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GANGLIOSIDES IN NERVOUS TISSUE CULTURES AND BINDING OF 125I-LABELLED TETANUS TOXIN, A NEURONAL MARKER (1977)

Dimpfel, W. ; Huang, R. T. C. ; Habermann, E.

Oxford, UK : Blackwell Publishing Ltd

Journal of neurochemistry 29 (1977), S. 0

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ISSN: 1471-4159

Source: Blackwell Publishing Journal Backfiles 1879-2005

Topics: Medicine

Notes: Abstract— —Continuous cell lines, primary cell cultures derived from embryonic CNS, and homogenates made from adult and embryonic CNS were compared with respect to their lipid pattern and their ability to bind 125I-labelled tetanus toxin. In parallel experiments de novo synthesis of gangliosides in the cell lines was studied, using [14C]glucosamine as precursor. Of the total lipid only gangliosides were specifically labelled by [14C]glucosamine. The patterns of the de novo synthesized gangliosides corresponded to those present in the respective cells.Pronounced binding of 125I-labelled toxin was only detectable in tissues containing long-chain gangliosides (ganglioside C which represents GDIb and GTI).Accordingly, hybrid (neuroblastoma x glioma) cells, due to their lack of long-chain gangliosides, bound just-discernible amounts of labelled toxin. When previously exposed to gangliosides, their binding of tetanus toxin tremendously increased.It was concluded that only the long-chain gangliosides in the neuronal cells are functionally involved in the binding of the tetanus toxin and that these acceptors of tetanus toxin can be transplanted.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1111/j.1471-4159.1977.tb09626.x

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BINDING CHARACTERISTICS OF 125I-LABELLED TETANUS TOXIN TO PRIMARY TISSUE CULTURES FROM MOUSE EMBRYONIC CNS (1977)

Dimpfel, W. ; Habermann, E.

Oxford, UK : Blackwell Publishing Ltd

Journal of neurochemistry 29 (1977), S. 0

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ISSN: 1471-4159

Source: Blackwell Publishing Journal Backfiles 1879-2005

Topics: Medicine

Notes: Abstract— The interaction of 125I-labelled tetanus toxin with cells in tissue cultures derived from embryonic CNS has been studied.The optimum toxin binding occurs about 2–3 weeks after transfer of the cells to culture conditions. The amount of label bound per culture was doubled at this time in comparison to the fourth day nfter inoculation.The amount of toxin bound depends on the concentration applied. It reaches its maximum 8 h after application then decreases slowly. Low amounts of radioactivity were still detectable 97 h after washing off the unbound toxin. Up to 80% of the label can be replaced by simultaneous application of‘cold’toxin. Fixation of the toxin is higher at 4°C than at 37°C.Preincubation of the cultures with neuraminidase prevents about 75% of the binding. The presence of cytochalasin B leads to a small but reproducible decrease of binding, whereas colchicine had no measurable effect.The radioactive (1251) material was identified by a double-isotope technique in disc gel electrophoresis before and after reductive cleavage of its disulphide bonds. In every test is was indistinguishable from 131I-labelled toxin added as standard.Our results largely parallel those obtained with synaptosomes and other systems. They suggest that gangliosides might be the acceptor molecules, and that the culture system will be suitable for studying the actions of this toxin in vitro.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1111/j.1471-4159.1977.tb06516.x

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3

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Rudolf Buchheim and the Beginning of Pharmacology as a Science (1974)

Habermann, E R

Palo Alto, Calif. : Annual Reviews

Annual Review of Pharmacology 14 (1974), S. 1-9

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ISSN: 0362-1642

Source: Annual Reviews Electronic Back Volume Collection 1932-2001ff

Topics: Medicine , Chemistry and Pharmacology

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1146/annurev.pa.14.040174.000245

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4

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Pharmakokinetische Besonderheiten des Tetanustoxins und ihre Beziehungen zur Pathogenese des lokalen bzw. generalisierten Tetanus (1970)

Habermann, E.

