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Radiation inactivation analysis of the binding of the A1 adenosine receptor antagonist, 8-cyclopentyl-1,3-dipropylxanthine to rat brain membranes yielded a radiation inactivation size of 58 kDa. In the presence of GTPyS this was reduced to 33 kDa, in good agreement with the size of the ligand-binding subunit detected after photoaffinity labelling. The data indicate that the structural association of A\(_1\) adenosine receptors with G-protein components is altered in situ in the presence of guanine nucleotides.
1 Adenosine and its metabolically stable analogue N.etbyl-carboxamidoadenosine (NECA) enhance histamine release from rat peritoneal mast cells when tbese are stimulated by calciummobilizing agents. NECA and adenosine shift the concentration-response curve of tbe calcium ionophore A23187 to lower concentrations. 2 The potencies of NECA or adenosinein enhancing A23187-induced histamine release are dependent on the Ievel of stimulated release in tbe absence of adenosine analogues. At high Ievels of release their potencies are up to 20 times higher than at low Ievels. Consequently, averaged concentration-response curves of adenosine and NECA for enhancing bistamine release are shallow. 3 The adenosine transport blocker S-(p-nitrobenzyl)-6-thioinosine (NBTI) has no effect by itself at low Ievels of stimulated histamine release, but abolishes the enhancing effect of adenosine. At high Ievels of release, however, NBTI alone enhances the release of histamine. 4 lt is concluded that adenosine and calcium reciprocally enhance the sensitivity of the secretory processes to the effects of the other agent. The Ievels of intracellular adenosine obtained by trapping adenosine inside stimulated mast cells are sufficient to enhance histamine release substantially, suggesting that this effect may play a physiological and pathophysiological role.
The tritiated analogue of 2-chloro-N6-cyclopentyladenosine (CCPA), an adenosine derivative with subnanomolar affinity and a 10000-fold selectivity for A1 adenosine receptors, has been examined as a new agonist radioligand. [3H]CCP A was prepared with a specifi.c radioactivity of 1.58 TBqjmmol ( 43 Ci/mmol) and bound in a reversible manner to A1 receptors from rat brain membranes with a high affinity K0 -value of 0.2 nmol/1. In the presence of GTP a K0 -value of 13 nmol/1 was determined for the low affinity state for agonist binding. Competition of several adenosine receptor agonists and antagonists for [3H]CCPA binding to rat brain membranes confrrmed binding to an A1 receptor. Solubilized A1 receptors bound [3H]CCPA with similar affinity for the high affinity state. At solubilized receptors a reduced association rate was observed in the presence of MgC12, as has been shown for the agonist [ 3H]N6-phenylisopropyladenosine ([3H]PIA). [3H]CCPA was also used for detection of A1 receptors in rat cardio myocyte membranes, a tissue with a very low receptor density. A K0 -value of 0.4 nmol/1 and a Bmax-value of 16 fmol/ mg protein was determined in these membranes. In human platelet membranes no specific binding of [3H]CCPA was measured at concentrations up to 400 nmoljl, indicating that A2 receptors did not bind [3H]CCPA. Based on the subnanomolar affinity and the high selectivity for A1 receptors [ 3H]CCPA proved to be a useful agonist radioligand for characterization of A 1 adenosine receptors also in tissues with very low receptor density.
In the present work we studied the pharmacological profile of adenosine receptors in guinea pig atria by investigating the effect of different adenosine analogues on 86Rb + -efflux from isolated left atria and on binding of the antagonist radioligand 8-cyclopentyl-1 ,3-[\(^3\)H]dipropylxanthine ([\(^3\)H]DPCPX) to atrial membrane preparations. The rate of \8^{86}\)Rb\(^+\) -effiux was increased twofold by the maximally effective concentrations of adenosine receptor agonists. The EC50-values for 2-chloro-N\(^6\)-cyclopentyladenosine (CCPA), R-N\(^6\)-phenylisopropyladenosine (R-PIA), 5'-Nethylcarboxamidoadenosine (NECA), and S-N\(^6\)-phenylisopropyladenosine (S-PIA) were 0.10, 0.14, 0.24 and 12.9 \(\mu\)M, respectively. DPCPX shifted the R-PIA concentration-response curve to the right in a concentration-dependent manner with a K\(_B\)-value of 8.1 nM, indicating competitive antagonism. [\(^3\)H]DPCPX showed a saturable binding to atrial membranes with a Bmax·value of 227 fmol/mg protein and a K\(_D\)-value of 1.3 nM. Competition experiments showed a similar potency for the three agonists CCPA, R-PIA and NECA. S-PIA is 200 times less potent than R-PIA. Our results suggest that the K\(^+\) channel-coupled adenosine receptor in guinea pig atria is of an A\(_1\) subtype.
Polymorphonuclear leukocyte (PMNL) infiltration is an important characteristic in psoriatic lesions. Elevated concentrations of the chemoattractant eicosanoid leukotriene B4 (L TB4) are present in psoriatic skin. Its chemotactic activity is mediated via high affinity receptors on PMNL. The goal of our work was to ascertain whether PMNL infiltration in psoriasis can be accounted for by functional abnormalities of the circulating PMNL due to alterations in the LTB4 receptor density or affinity (or both). No significant difference was found between patients with psoriasis, healthy controls and patients with another inflammatory dermatosis (atopic eczema) with regard to the binding parameters of LTB4 receptors on PMNL. Our findings suggest that PMNL accumulation in psoriatic skin may be the result of an excess of cutaneous hemoattractant rather than the increased readiness of psoriatic PMNL to migrate towards L TB4 due to altered LTB4 receptor density or affinity.
The diet contains a large number of constituents which can be nitrosated in the gastrointestinal tract (especially in the stomach) to potentially carcinogenic nitroso compounds (NOC). The nitrosation of food mixtures has been investigated with a number of assays, such as chemical analysis or detection of alkylating potential, mutagenicity and carcinogenicity. Relatively good information is available on the formation of stable nitrosamines using high nitrite concentrations. Little is known, however, about the formation of chemically unstable NOC at low nitrite concentration and their genotoxicity in target cells. A comparison of the precursor classes, alkylamines, aromatic amines, amino acids, amides and peptides, ureas and guanidines, reveals a vast range, both with respect to daily intake (105-fold) and nitrosation rate (104-fold both for 1st and 2nd order nitrite dependence). A total span of 108 results for the relative yield of NOC in the stomach. The endogenous NOC burden from dietary ureas and aromatic amines may represent as large a hazard as the intake of preformed NOC. Recent evidence also indicates that heterocyclic amines and phenols must be considered and that the half-life of nitrosated a-amino acids can be much longer than that of nitrosated primary alkylamines. In these classes, more information should be collected on dietary concentrations, on the nitrosation under realistic conditions and on the genotoxicity in stomach lining cells. Within a chemical precursor class, a wide range is seen with respect to alkylating potency. It cannot, therefore, be excluded that individual precursors within the top ranking classes might become more important than single preformed NOC. Not considered in the above analysis but probably just as important for a risk evaluation in a population is the knowledge of the nitrosation conditions and target cell susceptibility in individuals.
Neoplastic cell transfonnation induced by estrogens and some other carcinogen& such as benzene appears to involve the induction of mitotic aneuploidy rather than DNA damage and point mutations. As metabolic activation may also play an important roJe in the mechanism of carcinogenesis of these nongenotoxic compounds, we have studied the Interaction of reactive quinone metabolites of various estrogens and of benzene with the major microtubular protein, tubulin, in a cell-free system. Covalent binding of the radioactively labeled metabolites to the a- and 13-subunit of tubulin was found to depend on the structure of the metabolite. When the adducted tubulins were tested in vitro for their ability to polymerize to microtubules, Inhibition of microtubule assembly was obsened in every case, although to varying extents. It is proposed that the fonnation of covalent tubulin adducts may impair the formation of mitotic spindies and thus contribute to chromosomal nondisjunction and aneuploidy induction.
