Carotenoid composition in milo (Sorghum vulgare) shoots as affected by phytochrome and chlorophyll

The composition of coloured carotenoids in the milo shoot was investigated quantitatively (high performance liquid chromatography) during light-mediated plastidogenesis, including the time span of photodelay as caused by medium and high light fluxes. It was found that as long as only the far-red-absorbing form of phytochrome operates, the carotenoid pattern remains virtually the same as in complete darkness (violaxanthin and lutein as major constituents, traces of -carotene). On the other hand, the pattern changes dramatically in white or red light with increasing amounts of chlorophyll (lutein and -carotene dominate, -carotene showing the strongest relative increase). Photodelay during the early phase of plastidogenesis affects the carotenoid composition strongly. Increase of neoxanthin, violaxanthin and -carotene contents are diminished while lutein accumulation proves resistant towards chlorophyll-mediated photoinhibition. The photodelay can be diminished by an appropriate light pretreatment. The data indicate that light-mediated control over carotenoid accumulation is exerted at three levels: i) a coarse control through phytochrome, ii) fine tuning in connection with chlorophyll accumulation, iii) stabilization of holocomplexes against photodecomposition.Abbreviations GG14 high fluence rate green-yellow light - HPLC high-performance liquid chromatography - Chl chlorophyll - WL_w weak white light (1200 lx) - WL_m medium flux white light (12000 lx)     

Biochemical bone marrow markers and their significance in postmenopausal osteoporosis--a new method in the diagnosis of osteoporosis?]

This study analyzes the qualification of biochemical markers in the diagnosis of osteoporosis and evaluates the potential of a multiparametric classification of premenopausal and non-osteoporotic as well as osteoporotic postmenopausal women, which is based on biochemical marker profiles. For this evaluation data of 29 women in the age between 28-74 years were used. The classification of osteoporosis was done by the trabecular density of the lumbar spine using qCT-measurements. The biochemical markers of formation and resorption AP, bAP, OC, ucOC, PICP, PYD, DPD, NTX, BSP and vitamin K were analyzed on day 1 and 42 in all patients. For vitamin K we found significant distribution differences between non-osteoporotic and osteoporotic women (p<0.005). The crosslinks PYD and DPD showed weakly significant differences. All other parameters exhibited non-significant results. Vitamin K acted with a sensitivity of 64% and a specificity of 82%. The used multiparameter classification process improved sensitivity and specificity considerably. The parameter profiles of OC/PYD, vitamin K/PYD and vitamin K/bAP revealed the highest sensitivities with specificities of more than 82%.     

Opsonizing effect of serum and albumin gland extracts on the elimination of human erythrocytes from the circulation of Helix pomatia

The removal of human erythrocytes of the A₁ and B types from the circulation of the gastropod Helix pomatia follows an exponential curve. The elimination of the nonself particles is apparently dependent on serum opsonins as preincubation of A₁ and B erythrocytes in Helix serum increases the rate of their clearance. This conclusion is supported by our finding that secondary doses of nonsensitized A₁ erythrocytes injected 12–19 hr after a similar primary dose are cleared very slowly; however, the clearance rate returns to normal if erythrocytes comprising the second dose are preincubated with Helix serum. Furthermore, the elimination of second-dose A₁ erythrocytes is strongly enhanced after their pretreatment with agglutinating extracts of the albumin glands from H. pomatia and Cepaea (Helix) nemoralis. On the other hand, no opsonizing effect was obtained by pre-incubating A₁ erythrocytes in the agglutinating extract of the sponge Aaptos papillata.     

Kinetische Studien zur Phytochrominduzierten Proteinsynthese

Zusammenfassung In der vorliegenden Arbeit wurde geprüft, wie P₇₃₀, das aktive Phytochrom, den Proteinstoffwechsel in den Kotyledonen des Senfkeimlings (Sinapis alba L.) beeinflußt. Die Daten zur Kinetik des Proteingehalts im Dunkeln und im Dunkelrot, die Daten über die Inkorporation von Radioaktivität in die Proteinfraktion nach Applikation von ¹⁴C-Leucin (U) und die histochemischen Befunde von Häcker (1966) erlauben den Schluß, daß P₇₃₀ eine starke Proteinsynthese (Enzymund Strukturprotein) in den Kotyledonen bewirkt. Dies wird als eine Stütze für die Auffassung angesehen, daß P₇₃₀ in den Kotyledonen in erster Linie über eine differentielle Genaktivierung wirksam wird.

