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1

Electronic Resource

Identification of aluminium forms in tea leaves by ^2^7Al NMR

Nagata, T. ; Hayatsu, M. ; Kosuge, N.

Amsterdam : Elsevier

Phytochemistry 31 (1992), S. 1215-1218

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ISSN: 0031-9422

Keywords: Camellia sinensis ; Camelliaceae ; ^2^7Al NMR ; aluminium complex ; catechin ; fluorine ; leaf ; organic acid ; phenolic acid

Source: Elsevier Journal Backfiles on ScienceDirect 1907 - 2002

Topics: Biology , Chemistry and Pharmacology

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1016/0031-9422(92)80263-E

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2

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Aluminium kinetics in the tea plant using ^2^7Al and ^1^9F NMR

Nagata, T. ; Hayatsu, M. ; Kosuge, N.

Amsterdam : Elsevier

Phytochemistry 32 (1993), S. 771-775

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ISSN: 0031-9422

Keywords: Camellia sinensis ; Theaceae ; ^1^9F NMR ; ^2^7Al NMR ; aluminium complexes ; catechin ; fluorine ; kinetics.

Source: Elsevier Journal Backfiles on ScienceDirect 1907 - 2002

Topics: Biology , Chemistry and Pharmacology

Type of Medium: Electronic Resource

URL: http://linkinghub.elsevier.com/retrieve/pii/0031-9422(93)85202-3

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3

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Purine base pattern of camellia irrawadiensis

Nagata, T. ; Sakai, S.

Amsterdam : Elsevier

Phytochemistry 24 (1985), S. 2271-2272

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ISSN: 0031-9422

Keywords: C. sinensis ; Camellia irrawadiensis ; Theaceae ; caffeine ; leaf. ; tea ; theobromine

Source: Elsevier Journal Backfiles on ScienceDirect 1907 - 2002

Topics: Biology , Chemistry and Pharmacology

Type of Medium: Electronic Resource

URL: http://linkinghub.elsevier.com/retrieve/pii/S0031-9422(00)83024-1

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4

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Simultaneous determination of nicotine and cotinine in various human tissues using capillary gas chromatography/mass spectrometry (1994)

Urakawa, N. ; Nagata, T. ; Kudo, K. ; [et al.]

Springer

International journal of legal medicine 106 (1994), S. 232-236

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ISSN: 1437-1596

Keywords: Nicotine ; Cotinine ; Gas chromatography/mass spectrometry ; Human Tissue ; Distribution ; Smokers' level ; Nikotin ; Cotinin ; Gaschromatographie/Massenspektrometrie ; Menschliches Gewebe ; Verteilung ; Tabakraucher

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine , Law

Description / Table of Contents: Zusammenfassung Zur gleichzeitigen Bestimmung von Nikotin und Cotinin in verschiedenen Körpergeweben wurde eine zuverlässige und sensitive Methode mittels der Kapillar-Gas-Chromatographie/Massenspektrometrie entwickelt. Nikotin und Cotinin wurden durch einen 3-stufigen Extraktionsvorgang mit Chinolin als internem Standard isoliert und die Quantifizierung mittels der single ion monitoring-Technik durchgeführt, wobei für Nikotin das Ion m/z 133, für Cotinin m/z 176 und für Chinolin m/z 129 verwendet wurde. Die Detektionsgrenze lag in allen Geweben für Nikotin bei 5 ng/g und für Cotinin bei 10 ng/g, die Kalibrierung erbrachte lineare Verhältnisse im Bereich von 5–1.200 ng/g für Nikotin und im Bereich von 10–1.500 ng/g für Cotinin. Die Genauigkeit und Präzision der Methode wurde an verschiedenen Körpergeweben ausreichend bewiesen. Die Verteilung der beiden Verbindungen in verschiedenen Geweben wurde in 10 Fällen bestimmt. Die festgestellten Nikotinspiegel lagen hierbei bei Konzentrationen, die bei üblichen Tabakrauchern gemessen werden. Hohe Nikotinspiegel wurden in Leber, Niere, Milz und Lunge, niedrige Konzentrationen im Fettgewebe festgestellt. Die Cotinin-Konzentration lag in der Leber am höchsten. Das Gewebe-Blut-Verteilungsverhältnis für Nikotin und Cotinin war im Skelettmuskelgewebe am konstantesten, wobei die Konzentrationen hier jeweils nahe an den Konzentrationen im Blut lagen. Der Skelettmuskel ist somit das geeignetste Gewebe für toxikologische Untersuchungen, wenn die Asservierung von Blut nicht möglich ist.