Ethyl carbamate is found in fermented foods: bread contains 3-15 ng/g, stone-fruit brandies 200-20,000 ngfg, and about one-third of table-wine samples analysed contained more than 10 ng/g. In animals, ethyl carbamate is degraded to C02, H20 and NH3, with intermediate formation ofethanol. This degradation has been shown tobe inhibited (postponed) in the mouse by ethanol concentrations in the blood of about 0.15% and higher. A quantitatively minor pathway involves a two-step oxidation of the ethyl group to vinyl carbamate and epoxyethyl carbamate, the postulated electrophilic moiety that reacts with DNA. This reaction is probably the mode of the mutagenic action observed in many cellular and animal systems. The fact that only vinyl carbamate, but not ethyl carbamate, is mutagenic in a standard Ames test is probably because there is insufficient production of the intermediate oxidation product in the standard test. Consistent with this metabolism is the carcinogenic activity of ethyl carbamate in various animal species and in different organs; this activity can be seen even after a single high dose in early life. Quantitative analysis of the total tumour incidences after chronic exposure of rats and mice to 0.1-12.5 mg ethyl carbamate/kg body weightjday in the drinking-water showed a dose-related increase. The main target organs were the mammary gland (female rats and mice having similar susceptibilities) and the Jung (mice only). On the basis of sex- and organ-specific tumour data and with a linear extrapolation to a negligible increase of the lifetime tumour incidence by 0.0001% ( one additional tumour in one milüon individuals exposed for life), a "virtually safe dose .. of 20 to 80 ng/kg body weight/day was estimated. The daily burden reached under normal dietary habits without alcoholic beverages is in the range of about 20 ng/kg body weightfday. Regular table-wine consumption would increase the risk by a factor of up to five. Regular drinking of 20 to 40 ml stone-fruit brandy per day could raise the calculated lifetime tumour risk to near 0.01%.
Linear dose-response relationship for DNA adducts in rat liver from chronic exposure to aflatoxin B1
(1990)
Male F-344 rats were given eH]aßatoxin B1 (AFB1) in the drinking water at three exposure Ievels (0.02, 0.6, 20 J,Lgll, resulting in average dose Ievels of 2.2, 73, 2110 nglkg per day). After 4, 6 and 8 weeks, DNA was ~ted frorn the livers and analyzed for aßatoxin-DNA adducts. Tbe Ievel of DNA adducts did not increase significantly after 4 weeks, indicating that a steady-state for adduct formation and removal had nearly been reached. At 8 weeks, the adduct Ievels were 0.91, 32 and 850 nucleotide-aßatoxin adducts per to' nucleotides, i.e. clearly proportional to the dose. At the high dose Ievel, a near SO% tumor incidence would be expected in a 2-year bioassay with F -344 rats while the low dose used is within the range of estlmated human dietary exposures to aßatoxin in W estem countries. The proportionality seen between exposure and steady-state DNA adduct Ievel is discussed with respect to a linear extrapolation of the tumor risk to low dose.
Dose-response relationship and low dose extrapolation in chemical carcinogenesis [commentary]
(1990)
Data supporting various dose-respome relationships in chemical carcinogenesis are summarized. General principles are derived to explain the relationships between exposure dose, JI>NA adduct Ievel, induction of genetic changes, and tumor incidence. Some mechanistic aspects of epigenetic carcinogens (stimulation of ceU division and maldlfl'erentlation) are analyzed in a similar way. In a bomogeneous pnpulation, non-linearities are frequent. They are due to pbenomena of induction or saturation of enzymatic activities and to the multi-step nature of carcinog~: if a carcinogen acce1erates more than one step, the SUperposition of the dose- response curves for the indJvidual steps can result in an exponential relationship. A fourth power of the dose was the maximum seen in animals (fonnaldehyde). At the lowest dose Ievels, a proportionality between dose and tumor induction is postulated independent of the mechanism of action if the carcinogen aceeierotes the endogenous proass responsible for spootaneous tumor formation. Low-dose thresholds are expected only for situations where the carcinogen acts in a way that has no endogenous counterpart. Epidemiologfcal studies in humans show linear dose- response curves in all but two investigations. The difference from the strongly nonlinear slopes ·seen in animal studies could be due to the heterogeneity of the human population: if the individual sensitivity to a carcinogen is governed by a large number of genetic and Iife-style factors, the non-linea.rities will tend to cancel each other out and the dose- response curve becomes 'quasi-linear'.
Male rats were treated for 2 months with 1000 ppm nafenopin in the diet or for 4 or 7 days with a choline-devoid low-methionine diet. DNA was isolated from the livers and analyzed for the presence of cis-thymidine glycol-3'-phosphate (cis-dTGp) by 32P-postlabeling and for the Ievel of 8-hydroxy-deoxyguanosine (8-0H-dG) by electrochemical detection (ECD). In no DNA sample was the Ievel of cis-dTGp above the Iimit of detection of 1 modified thymidine per 106 nucleotides. With 8-0H-dG, a background Ievel of this modification of 20 8-0H-dG per 106 nucleosides was found in liver DNA of control rats, which was not affected by either treatment. It is postulated for thymidine glycol that a potential increase was below the Iimit of detection or was rapidly repaired in vivo and that the steady-state Ievel of endogenous 8-hydroxydeoxyguanosine appears not tobe influenced by the treatments chosen.
In a colorimetric assay using 4-( p-nitrobenzyl)pyridine (NBP) as a nucleophilic scavenger of alkylating agents, the nitrosation and alkylation reactions were investigated for a number of amino acids and derivatives. The alkylating activity increased with the square of the nitrite concentration. The nitrosation rate constants for aspartic acid, aspartame, and glycine ethylester ( = precursors C) were 0.08, 1.4 and ~ 0.2, respectively, expressed in terms of the pH-dependent \(k_2\) rate constant of the equation dNOCjdt = \(k_2\) • (C]· [nitrite]\(^2\) • The rates correlated inversely with the basicity of the amino group. The stability of the alkylating activity was astonishingly high, both in acid and at neutral pH. Half-lives of 500, 200, and 30 min were determined for aspartic acid (pH 3.5), aspartame (pH 2.5), and glycine ethylester (pH 2.5). Values of 60, 15, and 2 min; respectively, were found at pH 7. It is concluded that rearrangement of the primary N-nitroso product to the ultimate alkylating agent could be rate-limiting. The potential of nitrosated a-amino acids to bind to DN A in vivo was investigated by oral gavage of radiolabelled glycine ethylester to rats, followed irnmediately by sodium nitrite. DNA was isolated from stomach and liver and analysed for radioactivity and modified nucleotides. No indication of DNA adduct formation was obtained. Based on an estimation of the dose fraction converted from glycine ethylester to the nitroso product under the given experimental conditions, the maximum possible DNA-binding potency of nitroso glycine ethylester is about one order of magnitude below the methylating potency of N-nitrosomethylurea in rat stomach. The apparent discrepancy to the in vitro data could be due to efficient detoxification processes in mammalian cells.
A list ofendogenaus DNA·damaging agents and processes is given. Endogenaus e/ectrophiles are found with the cosubstrates of physiological transfer reactions (S-adenosylrnethionine for methylation, A TP for phosphorylation, NAD\(^+\) for ADP-ribosylation, acetyl CoA for acetylation). Aldehyde groups (glyceraldehyde- 3-phosphate, formaldehyde, open forms of reducing sugars, degradation products of peroxidation) or alkylating degradation products derived from endogenaus nitrose compounds represent additional possibilities. Radical-forming reactions include leakage of the superoxide anion radical from terminal cytochromes and redox cycles, hydroxyl radical formation by the Fenton reaction from endogenaus hydrogen peroxide, and the formation of lipid peroxides. Genetic instability by spontaneaus deaminations and depurinations as well as replicative instability by tautomer errors andin the presence of mutagenic metal ions represent a third important dass of endogenaus genotoxic processes. The postulated endogenaus genotoxicity could form the mechanistic basis for what is called 'spontaneous' tumor incidence and explain the possibility of an increased tumor incidence after treatment of animals with non-genotoxic compounds exhibiting tumor-promoting activity only. Individual differences are expected to be seen also with endogenaus DNA damage. The presence of endogenaus DNA darnage implies that exogenaus DNAcarcinogen adducts give rise to an incremental darnage which is expected to be proportional to the carcinogen dose at lowest Ievels. An increased tumor risk due to exposure to exogenaus genotoxic carcinogens could therefore be assessed in terms of the background DNA damage~ for instance in multiples of the mean Ievel or of the interindividual variability in a population.
