Covalent and noncovalent receptor-glucocorticoid complexes preferentially bind to the same regions of the long terminal repeat of murine mammary tumor virus proviral DNA

Dexamethasone 21-mesylate, an irreversible antiglucocorticoid in HTC cells, forms a covalent receptor-steroid complex which can be activated in cell-free systems. The molecular basis of its antiglucocorticoid activity is unknown; it might result from altered DNA sequence preferences and/or affinities of the covalent receptor-steroid complex. To test this hypothesis, the affinities of both covalent receptor-antagonist and noncovalent receptor-agonist complexes for defined DNA sequences were measured in a DNA binding competition assay. This assay requires neither purified complexes nor large quantities of DNA, yet it provides quantitative comparisons of the affinities of different double-stranded DNAs for binding receptor-steroid complexes. In this assay, activated covalent receptor-dexamethasone 21-mesylate complexes in crude cytosol bound to calf thymus DNA and cloned subregions of the long terminal repeat (LTR) of murine mammary tumor virus (MMTV) proviral DNA with approximately the same relative affinities as did noncovalent receptor-dexamethasone complexes. Both types of complex exhibited similar orders of preferential binding to DNA sequences. LTR subregions, as well as the entire LTR, were 2-20 times more potent competitors than calf thymus DNA. Cloned sequences from the 3' terminus of the LTR were more effective competitors than either the entire LTR or comparably sized DNAs from the 5' terminus. The DNA sequences with the greatest affinities for both covalent and noncovalent complexes are located within the region of -221 to -67. These studies support the theory that recognition by regulatory elements of specific DNA sequences upstream of responsive genes is an integral step of hormone action.(ABSTRACT TRUNCATED AT 250 WORDS)     

Further evidence for the protein coding potential of the mouse mammary tumor virus long terminal repeat: nucleotide sequence of an endogenous proviral long terminal repeat

The 3′ half of an endogenous mouse mammary tumor virus from a C3H mouse was cloned in the Charon 4A vector phage. A comparison of the proviral clone with previously published endogenous mouse mammary tumor virus restriction maps identified it as endogenous unit II (J. Cohen and H. Varmus, Nature [London] 278:418-423, 1979), which is present in all inbred mouse strains derived from the original Bagg albino × DBA cross. The nucleotide sequence of the unit II long terminal redundancy (LTR) was determined and compared with the sequence previously determined for the exogenous C3H virus LTR (Donehower et al., J. Virol. 37:226-238, 1981). Virtually all sequence differences between the two LTRs were base substitutions. The total amount of sequence divergence was 6.6%. The large open reading frame reported previously in the exogenous LTR was preserved in the endogenous LTR. In addition, the pattern of sequence divergence was highly nonrandom with respect to the putative amino acid codons of the two open reading frames. Most of the base substitutions in this region resulted in silent or conservative amino acid codon changes. The nonrandom divergence pattern indicates that selective forces are operating on this segment of DNA and argues that the putative protein is functional in the life cycle of mouse mammary tumor virus. Possible roles for the protein and its mode of expression are discussed.     

Auxintransport und Phototropismus

Summary Short illumination of excised coleoptiles (with or without apex) inhibits the subsequent transport of IAA-2-¹⁴C in these sections during darkness.To a certain extent the inhibition is dependent both on the light intensity and on the duration of illumination. Only the blue region of the visible spectrum is effective.The light induced inhibition is due to a decrease of the quantity of IAA transported; on the other hand, the velocity of transport remains unchanged.The inhibition of auxin transport can be observed only if coleoptiles contain endogenous or fed auxin during the preceding illumination period. Besides illumination inhibition of auxin transport can also be brought about by incubation of coleoptile sections with a previously illuminated IAA/FMN solution.Auxin transformed by peroxidase operates in the same way. The different oxidation products of IAA in the solutions used were identified: The only product which inhibits elongation growth and auxin transport was 3-M. The conversion of IAA to 3-M is accomplished by crude cell-free extracts from corn coleoptiles.An increased formation of labeled 3-M from IAA-2-¹⁴C during illumination of coleoptiles could be demonstrated.Since 3-M is not actively transported in coleoptiles, it must be assumed that 3-M functions as an inhibitor of auxin transport only at its site of formation.It is concluded that the phototropic curvature of coleoptiles and stems is triggered by the photooxidative formation of 3-M from IAA in the side exposed to light. The flow of growth substances will be partly blocked by 3-M in this side and can be directed to the shaded side.On the strength of these findings some phenomena of phototropism (transmission of stimulus, mneme, quantum yield) can easily be explained.

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Abkürzungen FMN Flayinmononucleotid - IES Indol-3-essigsäure - 3-M 3-Methylenoxindol - NES -Naphthylessigsäure Herrn Prof. Dr. L. Brauner zum 70. Geburtstag in Dankbarkeit gewidmet.     