Notes: Summary A reliable and sensitive method for the simultaneous determination of nicotine and cotinine concentrations in various human tissues was developed using capillary gas chromatography/mass spectrometry. Nicotine and cotinine were extracted using a 3-step solvent extraction procedure and quinoline as an internal standard. Quantification was carried out by single ion monitoring using ions of m/z 133 for nicotine, m/z 176 for cotinine and m/z 129 for quinoline. The lower limit of detection was 5 ng/g for nicotine and 10 ng/g for cotinine, in each tissue sample. The calibration curves of various tissues were linear in the concentration range from 5–1,200 ng/g for nicotine and 10–1,500 ng/g for cotinine. The accuracy and precision of this method were examined using human tissues and the results were satisfactory. The distribution of nicotine and cotinine was measured in tissues from 10 human autopsies. Nicotine was detected in every tissue examined at a level seen in habitual smokers. The nicotine concentration was high in the liver, kidney, spleen and lung, and low in adipose tissue. The cotinine level was highest in the liver. The tissue/blood concentration ratios of nicotine and cotinine were most stable in skeletal muscle, where the level of these drugs was close to that in whole blood. Skeletal muscle is, therefore, considered to be the most suitable tissue sample for toxicological examination, when acquisition of blood samples is not feasible.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01225411

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5

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Microtubule organizing centers in plant cells: localization of a 49 kDa protein that is immunologically cross-reactive to a 51 kDa protein from sea urchin centrosomes in synchronized tobacco BY-2 cells (1993)

Hasezawa, S. ; Nagata, T.

Springer

Protoplasma 176 (1993), S. 64-74

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ISSN: 1615-6102

Keywords: Cell cycle ; Microtubule ; Microtubule organizing center ; Synchronization ; Tobacco BY-2 cells

Source: Springer Online Journal Archives 1860-2000

Topics: Biology

Notes: Summary A 49 kDa protein in tobacco BY-2 cells has been found to be cross-reactive with antibodies raised against a 51 kDa protein that was isolated from sea urchin centrosomes and identified as a microtubule-organizing center (MTOC) in animal cells. Tracing the fate of the 49 kDa protein during progression of the cell cycle in highly synchronized tobacco BY-2 cells revealed that this protein was colocalized with plant microtubules (MTs): the location of the 49 kDa protein coincided with preprophase bands (PPBs), mitotic spindles and phragmoplasts. Furthermore, between the M and G1 phases, the 49 kDa protein was observed in the perinuclear regions, in which the initials of MTs are organizing to form cortical MTs. At the G1 phase the location of the 49 kDa protein in the cell cortex coincided with that of the cortical MTs. It appeared that the 49 kDa protein in the cell cortex was transported as granules from the perinuclear regions. Thus, it is highly probable that the 49 kDa protein, which reacts with antibodies against the 51 kDa protein in sea urchin centrosomes, plays the role of an MTOC in plant cells. Thus, the mechanisms for organizing MTs in higher organisms appear to share a common protein, even though the organization of MTs is superficially very different in plant and animal cells.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01378940

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6

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The role of microfilaments in the organization and orientation of microtubules during the cell cycle transition from M phase to G1 phase in tobacco BY-2 cells (1998)

Hasezawa, S. ; Sano, T. ; Nagata, T.