The effects of guanine nucleotides on binding of 8-cyclopentyl-1,3-[\(^3\)H]dipropylxanthine [\(^3\)H]DPCPX), a highly selective A\(_1\) adenosine receptor antagonist, have been investigated in rat brain membranes and solubilized A\(_1\) receptors. GTP, which induces uncoupling of receptors from guanine nucleotide binding proteins, increased binding of [\(^3\)H]DPCPX in a concentration-dependent manner. The rank order of potency for different guanine nucleotides for increasing [\(^3\)H]DPCPX bindingwas the same as for guanine nuc1eotide-induced inhibition of agonist binding. Therefore, a role for a guanine nucleotide binding protein, e.g., G\(_i\), in the regulation of antagonist binding is suggested. This was confirmed by inactivation ofGi by N-ethylmaleimide (NEM) treatment of membranes, which resulted in an increase in [\(^3\)H]DPCPX binding similar to that seen with addition of GTP. Kinetic and equilibrium binding studies showed that the GTP- or NEM-induced increase in antagonist binding was not caused by an affinity change of A\(-1\) receptors for [\(^3\)H]DPCPX but by an increased Bmu value. Guanine nucleotides had similar effects on membrane-bound and solubilized receptors, with the effects in the solubilized system being more pronounced. In the absence of GTP, when rnost receptors are in a high-affinity state for agonists, only a few receptors are labeled by [\(^3\)H]DPCPX. It is suggested that [\(^3\)H]DPCPX binding is inhibited when receptors are coupled to G\(_i\). Therefore, uncoupling of A\(_1\) receptors from G\(_i\) by guanine nucleotides or by inactivation of G\(_i\) with NEM results in an increased antagonist binding.
Key Words: Adenosine receptors-8 -Cyclopentyl-1,3-eH]dipropylxanthine-Antagenist binding-Guanine nucleotide effects. Klotz K.-N. et al. Guanine nucleotide etfects on 8-cyclopentyl-1 ,3-eH]dipropylxanthine binding to membrane-bound and solubilized A1 adenosine receptors of rat brain. J. Neurochem. 54, 1988-1994 (1990).
Active neuropeptide Y receptors were solubilized from rabbit kidney membranes using the zwitterionic detergent 3-[ (3-cholamidopropy l)dimethylammonio ]- 1-propanesulfonic acid (CHAPS). In membrane fragmentsandsoluble extracts neuropeptide Y bindingwas time dependent, saturable, reversible, and of high affinity. Scatchard analysis of equilibrium binding data indicated a single class of binding sites with respective Kn and Bmax values of 0.09 nM and 530 fmol/mg of protein for the membrane-bound receptors and 0.10 nM and 1585 fmol/mg of protein for the soluble receptors. Neuropeptide Y bindingwas specifically inhibited by the nonhydrolyzable GTP analog guanosine 5' -0- (3-thiotripbosphate) in a concentration-dependent manner, with IC\(_{50}\) values of 28 and 0.14 \(\mu\)M for membrane- bound and soluble receptors, respectively, suggesting that neuropeptide Y receptors are functionally coupled to GTP-binding regulatory proteins. CrossHoking studies were performed with the heterobifunctional N-hydroxysuccinimidyl-4-azidobenzoate and the monofunctional neuropeptide Y derivative, azidobenzoyl and led to the identification of a 100 kDa peptide that should represent the covalently labeled neuropeptide Y receptor.
Ich habe versucht darzulegen, daß mechanistische Überlegungen zur Extrapolation der Dosis-WirkungsBeziehung herangezogen werden können. Ein nichtlinearer Verlauf ist nicht nur bei den epigenetischen Kanzerogenen wahrscheinlich, sondern auch bei den DNA-bindenden. Echte Schwellen sind aber nur in solchen Fällen zu erwarten, wo kein endogenes Korrelat besteht. Immerhin können auch steile Nichtlinearitäten zu einer drastischen Risikoreduktion führen, so daß die Anstrengungen dahin gehen sollten, die Steigung und den Bereich des überproportionalen Abfalls experimentell zu zeigen. In einer heterogenen Population kann die 0 0- sis-Wirkungs-Kurve zusätzliche "Wellen" bekommen und wird dadurch grundsätzlich flacher. Im Extremfall ergibt sich eine lineare Dosis-Wirkungs-Beziehung unabhängig vom Wirkmechanismus des Kanzerogens. Diese Proportionalität zwischen tiefster Dosis und Effekt wird bei genotoxischen Kanzerogenen aus mechanistischen Gründen schon für eine homogene Population postuliert, doch kann dies in einer heterogenen Population auch bei epigenetischen Kanzerogenen in Frage kommen.
In addition to hormonal activity, genetic darnage has been proposed as an important factor in oestrogen-mediated carcinogenesis. However, as short-term tests for oestrogens usually fail to show DNA mutations, lesions other than dassie nuclear DNA mutation have to be considered. Oestrogeninduced mitochondrial darnage was studied in the yeast Saccharomyces cerevisiae. Stilbene-type, but not steroidal, oestrogens were found to induce respiration-dcficient petite mutation. The effect was inversely correlated with cytotoxicity and required aromatic hydroxyl groups at the stilbene molecule. It only occurred under growth conditions and apparently was not due to the A TPase inhibitory qualities of stilbene oestrogens. Other studies have shown that petite mutation clones, which can be induced by a variety of substances, contain altered mitochondrial DNA. The mechanism of petite mutation induction might be important in tumorigenesis by also acting on nuclear DNA or facilitating carcinogenesis by disturbance of mitochondrial function.
The ~fthetic oes~rog~n diethylsti~boestrol (DES) causes a dose-dependent elevation of the cytoplasuuc Ca concentratton m C6 rat ghoma cells. This Ca2+ rise is caused neither by Ca2+ influx nor ~-r release from the ~a2 + stores of the endoplasmic reticulum. Therefore it seems likely that DES mob!hzes Ca2+ from a nutochondrial source. The DES-induced Ca2+ signal is remarkably similar to the one mduced by the. tumou~ promotor ~hapsigargin. As this compound causes leakage of calcium from the endoplasmt~ rettculum tt ~ms posstble that DES induces a similar leakage from mitochondrial Ca2+ stores. It remaans to be estabhshed whether the DES-mediated rise in intracellular calcium is causally related to the tumour-promoting properties of this compound
Rtgulatory aclio11s Iaken to reduu tht risk of harmfultffects of exposure to chemieals ofltn arenot commensurDtt with the toxicologicDf risk SJsstS&ment. A numbtr of factors relating to psychology, sociology, economics Dntl politics rather than science and medicine afftct tht final decision. Wemer Lutz and colleagues illustratt the situation using tht feuktmia-indudng chtmiCJJI benzene as an examplt.
Effect of inhalation exposure regimen on DNA binding potency of 1,2-dichloroethane in the rat
(1991)
1 ,2-Dichloroethane (DCE) was reported to be carcinogenic in rats in a long-tenn bioassay using gavage in com oil (24 and 48 mg/kg/day), but not by inhalation (up to 150-250 ppm, 7 h/day, 5 days/week). The daily dose metabolized was similar in the two experiments. In order to address this discrepancy, the genotoxicity of DCE was investigated in vivo under different exposure conditions. Fernale F-344 rats (183-188 g) were exposed to [1,2-14C]DCE in a closed inhalation chamber to either a low, constant concentration (0.3 mg/l = 80 ppm for 4 h) or to a peak concentration (up to 18 mg/1 = 4400 ppm) for a few minutes. After 12 h in the chamber, the dose metabolized under the two conditions was 34 mg/kg and 140 mg/k:g. DNA was isolated from liver and lung and was purified to constant specific radioactivity. DNA was enzymaticaBy hydrolyzed to the 3' -nucleotides which were separated by reverse phase HPLC. Most radioactivity eluted without detectable or with little optical density' indicating that the major part of the DNA radioactivity was due to covalent binding of the test compound. The Ievel of DNA adducts was expressed in the dose-nonnalized units ofthe Covalent Binding Index, CBI = f.Lmol adduct per mol DNA nucleotide/ mmol DCE per kg body wt. In liver DNA, the different exposure regimens resulted in markedly different CBI values of 1.8 and 69, for "constant-low" and ''peak" DCE exposure Ievels. In the Jung, the respective values were 0.9 and 31. It is concluded that the DNA darnage by DCE depends upon the concentration-time profile and that the carcinogenic potency determined in the gavage study should not be used for low-Ievel inhalation exposure.