Untersuchungen üben die Rückreaktionen im Xanthophyll-Cyclus bei Chlorella,Spinacia und Taxus

Zusammenfassung Die als Rückreaktion bezeichnete Epoxidierung des Zea. ²über das Monoepoxid Anth. zum Diepoxid Viol. wird an verschiedenen pflanzlichen Objekten und unter verschiedenen Bedingungen untersucht.In Chlorella und den Nadeln von Taxus baccata ist sofort nach Beendigung der starken Belichtung die Rückumwandlung zu beobachten. Diese ist durch Begasung des Pflanzenmaterials mit reinem O₂ oder durch schwaches Licht noch etwas zu beschleunigen.In Blattscheibchen von Spinacia oleracea ist eine solche Epoxidierung unter Normalbedingungen (Dunkelheit, Luft) nicht festzustellen. Sie setzt erst unter dem Einfluß von schwachem Licht oder bei Zufuhr von O₂ (100%) ein. Das Fehlen der Rückreaktion hat seine Ursache in einem unter den gegebenen Versuchsbedingungen stattfindenden Spaltöffnungsverschluß, der während der Starklichtgabe beginnt und während der nachfolgenden Dunkelheit noch anhält, und einer daraus resultierenden Anaerobiose in den plastidenhaltigen Zellen. Durch eine Erhöhung der O₂-Spannung in diesen Zellen, entweder durch von außen zugeführten reinen O₂ oder durch intracelluläre Entwicklung von Photosynthese-O₂ (verbunden mit einer teilweisen Öffnung der Stomata), kommt es auch in den Spinatblättern zu einer Rückreaktion. Schwaches Licht kann also auf indirektem Weg die Rückreaktion beschleunigen.Die Konzentration des Zwischenproduktes Anth. nimmt bei der O₂-oder schwachlichtgeförderten Rückreaktion anfänglich stärker zu als das Endprodukt Viol. Daraus folgt, daß bei der Epoxidierung die beiden O-Atome nicht gleichzeitig, sondern nacheinander in die 5,6- und 5,6-Stellung des Zea. eingebaut werden.In isolierten Chloroplasten oder Zellfragmenten konnte bisher unter verschiedensten Bedingungen keine Rückreaktion nachgewiesen werden. Eine in gefriergetrockneten Zellen oder Chloroplasten durch Licht und O₂-Atmosphäre ausgelöste scheinbare Rückreaktion ist auf eine verschieden schnelle photooxidative Zerstörung der Carotinoide zurückzuführen.Die Epoxidierung des Zea., welche durch ein wahrscheinlich Cuhaltiges Enzym katalysiert wird, ist in vivo an das Vorhandensein von molekularem O₂ gebunden.

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Studies on the backward-reactions in the xanthophyll-cycle of Chlorella, Spinacia and Taxus

Summary The epoxidation of zeaxanthin to the di-epoxide violaxanthin via the mono-epoxide antheraxanthin (called the backward-reaction), is examined with several plant objects and under various conditions.In Chlorella and in the needles of Taxus baccata a backward-conversion can be observed immediately after the termination of strong illumination. The reaction can be accelerated somewhat by exposure of the plant material to pure O₂ or dim light.One cannot observe such an epoxidation in leaf disks of Spinacia oleracea under normal conditions (dark, air). It begins only under the influence of dim light or when pure oxygen is supplied. The absence of the backward-reaction under the given experimental conditions is a consequence of a closure of the stomata, which begins during the strong illumination and continues in the succeeding dark period; it is therefore a consequence of anaerobiosis in the plastid-containing cells. Yet a backward-reaction starts if the O₂-tension in the cells is increased either by pure O₂ given from outside or by the intracellular evolution of photosynthetic O₂ (associated with a partial opening of the stomata).The concentration of the intermediate antheraxanthin increases strongly more at the beginning of the O₂- or dim-light-promoted backward-reaction than the concentration of the endproduct violaxanthin. Hence it follows that during epoxidation the two O-atoms are added to the 5,6- and the 5,6-position of the zeaxanthin not simultaneously but one after the other.In isolated chloroplasts or cell fragments no backward-reaction could be observed under various conditions tested. An apparent backward-reaction in lyophilized cells or chloroplasts, which is triggered by light or O₂-atmosphere, is a result of the different velocity of the photooxidative destruction of carotenoids.The in vivo epoxidation of zeaxanthin, which probably is catalysed by a Cu-containing enzyme, only proceeds in the presence of molecular O₂.

     

吗啡耐受大鼠心房心钠素的释放及其基因转录

本工作应用心钠素放射免疫测定和分子杂交技术首次发现,吗啡耐受大鼠血浆心钠素水平显著降低,心房内心钠素含量明显升高,同时心房内心钠素特异性mRNA水平也相应提高,提示在吗啡耐受时大鼠心房内心钠素的合成和贮存增加,释放减少。     

Short chain alcohols activate guanine nucleotide-dependent phosphoinositidase C in turkey erythrocyte membranes