Springer

Naunyn-Schmiedeberg's archives of pharmacology 267 (1970), S. 1-19

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ISSN: 1432-1912

Keywords: Tetanus Toxin-Labelled Protein ; Spinal Cord ; Pharmaco-kinetics ; Radioimmunassay ; Tetanustoxin ; Markierte Proteine ; Rückenmark ; Phar-makokinetik ; Radioimmunassay

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 1. The preparation and properties of125I-labelled tetanus toxin are described. 2. After intravenous injection there is a short phase when the labelled toxin is rapidly removed from the blood plasma. This initial period is followed by a slow second phase of decay which has a longer duration. The first phase in very pronounced in rabbits, but not in rats. Unlabelled toxin is removed equally fast from rabbit plasma, as has been revealed by measuring the immunological reactivity (so-called “junction test”) and toxicity. 3. Thirty minutes after i.v. administration torabbits about 2/3 of the radioactive label are found in the liver. The highest concentration is attained in the spleen. 24 hours later, the bulk of the label has been excreted in the urine and faeces, which indicates catabolism of the toxin. In therat, the concentration in the liver is much less prominent, and the excretion of the label is slower. In both species, the central nervous system does not accumulate more than just measurable quantities of the label, even if the animals are given large toxic doses. 4. After injection into the left gastrocnemius muscle of the rat, the labelled tetanus toxin is absorbed very slowly from the site of administration. It is taken up by the corresponding N. ischiadicus and the lumbar region of the spinal cord. The injection of toxin into the anterior leg leads to concentration of radioactivity in the cervical area of the medulla. The arrival of the label in the spinal cord coincides approximately with the appearance of local tetanus. Sectioning of the N. ischiadicus prevents the appearance of the local tetanus of the lower extremity. The enrichment of the toxin in the lumbar cord is prevented in operated, but not in sham-operated rats. 5. When the spinal cord was subdivided into four sectors, the label was found to be greatly concentrated in the ipsilateral ventral sector of the segment corresponding with the injected extremity. This indicates transport into the ventral roots. 6. 131I-labelled tetanus antitoxin also disappears very slowly from the rat gastrocnemius. In contrast to labelled tetanus toxin, however, it is not concentrated in the spinal cord.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00997110

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Pharmakologische Charakterisierung der vasculÄren Schrankenfunktion gegenüber Erythrocyten und Albumin (1970)

Just, D. ; Urbanitz, D. ; Habermann, E.

Springer

Naunyn-Schmiedeberg's archives of pharmacology 267 (1970), S. 399-420

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ISSN: 1432-1912

Keywords: Vascular Permeability ; Haemorrhage ; Basement Membrane ; 125J-Human Albumin ; 51Cr-Erythrocytes ; GefÄ\permeabilitÄt ; HÄmorrhagie ; Basalmembran ; 125J-Humanalbumin ; 51Cr-Erythrocyten

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 1. Rabbits first received51Cr labelled erythrocytes and then125J-labelled human serum albumin intravenously, followed by the intracutaneous administration of the agents to be tested. The skin areas were excised and evaluated for escape of albumin and red blood cells. Three modes of vascular alteration have been distinguished: a) Increase of permeability for solutes, but not for erythrocytes, as caused by histamine and bradykinin (type I). b) True haemorrhage, as induced by collagenase or the snake venom factor called HR1. No prior increase of albumin permeability has been observed when following the dependence of collagenase action on time or when measuring the ratio between dose and effect, which is linear. Haemorrhage is always accompanied by escape of some additional protein (type II). c) Alterations of a mixed type, as caused by trypsin and chymotrypsin, to a lesser extent by the tenside lysolecithin. Haemorrhage is preceded and accompanied by massive leakage of albumin. For trypsin and chymotrypsin, the dose response ratio is semilogarithmic over a wide range, whereas for lysolecithin it is linear. Hyaluronidase is ineffective in rabbit vessels but enhances the escape of albumin in rats. Histamine release may be relevant as intermediary step since systemic pretreatment with mepyramine is partially preventive. 2. In order to correlate the in vivo findings with biochemical changes, glomerular basement membranes from rats were incubated with the agents mentioned. The release of proteins and peptides was measured by a modification of Folin's method. a) Bradykinin, histamine, and hyaluronidase are ineffective. b) The tenside lysolecithin solubilizes proteins and peptides when applied in high concentrations only. c) Collagenase and HR1 are about equieffective. d) Trypsin and chymotrypsin are about ten times more active than collagenase and HR1. 3. Therefore, haemorrhage and increase of albumin permeability are two clearly distinct phenomena. Our results support the following working hypothesis: Haemorrhage is due to damage of the stabilizing apparatus of the vessel, e.g. basement membranes and surrounding fibrils; the barrier for albumin, however, is to be sought in the endothelial layer of typical capillaries.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00997277

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6

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On the endogenous mechanism of kinin release (1971)

Jahrreiss, Rosemarie ; Habermann, E.