The formation of \(O^6\)-methyldeoxyguanosine (\(O^6\)-MedGuo) was determined by an immuno-slot-blot assay in DNA of various tissues of F344 rats exposed to N-methyl-N-nitrosourea (MNU) in the drinking waterat 400 ppm for 2 weeks. Although the pyloric region of the glandular stomach is a target organ under these experimental conditions, the extent of DNA methylation was highest in the forestomach (185 \(\mu\)mol \(O^6\)-MedGuojmol guanine). Fundus (91 J.!moljmol guanine) and pylorus (105 J.!moljmol guanine) of the glandular stomach, oesophagus (124 \(\mu\)mol/mol guanine) and duodenum (109 )lmoljmol guanine) showed lower Ievels of \(O^6\) - MedGuo but differed little between each other. Thus, no correlation was observed between target organ specificity and the extent of DNA methylation. This is in contrast to the gastric carcinogen, N-methyl-N'-nitro-N-nitrosoguanidine (MNNG), which preferentially alkylates DNA of the pylorus, the main site of induction of gastric carcinomas by this chemical. In contrast to MNU, the nonenzymic decomposition of MNNG is accelerated by thiol compounds (reduced glutathione, L-cysteine), which are present at much higher concentrations in the glandular stomach than in the forestomach and oesophagus. During chronic exposure to MNNG (80 ppm), mucosal cells immunoreactive to 0 6-MedGuo are limited to the luminal surface [Kobori et al. (1988) Carcinogenesis 9:2271-2274]. Although MNU (400 ppm) produced similar Ievels of \(O^6\)-MedGuo in the pylorus, no cells containing methylpurines were detectable by immunohistochemistry, suggesting a more uniform methylation of mucosal cells by MNU than by MNNG. After a single oral dose of MNU (90 mg/kg) cells containing methylpurines were unequivocally identified using antibodies to \(O^6\)-MedGuo and the imidazole-ring-opened product of 7-methyldeoxyguanosine. In the gastric fundus, their distribution was similar to those methylated by exposure to MNNG, whereas the pyloric region contained immunoreactive cells also in the deeper mucosallayers. After a 2-week MNU treatment, the rate of cell proliferation, as determined by bromodeoxyuridine immunoreactivity, was only slightly enhanced in the oesophagus andin the fundus, but markedly in the forestomach and the pyloric region of the glandular stomach. lt is concluded that the overall extent of DNA methylation, the distribution of alkylated cells within the mucosa and the proliferative response all contribute to the organ-specific carcinogenicity of MNU.
Radioligand binding to A\(_1\) adenosine receptors at brain membranes from seven species was investigated. The antagonist 8-cyclopentyl-1 ,3-[\(^3\)H]dipropylxanthine ([\(^3\)H]DPCPX) bound with affinities between 0.17 nM in sheep brain and 2.1 nM in guinea pig brain. Competition of several antagonists for [\(^3\)H]DPCPX binding showed that the most potent compounds were DPCPX with K\(_i\) values of 0.05 nM in bovine brain and 1.1 nM in guinea pig brain and xanthine amine congener (XAC) with K\(_i\) values of 0.03 nM in bovine brain and 5.5 nM in guinea pig brain. The differences in affinity of the agonist radio Iigand 2-chloro-N\(^6\) -[\(^3\)H]cyclopen tyladenosine ([\(^3\)H]CCP A) were less pronounced, rauging from a K\(_D\) value of 0.12 nM (hamster brain) to 0.42 nM (guinea pig brain). Agonist competition for [\(^3\)H]DPCPX binding of photoaffinity labelling, however, exhibited marked species differences. N-Ethylcarboxamidoadenosine (NECA) and S-N\(^6\)-phenylisopropyladenosine (S-PIA) showed 20 to 25-fold different K\(_D\) values in different species. NECA had a particularly high affinity in guinea pig brain and was only two-fold less potent than R-PIA. Thus, the difference from the "classical" A\(_1\) receptor profile (R-PIA > -NECA > S-PIA) is not sufficient to speculate that A\(_1\) receptor subtypes may exist that are coupled to different effector systems. Our data show that these difference can easily be explained by species differences.
The mechanism of the therapeutic and prophylactic effects of carbamazepine (CBZ) in affective psychoses is unknown but may in part be related to the potent competitive interaction of CBZ with adenosine-binding sites in the brain. The antioonvulsant and sedative properties of CBZ are reminiscent of the effects evoked by adenosine-agonists and contrast sharply with the opposite aclions of adenosine-antagonists like caffeine. However. indirect evidence suggests an antagonist- rather than an agonist-like activity of CBZ at adenosi11e-receptors. We have used various model systems, in which adenosine receptor subtypes mediate different second messenger-responses, to investigate this apparent paradox. CBZ was found to antagonize the A\(_1\) receptor-mediated inhibition of cydic AMP accumulation in cultured astroblasts and in GH3-cells. Furthermore, CBZ also inhibits the adenosine-induced increase in the level of cyclic AMP in cultured astroblasts, which is mediated by low-affinity A\(_{2b}\)-receptors. ln contrast, CBZ does not block the inhibition elicited by adenosine-agonists of the agonist-induced increased formation of inositolphosphates in human neutrophils, which is mediated by high-affinity A\(_{2a}\)-receptors. The specific antagonism by CBZ of A\(_1\)- but not of high-affinity A\(_{2a}\)-receptors was further supported by binding experiments using rat brain membranes. These results suggest tbat the paradox of CBZ's antagonistic effects at adenosine-receptors might be at least partially reconciled by a selective antagonistic action of CBZ at A\(_1\)recertors but not at high-affinity A\(_{2a}\)-receptors.
It has previously been shown that covalent incorporation of the photoreactive adenosine derivative (R)-2-azido-N6-p-hydroxyphenytisopropyladenosine [(R)-AHPIA] into the A, adenosine receptor of intact fat cells leads to a persistent activation of this receptor, resulting in a reduction of celular cAMP Ieveis [Mol. Pharmacol. 30:403-409 (1986)]. In contrast, covalent incorporation of (R)-AHPIA into human platelet membranes, which contain only stimulatory A2 adenosine receptors, reduces adenytate cyclase Stimulation via these receptors. This effect of (R)-AHPIA is specific for the A2 receptor and can be prevented by the adenosine receptor antagonist theophylline. Binding studies in-dicate that up to 90% of A2 receptors can be blocked by photoincorporation of (R)-AHPIA. However, the remaining 10-20% of A2 receptors are sufficient to mediate an adenylate cyclase Stimulation of up to SOOk of the control value. Similarly, the activation via these 10-20% of receptors occurs with a halflife that is only 2 times Ionger than that in control membranes. This indicates the presence of a receptor reserve, with respect to both the extent and the rate of adenytate cyclase Stimulation. These observations require a modification of the models of receptor-adenytate cyclase coupling, which is described in the accompanying paper [Mol. Pharmacol. 39:524-530 (1991)].
Mechanistic possibilitles responsible for nonlinear shapes of the dose-response relationship in chemical carcinogenesis are discussed. (i) Induction and saturation of enzymatic activation and detoxification processes and of DNA repair affect the relationship between dose and steady-state DNA adduct Ievel; (ii) The fixation of DNA adducts in the form of mutations is accelerated by stimulation of the cell division, for Jnstance due to regenerative hyperplasia at cytotoxic dose Ievels; (iii) The rate of tumor formation results from a superposition of the rates of the individual steps. It can become exponential with dose if more than one step is accelerated by the DNA damage exerted by the genotoxic carcinogen. The strongly sigmoidal shapes often observed for dose-tumor incidence relationships in animal bioassays supports this analysis. A power of four for the dose in the su~linear part of the curve is the maximum observed (formaldehyde). In contrast to animal experiments, epidemiological data ln humans rarely show a slgnificant deviation from linearity. The discrepancy might be explained by the fact that a I arge nu mber of genes contribute to the overall sensitivity of an individual and to the respective heterogeneity within the human population. Mechanistic nonlinearities are flattened out in the presence of genetic and life-style factors which affect the sensitivity for the development of cancer. For a risk assessment, linear extrapolation from the high-dose lncidence to the spontaneaus rate can therefore be approprlate in a heterogeneous population even if the mechanism of action would result in a nonlinear shape of the dose-response curve in a homogeneaus population.
Tbe alkylating potency of unstable N-nitrosamino acids and N-nitrosopeptides was investigated in vitro using 4-(para-nitrobenzyl)pyridine (NBP) as nucleophile. Of the amino acids, Met and those with an aromatic side chain were the most potent. The relative overall alkylating potency was 23:10:5:4:2:1: for Trp, Met, His, 1)rr, Phe and Gly, respectively. The homo-dipeptides were much more potent than the amino acids, with relative potencies of 400:110:100:8:3:1, for Trp-Trp, l)T-'I)T, Met-Met, Asp-Asp, Phe-Phe and Gly, respectively. In the one-phase reaction system (in which NBP is already present durlog the nitrosation reaction at acidic pH), all amino acids tested showed a second-order reaction for nitrite. In the two-phase system (in which NBP is added only after bringing the nitrosation reaction mixture to neutrality), all amino acids tested except one again showed a second-order reaction for nitrite (Phe, His, Asp and the dipeptide artiticial sweetener aspartame); only Met under these conditions bad a reaction order of one for nitrite. This could mean that nitrosation of the side chain of Metproduces a second N-nitroso product which is relatively stable in acid but reacts with NBP under neutral conditions. In the human stomach, this side-chain nitrosation might become more important than the reactions at the primary amino group, firstly because of the greater stability of the product(s) in acid and secondly because of the tirst-order reaction rate for nitrite. A decrease in nitrite concentration from the millimolar concentrations ofthe in-vitro assay to the micromolar concentrations in the stomach reduces the reaction rate by a factor of 1000 for the side-chain nitrosation, whereas a million-fold reduction will be observed for nitrosation of the amino group.
lt is known that 5-azacytidine (5-AC) induces tumors in several organs of rats and mice. The mechanisms of these effects are still poorly understood although it is known that 5-AC can be incorporated into DNA. Furthermore, it can inhibit DNA methylation. The known data on its clastogenic andjor gene mutation-inducing potential are still controversial. Therefore, we have investigated the kinds of genotoxic effects caused by 5-AC in Syrian hamster embryo (SHE) fibroblasts. Three different endp6ints (micronucleus formation, unscheduled DNA synthesis (UDS) and cell transforrnation) were assayed under similar conditions of metabolism and dose at target in this cell system. 5-AC induces morphological transformation of SHE cells, but not UDS. Therefore, 5-AC does not seem to cause repairable DNA lesions. Furthermore, our studies revealed that 5-AC is a potent inducer of mkronuclei in the SHE system. Immunocytochemical analysis revealed that a certain percentage of these contain kinetochores indicating that 5-AC may induce both clastogenic events and numerical chromosome changes.
