvate to ThDP and the second after two-electron reduction of the flavin.     

Demonstration of a retino-thalamo-hippocampal pathway in the rat

Investigations using double labeling by axonal transport of tracers have shown that in the rat, four nuclei of the anterior thalamus (anterior dorsal, anterior ventral, lateral anterior, bed nucleus of the stria terminalis) that project to the CA1 region of the hippocampus also receive a discrete input from the contralateral eye. The significance of this telencephalic visual pathway is discussed in a phylogenetic context.     

Tyrosine kinase receptors in the control of epithelial growth and morphogenesis during development

The c-ros, c-met and c-neu genes encode receptor-type tyrosine kinases and were originally identified because of their oncogenic potential. However, recent progress in the analysis of these receptors and their respective ligands indicate that they do not mediate exclusively mitogenic signals. Rather, they can induce cell movement, differentiation or morphogenesis of epithelial cells in culture. Interestingly, the discussed receptors are expressed in embryonal epithelia, whereas direct and indirect evidence shows that the corresponding ligands are produced in mesenchymal cells. In development, signals given by mesenchymal cells are major driving forces for differentiation and morphogenesis of epithelia; embryonal epithelia are generally unable to differentiate without the appropriate mesenchymal factors. The observed activities of these receptor/ligand systems in cultured cells and their expression patterns indicate that they regulate epithelial differentiation and morphogenesis also during embryogenesis and suggest thus a molecular basis for mesenchymal epithelial interactions.     

Importance of cytomatrix-bound polysomes to synthesis of lysine-containing proteins in triticale germs under ABA treatment

The influence of exogenous abscisic acid (ABA) on the content of free polysomes (FP), membrane-bound polysomes (MBP), cytoskeleton-bound polysomes (CBP) and cytomatrix-bound polysomes (CMBP) in triticale germs as well as in vitro protein synthesis by these four polysomal fractions were studied. During translation, proteins were biotinylated for chemiluminescence detection. We have found that ABA changed both the content of FP, MBP, CMP and CMBP in germ tissue, and their subsequent translation activity. At 100 μM ABA, the content of FP and MBP was over fourfold lower compared to the control, whereas the amounts of CBP and CMBP were about two- and threefold higher, respectively. Moreover, the estimation of the share of polysomes in each ribosomal fraction (sub-units, monosomes, polysomes) showed that, at 100 μM ABA, cytomatrix-bound polysomes, which constituted 90% of polysomes, were the predominant class in ABA-treated germs while membrane-bound polysomes, which made up 82% of polysomes, dominated in the control. A high level of CMBP in ABA-treated tissues may indicate that this class of polysomes participates in ABA-induced synthesis of proteins. In turn, the inhibition of MBP under ABA-treatment is probably due to the delayed protein synthesis which takes place on these polysomes. We identified two lysine-containing proteins synthesized on both of the above classes of polysomes, whose synthesis was altered due to ABA application. Synthesis of a 47 kDa protein on MBP was inhibited, while synthesis of a 79 kDa protein on CMBP is strongly enhanced by ABA influence. The importance of these findings is discussed.     

Der DNS-Gehalt von Kotyledonen und Hypokotyl des Senfkeimlings (Sinapis alba L.) bei der phytochromgesteuerten Photomorphogenese

Zusammenfassung Der DNS-Gehalt und somit auch die Zellzahl von Kotyledonen und Hypokotyl des Senfkeimlings sind zwischen 36 und 60 Std nach Aussaat sowohl im Dunkel als auch im Dunkelrot weitgehend konstant. Die durch Phytochrom bewirkte Zunahme des RNS-und Proteingehaltes (Weidner u. Mitarb., 1965) muß deshalb als eine RNS-bzw. ProteinZunahme pro Zelle aufgefaßt werden. Dieser Befund stützt die Vorstellung einer differentiellen Genaktivierung durch P₇₃₀ (z.B. Mohr, 1966).—Die weitgehend konstante Zellzahl von Hypokotyl und Kotyledonen während des von uns verwendeten Experimentierzeitraumes ist eine wichtige Voraussetzung für die Vergleichbarkeit biochemischer Daten, z.B. bei kinetischen Studien (vgl. Mohr, 1966).

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The DNA contents of cotyledons and hypocotyl of the mustard seedling (Sinapis alba L.) during phytochrome-mediated photomorphogenesis

Summary DNA contents and accordingly cell numbers of cotyledons and hypocotyl of the mustard seedling were virtually constant during the experimental period (between 36–60 hours after sowing) in the dark as well as under the influence of P₇₃₀, the active phytochrome (Table).—Therefore the phytochromemediated increase of the RNA and protein contents (Weidner et al., 1965) must be understood as an increase of RNA and protein per cell. This fact is in agreement with the conception of differential gene activation mediated by P₇₃₀ (Mohr, 1966). The virtually constant DNA contents during the period of time which is regularly used for experimentation on photomorphogenesis in our laboratory (36–60 hours after sowing; Mohr, 1966) is an important prerequisite for comparing biochemical data under the point of view of differential gene activation, e.g. in kinetical studies in the dark and under continuous far-red light.