Springer

Naunyn-Schmiedeberg's archives of pharmacology 269 (1971), S. 85-100

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ISSN: 1432-1912

Keywords: Kininogens ; Kallikreins ; Bradykinin ; Protease Inhibitors ; Hageman Factor

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 1. Prekallikrein, prepared according to Nagasawaet al., has been purified further by agarose gel electrophoresis. It can be activated directly by Hageman factor and by solid phase trypsin. Its specific activity (benzoyl arginine ethyl ester as substrate) was 13.2 μM min−1 mg−1. Gel filtration on a calibrated column of sephadex G 200 revealed a molecular weight of 101,000, which is close to the value reported for casein-activated kallikrein. 2. The contact-activated bovine enzyme was very similar to casein-activated porcine kallikrein. Both enzymes hydrolyzed benzoyl arginine ethyl ester and tosylarginine methyl ester with about the same speed. The sensitivity of the two preparations against trasylol®, soy bean inhibitor, and serum inhibitor was also not different. 3. In contrast to previous assumptions, purified bovine LMW kininogen (MW 50,000) proved to be substrate for contact-activated kallikrein. As with the caseinactivated enzyme, the total bradykinin content of the kininogen could be released. 4. Serum, even when heated previously to 61°C, contains inhibitors against kallikreins activated by contact or casein, as well as against trypsin. Whereas pretreatment according to Diniz and Carvalho (pH about 2; 98°C) renders the serum more susceptible to trypsin, such denaturated substrate is less accessible for both kallikreins. Serum or plasma pretreated according to Horton (pH2; 37°C), yield at least 50% of the kinin activity obtained with trypsin, irrespective of the kallikreins used. 5. When acid-treated (according to Horton) 61°-serum has been incubated first with casein-activated kallikrein, contact-activated enzyme does not release additional kinin activity and vice versa. 6. Plasma which has been rotated exhaustively with glass, nevertheless contains substrate for contact-activated kallikrein. 7. Addition of Hageman factor to Horton's substrate does not increase the kinin yield above that obtained by glass-contact of normal plasma. Addition of prekallikrein, however, increases the kinin yield about threefold. Therefore, neither Hageman factor nor substrate, but the actual amount of active kallikrein limits the kinin yield upon glass activation. 8. Our experiments with serum kallikreins and their substrates can be interpreted without assuming a distinct, contact activated kinin system.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01422018

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The prothrombin-activating principle from Echis carinatus venom (1972)

Schieck, A. ; Kornalik, F. ; Habermann, E.

Springer

Naunyn-Schmiedeberg's archives of pharmacology 272 (1972), S. 402-416

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ISSN: 1432-1912

Keywords: Snake Venom ; Blood Coagulation ; Prothrombin ; Hemorrhage ; Proteolysis

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 1. The procoagulant from Echis carinatus venom, which is known to convert prothrombin into thrombin, has been purified by chromatography on calcium hydroxylapatite and DEAE cellulose. Final purification, when necessary, can be achieved by disc gel electrophoresis. A final concentration of 0.5 μg/ml coagulates human citrate plasma in 70 sec. 2. The bulk of hemorrhagic, caseinolytic and fibrinogenolytic activities present in the starting venom is removed during purification, but the procoagulant causes some fibrinogenolysis, gelatinolysis, caseinolysis and hemorrhage, even when homogenous in disc gel electrophoresis. This argues for a proteolytic nature of the procoagulant activity. It is resistant against diisopropyl fluorophosphate and is not, therefore, an esteroprotease. Other protease inhibitors (from soy bean, lima bean, bovine pancreas and bovine serum) are also without effect. 3. The molecular weight is approximately 86 000, as determined by gel filtration. On isoelectric focusing in solution, its isoelectric point is pH 4.4±0.1. The procoagulant is relatively unstable; for instance, its pH-stability is restricted to values between 6 and 10.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00501247

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8

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Distribution of 125I-tetanus toxin and 125I-toxoid in rats with generalized tetanus, as influenced by antitoxin (1973)

Habermann, E. ; Dimpfel, W.