A\(_1\) adenosine receptors in coated vesicles have been characterized by radioligand binding and photoaflinity labelling. Saturation experiments with the antagonist 8-cyclopentyl-1 ,3-[\(^3\)H]dipropyl-xanthine ([\(^3\)H]DPCPX) gave a Kdvalue of 0.7 nM and a Bmax value of 82± 13 fmol/mg protein. For the highly A\(_1\)-selective agonist 2-chloro-N\(^6\)-[\(^3\)H]cyclopentyladenosine ([\(^3\)H]CCPA) a Kd value of 1.7 nM and a Bmax value of 72 ± 29 fmol/mg protein was estimated. Competition of agonists for [\(^3\)H]DPCPX binding gave a pharmacological profile with R-N\(^6\)-phenylisopropyladenosine (R-PIA) > CCPA > S-PIA > 5'-N-ethylcarboxamidoadenosine (NECA), which is identical to brain membranes. The competition curves were best fitted according to a two-site model, suggesting the existence of two affinity states. GTP shifted the competition curve for CCP A to the right and only one affinity state similar to the low affinity state in the absence of GTP was detected. The photoreactive agonist 2-azido-N\(^6\)- \(^{125}\)I-p-hydroxyphenylisopropyladenosine ([\(^{125}\)I]AHPIA) specifically labelled a single protein with an apparent molecular weight of 35,000 in coated vesicles, which is identical to A\(_1\) receptors labelled in brain membranes. Therefore, coated vesicles contain A\(_1\) adenosine receptors with similar binding characteristics as membrane-bound receptors, including GTP-sensitive high-affinity agonist binding. Photoaffinity labelling data suggest that A\(_1\) receptors in these vesicles are not a processed receptor fonn. These results confirm that A\(_1\) receptors in coated vesicles are coupled to a G-protein, and it appears that the A\(_1\) receptor systems in coated vesicles andin plasma membranes are identical.
The intake of known dietary carclnogens was compiled and the cancer risk was estlmated on the basis of carcinogenic potencies in animals as derived from the Carcinogenic Potency Database by Gold and co-workers. The total cancer risk was compared with the number of cancer cases attributed by epidemiologists to dietary factors (one-third of all cancer cases, i.e. -80 000 per one million Jives). Except for alcohol, the known dietary carcinogens could not account for more than a few bundred cancer cases. Tbis was seen both with tbe DNA-reactive carcinogens (beterocyclic aromatic amines, polycyclic aromatic hydrocarbons, N-nitroso compounds, estragole, aflatoxin B., ethyl carbamate, to name the most important factors) as wen as with those carclnogens wbich have not been shown to react with DNA (e.g. caffelc acid and the carcinogeruc metals arsenic and cadmium). Residues and contaminants turned out to be negligible. Among the various pmsibilities to explain the discrepancy we investigated the roJe of ovemutritlon. Dietary restriction in animals is weil known for its strong reducing effect on spontaneous tumor formation. These data can be used to derive a carcinogenic potency for excess macronutrients: tbe tumor incidence seen with the restrlcted animals is taken as a control value and the increased tumor incidence in the animals fed ad libitum is attributed to the additional feed iotake. For excess standard diet in rats, a carcinogenic potency TD50 of 16 glkg/day was deduced from a recent study. Ovemutrition in Switzerland, estimated to be 5.5 kcallkg/day, was converted to excess food (1.9 g/kg/day) and tbe cancer incidence was calculated. The result, 60 000 cancer cases per one million Jives, is provocatively close to the number of cases not explained by the known dietary chemical carcinogens. Mechanistic studies will be required to test our hypothesis and investigate the role of different types of macronutrients in ovemutrition.
Styrene-7,8-oxide (SO), the main intennediate metabolite of styrene, induces hyperkeratosis and tumors in the forestomach of rats and mice upon chronic administration by gavage. The aim of this study was to investigate wbether DNA binding could be responsible for the carcinogenic effect observed. [7-\(^3\)H]SO was administered by oral gavage in com oll to male CD rats at two dose levels (1.65 or 240 mg/kg). After 4 or 24 h, forestomach, glandular stomach and Uver were exclsed, DNA was isolated and its radioactivity detennined. At the 4 h time polnt, the DNA radioactivity was below the Iimit of detection in the torestornach and the liver. Expressed in the units of the covalent bindlng Index, CBI = (pmol adduct/mol DNA nucleotide)/(mmol cbemical administeredlkg body wt), the DNA-binding potency was below 2.6 and 2.0 respectively. In the glandular stomach at 4 b, and in most 24 b samples, DNA was slightly radiolabeled. Enzymatic degradation of the DNA and separation by HPLC ofthe normal nucleotides sbowed that the DNA rad.ioactivity represented biosynthetic incorporation of radlolabel into newly synthesized DNA. The Iimit of detection of DNA adducts in the glandular stomach was 1.0. In a second experlment, [7-\(^3\)H]SO was administered by i.p. injection to male 86C3Fl rnice. Liver DNA was analyzed after 2 h. No radloactivity was detectable at a Iimit of detection of CBI < 0.6. In agreement with the relatively long half-life of SO in animals, the cbemical reactivity of SO appears to be too low to result in a detectable production of DNA adducts in an in vivo situation. Upon comparison with the DNA-binding of other carcinogens, a purely genotoxic mechanism of tumorigenJc action of SO is unlikely. The observed tumorigenic potency in the forestomach could be the result of strong tumor promotion by high-dose cytotoxicity foUowed by regenerative hyperplasia.
Photoaffinity-labeled N-formyl chemotactic peptide receptors from human neutrophils solubilized in octyl glucoside exhibit two forms upon sucrose density gradient sedimentation, with apparent Sedimentation coefficients of approximately 4 and 7 S. Tbe 7 S form can be converted to the 4 S form by guanosine 5' -0- (3-thiotriphosphate) (GTP-yS) with an EC&o of -20 nM, suggesting that the 7 S form may represent a physical complex of the receptor with endogenous G protein (Jesaitis, A. J., Tolley, J. 0., Bokoch, G. M., and Allen, R. A. (1989) J. Cell Biol. 109, 2783-2790). To probe the nature of the 7 S form, we reconstituted the 7 S form from the 4 S form by adding purified G protein. The 4 S form, obtained by solubilizing GTP-yS-treated neutrophil plasma membranes, was incubated with purified (>95%) G. protein from bovine brain (containing both G\(_{ia1}\) and G\(_{ia2}\)) or with neutrophil G protein (G\(_a\)), and formation of the 7 S complex was analyzed on sucrose density gradients. The EC\(_{50}\) of 7 S complex formation induced by the two G proteins was 70 \(\pm\) 25 and 170 \(\pm\) 40 DM for G\(_a\) and G\(_1\), respectively. No complexation was measurable when bovine transducin (G\(_t\)) was used up to 30 times the EC\(_{50\) for G\(_a\). The EC\(_{50}\) for G\(_t\) was the same for receptors, obtained from formyl peptide-stimulated or unstimulated cells. The addition of 10 \(\mu\)M GTP-yS to the reconstituted 7 S complex caused a complete reversion of the receptor to the 4 S form, and anti-G\(_1\) peptide antisera immunosedimented the 7 S form. ADP-ribosylation of Gt prevented formation of the 7 S form even at 20 times the concentration of unribosylated G. normally used to attain 50% conversion to the 7 S form. These observations suggest that the 7 S species is a pbysical complex containing N-formyl chemotactic peptide receptor and G protein.