Springer

Protoplasma 202 (1998), S. 105-114

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ISSN: 1615-6102

Keywords: Cell cycle ; Elongation factor 1α ; Microfilament ; Microtubule ; Tobacco BY-2 cell line

Source: Springer Online Journal Archives 1860-2000

Topics: Biology

Notes: Summary During cell cycle transition from M to G1 phase, micro-tubules (MTs), organized on the perinuclear region, reached the cell cortex. Microfilaments (MFs) were not involved in this process, however, MFs accumulated to form a ring-like structure in the division plane and from there they elongated toward the distal end in the cell cortex. Subsequently, when MTs elongated along the long axis of the cells, towards the distal end, the MTs ran into and then associated with the predeveloped MFs in the cell cortex, suggesting the involvement of MFs in organizing the parallel oriented MTs in the cell cortex. When cortical MTs were formed in the direction transverse to the long axis of cells, the two structures were again closely associated. Therefore, with regards to the determination of the direction of organizing MTs, predeveloped MFs may have guided the orientation of MTs at the initial stage. Disorganization of MFs in this period, by cytochalasins, prevented the organization of cortical MTs, and resulted in the appearance of abnormal MT configurations. We thus demonstrate the involvement of MFs in determining the orientation and organization of cortical MTs, and discuss the possible role of MFs during this process.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01280879

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7

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Sites of microtubule reorganization in tobacco BY-2 cells during cell-cycle progression (1997)

Hasezawa, S. ; Kumagai, F. ; Nagata, T.

Springer

Protoplasma 198 (1997), S. 202-209

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ISSN: 1615-6102

Keywords: Cell cycle ; Elongation factor 1α ; Microtubule reorganization ; Microfilament ; Tobacco BY-2 cells

Source: Springer Online Journal Archives 1860-2000

Topics: Biology

Notes: Summary The sites of microtubule (MT) reorganization were examined in synchronized tobacco BY-2 cells. The MTs of these cells were completely destroyed by a combined cold and drug treatment at 0 °C with 100 μM propyzamide for 3 h. After the cells were washed and cultured at 30 °C, the reorganization of MTs was observed in detail. Sites for MT reorganization at each stage of the cell cycle were identified on the cell cortex and nuclei, the mitotic apparatus, the nuclei (or the nuclei and cell cortex), and the cell cortex in the S-G2 phase, M phase, M/G1 interface, and g1 phase, respectively. The polypeptide synthesis elongation factor (EF)-1α is co-localized with these sites of MT reorganization. At some stages, microfilaments (MFs) were found to be involved in the reorganization of MTs. Based on these results, the mode of MT reorganization during cell cycle progression is discussed.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01287569

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8

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Forensic analysis of triazolam in human tissues using capillary gas chromatography (1991)

Kudo, K. ; Nagata, T. ; Imamura, T. ; [et al.]

Springer

International journal of legal medicine 104 (1991), S. 67-69

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ISSN: 1437-1596

Keywords: Triazolam ; Estazolam ; Capillary GC/NPD ; Human tissue ; Forensic toxicology ; Triazolam ; Estazolam ; Kapillar-Gaschromatographie/NPD ; Menschliches Gewebe ; Forensische Toxikologie

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine , Law

Description / Table of Contents: Zusammenfassung Eine zuverlässige und empfindliche Methode wurde entwickelt, um die Konzentrationen des hypnotischen Medikaments Triazolam in menschlichen Geweben, einschließlich fauler Gewebe bestimmen zu können. Die Methode besteht aus einer dreistufigen Flüssig-Flüssig-Extraktion, einem Clean up an Kieselgel und Gaschromatographie mit einem Stickstoff-PhosphorDetektor und einer Kapillarsäule. Als interner Standard wurde Estazolam benutzt. Die Eichkurve war im Konzentrationsbereich zwischen 1 ng/g und 1 gg/g linear, und die untere Nachweisgrenze betrug 0.5 ng/g. Es wurde eine forensische Untersuchung über die toxikologischen Effekte von Triazolam an faulem Gewebe durchgeführt.

Notes: Summary A reliable and sensitive method has been developed to assess the concentrations of the hypnotic drug triazolam in human tissues, including putrefied tissues. The method involves a 3-step solvent extraction, cleanup on a silica gel column and gas chromatography using a nitrogen phosphorus detector and a capillary column. Estazolam was used as an internal standard. The calibration curve was linear over the concentration range 1 ng/g1 gm/g and the lower limit of detection was 0.5 ng/g. A forensic study was performed on the toxicological effects of triazolam using putrefied tissues.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01626033

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