Springer

Naunyn-Schmiedeberg's archives of pharmacology 276 (1973), S. 327-340

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ISSN: 1432-1912

Keywords: Tetanus Toxin ; Pharmacokinetics ; Central Nervous System ; Iodine Labelling ; Receptors

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary In order to understand the symptomatology of generalized tetanus from the pharmacokinetics of the toxin, 125I-labelled toxin was injected i.v. in rats without and with antitoxin. 1. After a few hours latency, brain stem and spinal cord concentrate radioactive material up to the third day. The decline of radioactivity is very slow, semilogarithmic, and can be followed up to the 24th day after injection. In contrast, forebrain and cerebellum do not bind measurable radioactivity. Less than 1% of the radioactivity injected is found in the CNS. 2. The symptoms of tetanus start some time after the bulk of labelled toxin has been taken up by the CNS. They cease before all radioactivity has left it. 3. Antitoxin, given simultaneously, prevents the onset of symptoms and the uptake of radioactivity by the CNS. When given 10 h after labelled toxin, it nearly abolishes the fixation and still prevents the onset of symptoms. When given 48 h after toxin, it is nearly ineffective in both respects. Antitoxin first delays, then enhances the elimination of labelled toxin from the blood. 4. Labelled antitoxin is not enriched in the CNS. 5. The uptake of radioactivity into various parts of spinal cord corresponds well to their relative content in grey matter. 6. The pharmacokinetic behaviour of 125I-toxoid resembles that of toxin. However, in order to get measurable fixation to the CNS at least 50 times higher amounts are to be applied. It is concluded that the barrier between blood and CNS is practically impermeable to tetanus toxin. The results can be harmonized best with the assumption that generalized tetanus is nothing else than a multiple local tetanus.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00499887

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Histoautoradiographic localisation of 125I-labeled tetanus toxin in rat spinal cord (1973)

Dimpfel, W. ; Habermann, E.

Springer

Naunyn-Schmiedeberg's archives of pharmacology 280 (1973), S. 177-182

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ISSN: 1432-1912

Keywords: Tetanus Toxin ; Iodine Labeling ; Spinal Cord ; Histoautoradiography

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 125I-labeled tetanus toxin was injected intravenously and intramuscularly in rats. Specific localisation within the spinal cord was obtained by histoautoradiography. 1. In generalized tetanus grain density was maximal in the ventral grey matter of spinal cord. The grains were closely correlated to the motoneurons and their neuropil. Other areas showed background activity only. 2. In local tetanus the injected side was labeled selectively. High grain density regularly covered a distinct group of motoneurons and their neuropil. 3. There is some evidence for intracellular accumulation of the toxin since the maximum of grain density was found over the perikarya whilst the nucleus corresponded to a minimum. 4. Cells yielding high grain density were less intensively stained with toluidine blue than neighbouring unlabeled cells. It is concluded from these experiments that tetanus toxin develops its action within or around selected motoneurons and that it induces morphological alterations there.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00499178

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Distribution of 125I-tetanus toxin and 125I-toxoid in rats with local tetanus, as influenced by antitoxin (1972)

Habermann, E.

Springer

Naunyn-Schmiedeberg's archives of pharmacology 272 (1972), S. 75-88

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ISSN: 1432-1912

Keywords: Tetanus Toxin ; Tetanus Antitoxin ; Local Tetanus ; Spinal Cord

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 0 1. Local tetanus was produced in rats by application of sublethal doses of 125I-tetanus toxin into the right m. gastrocnemius. Radioactivity was found in the lumbar part of the spinal cord for at least 24 days which is indicative of a long-lasting binding of toxin to its target organ. Radioactivity appears in the lumbar region before local tetanus becomes manifest. 2. The influence of antitoxin on both local tetanus and radioactivity of the lumbar cord heavily depends on the time of its application. When it is injected simultaneously into a foreleg, it prevents the symptoms and the spinal concentration process. When given ten hours after toxin, it does not change appreciably the severity of local tetanus; it diminishes, however, the radioactivity accumulating in the spinal cord. Antitoxin, given 48 hours after toxin, is ineffective in both respects. 3. 22 hours after application, about 9% of the initial radioactivity still persists in the injected leg; 50 hours after application, only 1–2% are still present. 4. Plasma radioactivity is measurable for between 50 and 96 hours in animals given 125I-toxin i.m. It is higher in animals having received antitoxin 10 hours after the toxin or simultaneously with toxin. 5. Labelled toxoid was prepared by formol treatment of labelled toxin. Following i.m. injection, toxoid was bound to a lesser degree and for a shorter time by the lumbar cord than was toxin. Like toxin, toxoid was found in the ipsilateral sciatic nerve, and simultaneous application of antitoxin prevented its appearance there as wells as in the lumbar cord. As with toxin, plasma radioactivity after injection of labelled toxoid was increased by simultaneous application of antitoxin into another leg. 6. It is concluded that antitoxin prevents the entrance of toxin into the spinal cord, but does neither remove nor detoxify appreciable amounts of radioactive material once fixed.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00498795

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