In the search for more selective A2-receptor agonists and on the basis that appropriate substitution at C2 is known to impart selectivity for A\(_2\) receptors, 2-alkynyladenosines 2a-d were resynthesized and evaluated in radioligand binding, adenylate cycla.se, and platelet aggregation studies. Binding of [\(^3\)H]NECA to A\(_2\) receptors of rat striatal membranes was inhibited by compounds 2a-d with K\(_i\) values ranging from 2.8 to 16.4 nM. 2-Alkynyladenosines also exhibited high-affmity binding at solubilized A\(_2\) receptors from human platelet membranes. Competition of 2-alkynyladenosines 2a-d for the antagonist radioligand [\(^3\)H]DPCPX and for the agonist [\(^3\)H]CCPA gave K\(_i\) values in the nanomolar range, and the compounds showed moderate A\(_2\) selectivity. In order to improve this selectivity, the correaponding 2-alkynyl derivatives of adenosine-5'-N-ethyluronamide 8a-d were synthesized and tested. A\(_1\) expected, the 5'-N-ethyluronamide derivatives retained the A\(_2\) affinity whereas the A\(_1\) affinity was attenuated, resulting in an up to 10-fold increase in A\(_2\) selectivity. A similar patternwas observed in adenylate cyclase assays andin platelet aggregation studies. A 30- to 45-fold selectivity for platelet A\(_2\) receptors compared to A\(_1\) receptors was found for compounds 8a-c in adenylate cyclase studies.
Reduction of postischemic leukocyte-endothelium interaction by adenosine via A\(_2\) receptor
(1992)
The adhesion of leukocytes to the endothelium of postcapillary venules hallmarks a key event in ischemia-reperfusion injury. Adenosine has been shown to protect from postischemic reperfusion injury, presumably through inhibition of postischemic leukocyte-endothelial interaction. This study was performed to investigate in vivo by which receptors the effect of adenosine on postischemic leukocyte-endothelium interaction is mediated. The hamster dorsal skinfold model and fluorescence microscopy were used for intravital investigation of red cell velocity, vessel diameter, and leukocyte-endothelium interaction in postcapillary venules of a thin striated skin muscle. leukocytes were stained in vivo with acridine orange (0.5 mg kg\(^{-1}\) min\(^{-1}\) i.v. ). Parameters were assessed prior to induction of 4 h ischemia to the muscle tissue and 0.5 h, 2 h, and 24 h after reperfusion. ·Adenosine, the adenosine A1-selective agonist 2-chloro-N\(^6\) -cyclopentyladenosine (CCPA), the Arselective agonist CGS 21,680, the non-selective adenosine receptor antagonist xanthine amine congener {XAC), and the adenosine uptake blocker S-(p-nitrobenzyl)-6-thioinosine (NBTI) were infused viajugular vein starting 15 min priortorelease of ischemia until 0.5 h after reperfusion. Adenosine and CGS 21,680 significantly reduced postischemic leukocyte-endothelium interaction 0.5 h after reperfusion (p< 0.01), while no inhibitory effect was observed with CCPA. Coadministration of XAC blocked the inhibitory effects of adenosine. Infusion of NBTI alone effectively decreased postischemic leukocyte-endothelium interaction. These findings indicate that adenosine reduces postischemic leukocyte-endothelium interaction via A\(_2\) receptor and suggest a protective role of endogenous adenosine during ischemia-reperfusion.
We have previously reported that in several renal cell types, adenosine receptor agonists inhibit adenylyl cyclase and activate phospholipase C via a pertussis toxin-sensitive G protein. In the present study, in 28A cells, both uf these adenosine receptor-mediated responses were inhibited by 8-cyclopentyl-1,3-dipropylxanthine (DPCPX). a highly selective A1 adenosine receptor antagonist. The binding characteristics of the adenosine A 1 receptor in the 28A renal cell line were studied using the radiolabeled antagonist f:1H]DPCPX to determine whether two separate binding sites could account for these responses. Saturation binding of [: 1H]DPCPX to 28A cell membranes revealed a single class of A1 binding sites with an apparent Kd value of 1.4 nM and maximal binding capacity of 64 fmol/mg protein. Competition experiments with a variety of adenosine agonists gave biphasic displacement curves with a pharmacological profile characteristic of A1 receptors. Comparison of [: 1H]DPCPX competition binding data from 28A cell membranes with rabbit brain membranes, a tissue with well-characterized A1 receptors, reveals that the A 1 receptor population in 28A cells has similar agonist binding affinities to the receptor population in brain but has a considerably lower density. Addition of guanosine ;)' -triphosphate ( 100 ,uM) to 28A cell membranes caused the competition curves to shift from biphasic to monophasic. indicating that the A1 receptors exist in two interconvertible affinity states because of their coupling to G proteins. In the absence of evidence for subpopulations of the A1 receptor, it appears that in 28A cells. A single A1 receptor population. As defined by ligand binding characteristics, couples via one or more pertussis toxin-sensitive guanine nucleotide binding proteins to two different biological signaling mechanisms.
Some chromosomes in transformed rat cells and somatic cell hybrids fail to display the presence of kinetochore proteins as detected by antikinetochore antibodies. Suchchromosomes (K- Chromosomes) may constitute a novel mechanism for the genesis of aneuploidy. Wehave analyzed primary~ immortalized and malignant marnmalian cells for the presence of kinetochore proteins and micronuclei. Our resuJts suggest a correlation of the K- chromosome and micronucleus frequency with the variability in chromosome number. Upon in situ hybridization with the minor satellite and alpha satellite sequences some Kchromosomes showed a signal. This indicates that the observed lack of kinetocbores is not necessarily due to a lack of centromeric DNA. We conclude that dislocated K- chromosomes may become incorporated into micronuclei which are prone to loss. Such events would be associated with the generation of aneuploidy.
Tbe benzodiazepines are a class of d.rugs that are widely used in the treatment of various psychiatric disorders. One member of um ~' oxazepam, is also a common metabolite of sevmd other benzod.iazepines. Since the evidence for the genetic toxicity and carcinogenic properties of these compounds is incol:lsb1ent, we investigated the oxazepam-induced fonnation of micronuclei in Syrian Hamster embryo fibroblast (SHE) cells, human amniotic fluid fibroblast-like (AFFL) cells and LS178Y mouse cells. A dose-dependent increase in micronucleus fractions was found in all tbree ceU llnes. The time course of micronucleus induction in L5178Y cells showed a maximum at 5 h after treatment, suggesting that the micronuclei were fonned in the first mitosis after treatment. Kinetochore staining (CREST -antiserum) revealed the presence of kinetochores in -SO% of the micronuclei in aU tbree ceU types. ThJs resu1t was further confinned by in situ bybridization in LS178Y cells and indicates tbe presence of wbole Chromosomes or centric fragments as weU as acentric fragments in the oxazepam-induced micronuclei. The LS178Y cells did not show a mutagenic response to oxazepam at any of the doses or expression times used.
5-Azacytidine was originally developed to treat human myelogenous leukemia. However, interest in this compound has expanded because of reports of its ability to affect cell differentiation and to alter eukaryotic gene expression. In an ongoing attempt to understand the biochemical effects of this compound, we examined the effects of 5-azacytidine on mitosis and on micronucleus formation in mammalian cells. In L5178Y mouse cells, 5-azacytidine induced micronuclei at concentrations at which we and others have already reported its mutagenicity at the tk locus. Using CREST staining and C-banding studies, we showed that the induced micronuclei contained mostly chromosomal fragments although some may have contained whole chromosomes. By incorporating BrdU into the DNA of SHE cells, we determined that micronuclei were induced only when the compound was added while the cells were in S phase. Microscopically visible effects due to 5-azacytidine treatment were not observed until anaphase of the mitosis following treatment or thereafter. 5-Azacytidine did not induce micronuclei via interference with formation of the metaphase chromosome arrangement in mitosis, a common mechanism leading to aneuploidy. SupravitalUV microscopy revealed that chromatid bridges were observed in anaphase and, in some cases, were sustained into interphase. In the first mitosis after 5-azacytidine treatment we observed that many cells were unable to perform anaphase separation. All of these observations indicate that 5-azacytidine is predominantly a clastogen through its incorporation into DNA.