The ability of alcohols to regulate inositol lipid-specific phospholipase C (phosphoinositidase C) was examined in turkey erythrocyte ghosts prepared by cell lysis of erythrocytes which were prelabeled with [3H] inositol. Guanosine 5'-[gamma-thiotriphosphate] GTP[S] stimulated the production of both [3H]inositol bisphosphate (18-fold) and [3H]inositol trisphosphate (6-fold) in this system. The accumulation of [3H]inositol bisphosphate and [3H]inositol trisphosphate was linear up to 8 min following an initial lag period of 1-2 min. Ethanol (300 mM) reduced the lag period for [3H]inositol phosphate accumulation at submaximal GTP[S] concentrations and caused a shift to the left (3-fold) in the dose-response curve. Other short chain alcohols, methanol (300 mM), 1-propanol (200 mM), and 1-butanol (50 mM) also enhanced the accumulation of [3H] inositol phosphates in the presence of submaximal GTP[S] concentrations. Receptor activation by the purinergic agonist adenosine 5'-[beta-thio]disphosphate (ADP[S]) (10 microM) also reduced the lag period for [3H] inositol phosphate formation and shifted the GTP[S] dose response to the left (10-fold). In addition, ADP[S] increased the response to maximal GTP[S] concentrations. The formation of [3H]inositol phosphates induced by GTP[S] was associated with a concomitant decrease in labeling of both [3H]phosphatidylinositol monophosphate and [3H]phosphatidylinositol bisphosphate, but no decrease in [3H]phosphatidylinositol was observed. All of the alcohols tested enhanced the breakdown of [3H]polyphosphoinositides in the presence of GTP[S]. The dose response to guanosine 5'-[beta gamma-imino]triphosphate for [3H]inositol phosphate formation was displaced to the left by ethanol (300 mM) and ADP[S] (10 microM) (2- and 7-fold), respectively. ADP[S] also enhanced the maximal response to guanosine 5'-[beta gamma-imino]triphosphate. The [3H]inositol phosphate formation produced in response to NaF was unaffected by either ethanol or receptor activation. These results indicate that alcohols initiate an activation of phosphoinositidase C, mediated at the level of the regulatory guanine nucleotide-binding protein.     

Production of DON-related trichothecenes byFusarium graminearum Schw from Krasnodarski krai of the USSR

34Fusarium graminearum Schw isolates produced 4-deoxynivalenol to form significant amounts of 4, 7 — dideoxynivalenol and lesser amounts of 4 — deoxynivalenol monoacetates on grain substratesin vitro. This is the first report on the capability a large group of naturally occurring isolates to produce 4,7-dideoxynivalenol. The average levels of 4,7-dideoxynivalenol on rice, corn, barley, and wheat as a substrate were respectively 26.8, 14.0, 12.8, and 10.5% of the level of 4-deoxynivalenol. 4, 7 — dideoxynivalenol was present in all examined naturally contaminated wheat kernel samples at levels of 1.7 to 7.9% of the level of 4-deoxynivalenol. These findings suggest that more attention should be given to the occurrence of 4,7-dideoxynivalenol in cereals.     

Rapid reactions of spruce cells to elicitors released from the ectomycorrhizal fungus Hebeloma crustuliniforme, and inactivation of these elicitors by extracellular spruce cell enzymes

Elicitors released from hyphae or cell walls of the ectomycorrhizal fungus Hebeloma crustuliniforme (Bull. ex Fries.) Quél. induced in suspension-cultured cells of Picea abies (L.) Karst. a set of fast reactions: (i) an immediate efflux of Cl^– into the medium, followed by a K⁺ efflux; (ii) an influx of Ca²⁺ (measured as accumulation of ⁴⁵Ca²⁺ in the cells); (iii) a phosphorylation of a 63-kDa protein and dephosphorylation of a 65-kDa protein (detectable by 4 min after elicitor application); (iv) an alkalinization of the medium, and (v) a transient synthesis of H₂O₂. The removal of extracellular Ca²⁺ by EGTA delayed the elicitor-induced alkalinization. A further reduction of this response could be achieved by TMB-8 an inhibitor of Ca²⁺ release from intracellular stores. Moreover, the inhibition of protein kinase activity by staurosporine prevented the extracellular alkalinization completely. However, the effectiveness of the elicitors in inducing the extracellular alkalinization was strongly impaired by constitutively secreted enzymes of spruce cells which cleaved the elicitors to inactive fragments. It is suggested that in ectomycorrhizae the efficacy of elicitors released from fungal cell walls is controlled by apoplastic enzymes of the host; the plant itself is able to reduce the activity of fungal elicitors on their way through the plant cell wall. But those elicitors which finally reach the plasma membrane of host cells induce reactions that are similar to the early defense reactions in plant-pathogen interactions.Abbreviations DW dry weight - FW fresh weight - TMB-8 3,4,5 trimethoxybenzoic acid 8-(diethylamino)-octyl ester We thank Prof. M. Zenk (Universität München, Germany) for providing spruce cell cultures, and Dr. I. Kottke (Universität Tübingen, Germany) for isolates of Hebeloma crustuliniforme Tü 704. We are also thankful to Dr. W. Mayer (Universität Tübingen) for valuble discussions. This work was supported by Deutsche Forschungsgemeinschaft. B. Zitterell-Haid was financed by Graduiertenkolleg Interaktion in Waldökosystemen (supported by Deutsche Forschungsgemeinschaft) and G. Hebe by a scholarship of the Landesgraduiertenförderungsgesetz.