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Kinetical studies on phytochrome-induced protein synthesis

Summary Phytochrome control of protein metabolism has been analyzed in the cotyledons of the mustard seedling (Sinapis alba L.) which can be regarded as being representative of dicotyledonous seedlings. A mustard seedling is a closed system for nitrogen under our experimental conditions. Fig. 2 shows the kinetics of protein content in the cotyledons of the mustard seedling in darkness and under the influence of continuous far-red irradiation, i.e. under the influence of a low but virtually constant concentration of phytochrome 730. —In order to understand these two curves it must be realized that the cotyledons of the mustard seedling contain much storage protein which will be degraded during the development of the seedling. The resulting amino acids are either translocated to other parts of the seedling or used within the cotyledons for the synthesis of enzymes and structural protein. —Histochemical studies have shown (Häcker, 1966) that under the influence of far-red light the degradation of storage protein in the cotyledons is enhanced; at the same time, however, phytochrome 730 stimulates a strong de novo synthesis of structural and enzyme protein in the cotyledons. —This interpretation of the data on protein content is supported by evidence of the phytochrome-enhanced incorporation of ¹⁴C into the protein fraction after an application of ¹⁴C-Leucine (U) (Figs. 5, 6). — All present findings on phytochrome-controlled protein synthesis agree with the hypothesis that phytochrome 730 exerts its function through a differential gene activation (Mohr, 1966b).

     

Photooxidative damage to plastids affects the abundance of nitrate-reductase mRNA in mustard cotyledons

It was found previously that in the mustard (Sinapis alba L.) seedling (Schuster et al. 1989, Planta 177, 74–83) the action of nitrate and phytochrome on the appearance of cytosolic nitrate reductase (NR) is abolished if the plastids are damaged by photooxidation. In the present study this finding has been corroborated by the following results: (i) the appearance and disappearance of NR activity are strictly correlated with the appearance and disappearance of immunoresponsive NR protein; (ii) the appearance of NR correlates with the appearance of translatable NR mRNA; (iii) photodestruction of the plastids strongly reduces the level of NR mRNA. It is concluded that the dependence of the NR level on the state of the plastids can be detected at the level of its mRNA and is not attributable to an inactivation of the enzyme.Abbreviations NR nitrate reductase (EC 1.6.6.1) This research was supported by a grant from the Deutsche Forschungsgemeinschaft. We are greatly indebted to Dr. Ann Oaks (University of Guelph, Ontario, Canada) for the gift of antiserum.     

Characterization and identification of 6 mutagens in opium pyrolysates implicated in oesophagel cancer in Iran

Previous epidemiological studies have indicated an association between the ingestion of opium pyrolysates, dietary deficiencies, and a high incidence of oesophageal cancer in subjects in north-east Iran. Laboratory studies have shown that pyrolysates of opium and particularly of morphine, a major opium alkaloid, are highly mutagenic in bacteria and induce sister-chromatid exchanges in mammalian cells after metabolic activation. We now report the ability of these pyrolysates to transform Syrian hamster embryo cells in culture and present some evidence for their carcinogenicity in mice and hamsters following topical, subcutaneous, intratracheal and intragastric administration. 6 of the most abundant mutagenic compounds present in morphine pyrolysate were isolated and purified by high-performance liquid chromatography and characterized by gas chromatography/mass spectrometry and ¹H-Fourier transform nuclear magnetic resonance spectroscopy. These hitherto unknown compounds, all containing a hydroxy-phenanthrene moiety, were identified as: 3-methyl-3H-naphth[1,2-e]indol-10-ol; 1,2-dihydro-3-methyl-3H-naphth[1,2-e]indol-10-ol; 6-methylaminophenanthren-3-ol; 2-methylphenanthro[3,4-d][1,3]oxazol-10-ol; 2,3-dimethyl-3H-phenanthro[3,4-d]imidazol-10-ol and 2-methyl-3H-phenanthro[3,4-d]imidazol-10-ol. Mutagenicity in Salmonella typhimurium TA98 of these compounds increased in the order listed, the last compound being 35 times more active than benzo[a]pyrene. The mechanisms, by which these mutagens are formed and metabolically activated are discussed.     