1.2-Dioxetanes, very reactive and high energy molecules. are involved as labile intermediates in dioxygenase- activated aerobic metabolism and in physiological processes. Various toxico1ogica1 tests reveal that dioxetanes are indeed genotoxic. In supercoiled DNA of bacteriophage PM2 they induce endonucleasesensitive sites, most of them are FPG protein-sensitive base modifications (8-hydroxyguanine, fonnamidopyrimidines). Pyrimidinedimersand sites ofbase loss (AP sites) which were probed by UV endonuclease and exonuclease 111 are minor lesions in this system. While the alky1-substituted dioxetanes do not show any significant mutagenic activity in different Salmonella typhimurium strains, heteroarene dioxetanes such as benzofuran and furocoumarin dioxetanes are strongly mutagenic in S. typhimurium strain TA I 00. DNA adducts formed with an intermediary alkyJating agent appear to be responsible for the mutagenic activity of benzofuran dioxetane. We assume that the benzofuran epoxides, generated in situ from benzofuran dioxetanes by deoxygenation are the ultimate mutagens of the latter. since benzofuran epoxides are highly mutagenic in the S. typhimurium strain TAIOO and they form DNA adducts. as detected by the 212Ppostlabelling technique. Our results imply that the type of D NA darnage promoted by dioxetanes is dependent on the structural feature of dioxetanes. Furthermore, the direct photochemical DNA darnage by energy transfer. i.e., pyrimidine dimers, plays a minor role in the genotoxicity of dioxetanes. Instead, photooxidation dominates in isolated DNA. while radical darnage and alkylation prevail in the cellular system.
When human neutrophils become desensitized to formyl peptide chemoattractants, the receptors (FPR) for these peptides are converted to a high affinity, GTP-insensitive form that is associated with the Triton X-1 00- insoluble membrane skeleton from surface membrane domains. These domains are actin and fodrin-rich, but G protein-depfeted suggesting that FPR shuttling between G protein-enriched and depleted domains may control signal transduction. Todetermine the molecular basis for FPR interaction with the membrane skeleton, neutrophil subcellular fractions were screened for molecules that could bind photoaffinity-radioiodinated FPR solubilized in Triton X-1 00. These receptors showed a propensity to bind to a 41- to43-kDa proteinband on nitrocelluloseoverlays of SOS-PAGE-separated cytosol and plasma membrane fractions of neutrophils. This binding, as weil as FPR binding to purified neutrophil actin, was inhibited 50% by 0.6 \(\mu\)M free neutrophil cytosolic actin. Addition of greater than 1 \(\mu\)M G-actin to crude or lectin-purified Triton X-1 00 extracts of FPR from neutrophil membranes increased the sedimentationrate of a significant fraction of FPR two to three fold as measured by velocity sedimentation in Triton X-1 00-containing linear sucrose density gradients. Addition of anti-actin antibodies to FPR extracts caused a concentration-dependent immunoprecipitation of at least 65% of the FPR. More than 40% of the immunoprecipitated FPR was specifically retained on protein A affinity matrices. Membrane actin was stabilized to alkaline washing when membranes were photoaffinity labeled. Conversely, when purified neutrophil cytosolic actinwas added to membranes or their digitonin extracts, after prior depletion of actin by an alkaline membrane wash, photoaffinity labeling of FPR was increased two- to fourfold with an EC\(_{50}\) of approximately 0.1 \(\mu\)M actin. We conclude that FPR from human neutrophils may interact with actin in membranes to form Triton X-1 00-stable physical complexes. These complexes can accept additional G-actin monomers to form higher order molecular complexes. Formation of FPR-actin complexes in the neutrophil may play a role in the regulation of chemoattractantinduced activation or actin polymerization.
The question addressed was whether Stimulation of cell proliferation could be responsible for tumor induction in the torestornach by styrene 7,8-oxide (SO). Male F344 rats were treated for 4 weeks with 0, 137,275, and 550 mglkg SO by p.o. gavage 3 times/week. Positive controls received 0, 0.5, I, and 2% butylated hydroxyanisole (BHA) in the diet for 4 weeks. Twenty-four h before termination of the experlment, the rats were implanted s.c. with an osmotic minipump deliverlog S-bromo-2'-deoxyuri· dine (BrdU). Cell proliferation in the forestomach was assessed by immunohistochemistry for BrdU incorporated into DNA. Cell number/mm section length and fraction of replicating cells (labeling Index) were determined in 3 domains of the forestomach, the saccus caecus, the midregion, and the prefundic region. With the exception of the prefundic reglon of the low-dose SO group, a significant increase of the labeling index was found in all regions both with SO and BHA. Rats treated with BHA showed, in addition, a dose-dependent increase in number and size of hyperplastic lesions. This was most pronounced in the prefundic region where carcinomas were reported to be localized. In this region, the number of dividing cells/mm section length was increased up to 17-fold. With SO, only marginal morphological changes were occasionally observed, despite the fact that the respective long-term treatment bad been reported to result in a higher carcinoma incidence than treatment with BHA. It ls concluded that the rate of replicating cells alone, numerically expressed by the labeling Index, is an lnsufficient tool for interpretlog the role of cell division in carcinogenesis. It is postulated that SO and BHA induce forestomach tumors via different mechanisms. While hyperplasia in the prefundic region most likely dominates the carcinogenicity of BHA, a mechanism combining marginal genotoxicity with strong promotion by increased cell proliferation appears to be involved in the tumorigenic action of SO.
'lbe mouse skin tumor model was used to investigate whether the Ievel of DNA 8dducts and/or the rate of cell division in the epidermis are indicators of the risk of cancer formation for an individual in an outbred animal popul8tion. A high risk was considered to be reftected by 8 short latency period for the 8ppearance of 8 papilloma. Fernale NMRI mice were treated twice weekly with 2.5 nmol 7 ,12-dimethylbenz[a]antbracene (DMBA) and 3 nmoi12-0-tetradecanoylphorbol-13- 8cetate (TPA) and the appearance of papillomas was registered. The first papilloma 8ppeared after 7.5 weeks. After 17 weeks, when 12 of 14 mice bad 8t least one papilloma, an osmotic minipump deliverlog 5-bromo-2'deoxyuridine (BrdU) was implanted into eacb mouse for 24 h. The mice were killed after 24 h ~d the epidermis was analyzed for D:MBA-nucleotide 8dducts by 32p.postlabeling, for the cell number per unit skin length, and for the labeling index for DNA synthesls. Unexpectedly, D:MBA-nucleotide 8dduct Ievels were highest in those anima1s wbich showed the Iongest latency periods. Adduct Ievels were negatively correlated with the 18beling index, indicating that dilution of adducts by cell division was a predominant factor in determining average adduct concentrations. Individual tumor-latency time was not corTelated with either cell ntunber or labeling index. This could be due to the fact that the measurements only provided 8veraged data and gave no infonnation on the specific situation in clones of premalignant cells. Under the conditions of tbis assay, therefore, neither DNA adduct Ievels nor information on the average kinetics of cell division bad a predidive value for the individual amcer risk withln a group of outbred animals receiving the same treatment
2-Acetylaminofluorene (2-AAF) was administered at Ievels of 0, 300 and 600 ppm in the diet for 28 days to female transgenic micc bearing the lacl genein a Iambda vector (Big Blue® mice). The Iambda vector was excised from liver DNA and packaged in vitro into bacteriophage particles which were allowed to infect E. coli bacteria, forming plaques on agar plates. Approximately 10\(^5\) plaques wcre screened per animal for the appearance of a bluc colour, indicative of mutations in the lac/ gcnc which had resulted in an inactive gene product. Background mutation rate was 2.7 x 10\(^{-5}\) (pooled results of two animals, 8 mutant plaques/289 530 plaques). At 300 ppm in the diet, the rate of 3.5 X 10\(^{-5}\)(8/236 300) was not significantly increased over background. At 600 ppm in the dict, the rate increased approximately 3 fold to 7.7 x 10\(^{-5}\) (17 /221240). In comparison to the usual single or 5-day carcinogen exposure regimes, the 4-week exposure protocol allowed the use of much lower dose Ievels 00-1000 fold lower). Overt toxicity could thus be avoided. The daily doses used were somewhat higher than those required in 2-year carcinogenicity studies with 2·AAF.
Signal transduction via receptors for N-formylmethionyl peptide chemoattractants (FPR) on human neutrophils is a highly regulated process. It involves direct interaction of receptors with heterotrimeric G-proteins and may be under thc control of cytoskeletal clemcnts. Evidencc exists suggesting that thc cytoskeleton and/or the membrane ske1eton determines the distribution of FPR in the plane of the plasma membrane, thus controlling FPR accessibility to different protcins in functionally distinct membrane domains. In desensitized cells, FPR are restricted to domains which are depleted of G proteins but enriched in cytoskeletal proteins such as actin and fodrin. Thus, the G protein signal transduction partners of FPR become inacccssible to the agonist-occupied receptor, preventing cell activation. We are investigating the molecular basis for the interaction of FPR with the membrane skeleton, and our results suggest that FPR, and possibly other receptors, may directly bind to cytoskeletal proteins such as actin.