AlgR-binding sites within the algD promoter make up a set of inverted repeats separated by a large intervening segment of DNA.

Activation of algD by AlgR is essential for mucoidy, a virulence factor expressed by Pseudomonas aeruginosa in cystic fibrosis. Two AlgR-binding sites, RB1 and RB2, located far upstream from the algD mRNA start site, are essential for the high-level activity of algD. However, the removal of RB1 and RB2 does not completely abolish inducibility of algD in response to environmental signals. In this work, a third binding site for AlgR, termed RB3, near the algD mRNA start site was characterized. Deletion of RB3 abrogated both the AlgR-binding ability and the residual inducibility of the algD promoter. DNase I footprinting analysis of RB3 resulted in a protection pattern spanning nucleotides -50 to -30. Eight of 10 residues encompassing a continuous region of protection within RB3 (positions -45 to -36) matched in the inverted orientation the conserved core sequence (ACCGTTCGTC) of RB1 and RB2. Quantitative binding measurements of AlgR association with RB1, RB2, and RB3 indicated that AlgR had significantly lower affinity for RB3 than for RB1 and RB2, with differences in the free energy of binding of 1.05 and 0.93 kcal/mol (4.39 and 3.89 kJ/mmol), respectively. Altering the core of RB2 to match the core of RB3 significantly reduced AlgR binding. Conversely, changing the core of RB3 to perfectly match the core of RB2 (mutant site termed RB3*) improved AlgR binding, approximating the affinity of RB2. RB3*, in the absence of the far upstream sites, showed an increase in activity, approaching the levels observed with the full-size algD promoter. Changing 4 nucleotides in two different combinations within the core of RB3 abolished the binding of AlgR to this site and resulted in a significant reduction of promoter activity in the presence of the far upstream sites. Thus, (i) the core sequence is essential for AlgR binding; (ii) the three binding sites, RB1, RB2, and RB3, are organized as an uneven palindrome with symmetrical sequences separated by 341 and 417 bp; and (iii) all three sites participate in algD activation.     

Photosynthese und Photomorphogenese bei Farnvorkeimen vonDryopteris filix-mas

Summary Under conditions of identical rate of photosynthesis (measured by dry weight increase under steady state conditions) growth and differentiation of the gametophytes of ferns (e.g.Dryopteris filix-mas) are completely different in red and blue light. In the blue light normal growth and morphogenesis take place and normal two or three-dimensional prothallia are formed (Fig. 3). In the red, however, the prothallia look very similar to those growing in complete darkness: they grow as one-dimensional filaments (Fig. 1).It has been shown in this paper that photosynthesis, which is important as a source of organic material and free energy, has no influence at all on morphogenesis. Morphogenesis, i.e. the formation of normal prothallia instead of filaments, is controlled by a photoreactive system which depends on blue light of suitable intensity and which is not related to photosynthesis as such. If no blue light is present no morphogenesis occurs in spite of high photosynthetic activity.In our opinion theprimary products of photosynthesis are the same in all wavelengths. But now the photomorphogenic light reaction which depends on blue light apparently directs the flow of metabolites. In this way even the same initial products of CO₂ fixation may lead subsequently to rather different photosynthetic products and consequently to the very great difference between prothallia growing with or without blue light.The addition of sucrose has practically no influence on growth and morphogenesis under our conditions. On the basis of our results we cannot agree with the general conclusions drawn byMiller andMiller (1961) who regard photosynthesis as a photomorphogenetic system in these gametophytes of ferns.Mit 6 Textabbildungen.Herrn Professor Dr.E. G. Pringsheim in Verehrung zum 80. Geburtstag.