Diethylstilbestrol alters the morphology and calcium levels of growth cones of PC12 cells in vitro
(1993)
Diethylstilbestrol (DES) is a synthetic estrogen with carcinogenic properties. DES is known to alter cytoskeletal components, including the organization of actin stress fibres in C6 rat glioma cells. ln a test of the hypothesis that DES disrupts actin Filaments of growth cones in neuron-like cells, DES-induced changes in filopodial lengths were quantified in rat pheochromocytoma (PC12) cells in vitro. DES significantly altered growth cone morphology, with collapse of growth cone filopodia and neurite retraction invariably occurring at a concentration of 10 MikroM. At 5 MikroM DES, transient reductions in total filopodiallengths occurred. At DES concentrations of 0.1 nM and 1 nM, reductions in total filopodiallengths occurred in a fraction of growth cones. Evidence exists which shows that growth cone activity and morphology are intimately linked to Ieveis of intracellular, free calcium and that DES increases such levels. Measurements of free intracellular calcium levels by fluorescence microscopy, at times concurrent with the DES-induced reduction in total filopodial lengths, showed that calcium levels were indeed significantly increased by 10 MirkoM DES. Labelling of filamentaus actin (f-actin) with FITC-phalloidin showed that the f-actin distribution in growth cones exposed to DES could not be differentiated from the distribution found in spontaneously retracting growth cones. Tagether with evidence which showed that growth cone motility was not affected, the results are taken to indicate that DES, rather than acting directly on the cytoskeleton, exerts its effects indirectly, by a calcium-induced destabilization of actin filaments in the growth cone.
Wben irradiated at 360 nm, furocoumarins with a hydroperoxide group in a side chain effciently give rise to a type of DNA damage that can best be explained by a photoinduced generation of hydroxyl radicals from the excited pbotosensitizers. The observed DNA damage profiles, i.e. the ratios of single-strand breaks, sites of base loss (AP sites) and base modifications sensitive to fonnamidopyrimidine-DNA glycosylase (FPG protein) and endonuclease m, are similar to the DNA damage profile produced by hydroxyl radicals generated by lonizing radiation or by xanthine and xanthine oxidase in the presence of Fe(III)-EDTA. No such damage is observed with the corresponding furocoumarin alcohols or in the absence of near-UV radiation. The damage caused by the photo-excited hydroperoxides is not influenced by superoxide dismutase (SOD) or catalase or by D2O as solvent. The presence of t-butanol, however, reduces both the formation of single-strand breaks and of base odifications sensitive to FPG protein. The cytotoxicity caused by one of the hydroperoxides in L5178Y mome lymphoma cells is found to be dependent on the near-UV irradiation and to be much higher than that of the corresponding alcohol. Therefore the new type of photoinduced damage occurs inside cells. Intercalating photosensitizers with an attached hydroperoxide group might represent a novel and versatile class of DNA damaging agents, e.g. for phototherapy.
An improved 32P-postlabelling assay for detection and quantitation of styrene 7,8-oxide-DNA adducts
(1993)
Using DNA modified with [7-3H]styrene 7,8-oxide (SO) in vitro we have standardized the 32P-postlabelling assay for detecting SO-DNA adducts. Nuclease P 1-enriched adducts were 32P-labelled and purified by high-salt ( 4.0 M ammonium formate, pH 6.1} C1s reverse-phase TLC. After elution from the layer with 2-butoxyethanol:H20 (4:6), adducts were separated by two-dimensional PEI cellulose TLC in non-urea solvents (2.0 M ammonium formate, pH 3.5, and 2.7 M sodium phosphate, pH 5.6). One major, three minor and several trace adducts were detected. The efficiency of the kinase reaction depended on the ATP concentration. Use of standard labelling conditions (['Y· 32P]ATP, <3000 Ci/mmol; <2 Mikromol) resulted in poor ( 4-7%) adduct recovery. An ATP concentration of 40 Mikromol, however, increased the labeJling efficiency by a factor of 5-8 (35-55% based on 3H-SO labelied DNA). The results indicate that the new separation technique is suitable for the relatively polar SO-DNA adducts and that high labelling efficiency can be achieved.
[7-3H)Styrene 7,8-oxide was administered by oral gavage to male CD rats at a dose of 1.3 mg/kg. After 4 h, the forestomach was excised, DNA was isolated, purified to constant specific radioactivity and degraded nzymatically to the 3 '-nucleotides. Highperformance liquid chromatography fractions with the normal nucleotides contained most of the radiolabel, but a minute level of adduct label was also detccted. Using the units of the covalent binding index (micromoles adduct per mole DNA nucleotide)/(millimole chemical administered per kilogram body weight), a DNA binding potency of 1.0 was derived. A comparison of the covalent binding indices and carcinogenic potencies of other genotoxic forestarnach carcinogens showed that the tumorigenic activity of styrene oxide is unlikely to be purely genotoxic. Therefore, styrene oxide was compared with 3-tbutylhydroxyanisole (BHA) with respect to stimulation of cell proliferation in the forestomach. Male Fischer 344 rats were treated for four weeks at three dose levels of styrene oxide (0, 137, 275 and 550 mg/kg, three times per week by oral gavage) and BHA (0, 0.5, 1 and 2% in the diet); the highest doses had been reported to result in 84% and 22% carcinomas in the forestomach, respectively. Cell proliferation was assessed by incorporation of bromodeoxyuridine into DNA and immunohistochemical analysis. An increase in the lablling indexwas found in a11 treated animals. In the prefundic region of the forestomach, the labeHing index increased significantly, from 42% (controls) to 54% with styrene oxide and from 41 to 55% with BHA. Rats treated with BHA also had severe hyperplastic lesions in the prefundic region, i.e., at the location of BHA-induced forestomach carcinomas. The number of cells per millimetre of section length was increased up to 19 fold. Hyperplastic lesions were not seen with styrene oxide, despite the higher tumour incidence reported with this compound. We conclude that the carcinogenicity of styrene oxide to the forestomach most probably involves a mechanism in which marginal genotoxicity is combined with promotion by increased cell proliferation.
Known mutagens and carcinogens in the dict were compiled and the risk of cancer was estimated on the basis of average exposure Ievels in Switzerland and carcinogenic potencies from rodent bioassays. The analysis showed that, except for a1cohol, the sum of all known dietary carcinogens could only explain a few percent of the cancer deaths attributed by epidemiologists to dietary factors. The discrepancy was explained by a "carcinogenicity" of excess macronutrients. This hypothesis was based on an evaluation of dietary restriction experiments in rats and mice, where a dramatic reducing effect on spontaneaus tumour formation was seen. From these experiments, a "carcinogenic potency" was deduced for food in excess (TD50 approximately 16 g/kg per day). Ovemutrition in Switzerland was converted into excess food intake and the cancer risk estimated on the basis ofthe TD50 value. The resulting risk of60,000 cases per one million lives wou1d aJlow to explain by overnutrition almost all "diet-related" cancer deaths in humans.
The rate limiting step in 5-fluorouracil catabolism is catalyzed by the enzyme dihydropyrimidine dehydrogenase. Since degradation of 5-fluorouracil decreases its efficacy in chemotherapy, the inhibition of its catabolism is a promising tool. We investigated the formation of micronuclei in vitro in mouse L5178Y cells. 5-fluorouracil induced an increase in micronucleus frequency, which could significantly be enhanced by the concurrent application of 2,6-dihydroxypyridine, an inhibitor of dihydropyrimidine dehydrogenase. The 5-fluorouracil concentration necessary to reach maximal genotoxic effects could be reduced to half in the presence of inhibitor. 2,6-Dihydroxypyridine alone and the naturally occuring enzyme substrate uracil did not induce micronucleus formation. Combined application of the chemotherapeutic agent 5-fluorouracil and an inhibitor of its could reduce side-effects by lowering the effective dose of the active drug. With this study we provide further support for the usefulness of this concept.
This study was designed to investigate a previously unidentified potential mechanism for mutation induction as well as to clarify a biological comequence of micronucleus formation. We compared the induction of micronuclei with mutation inductioo as measured by trißuorothymidine (TFI') resistance in mouse L5178Y cells using four aneugens: colcemid, diethylstilbestrol, griseofulvin and vioblastine. AU four compounds induced micronuclei which appeared in the first cell cycle after treatment. More than 85% of the micronuclei induced by each compound stained positive for the presence of kinetochores implying that the micronuclei contained wbole cbromosomes. However, these same compounds were unable to induce TFf resistance under tbree different treatment regimes. We concluded that tbese compounds, under conditions where tbey induce primarily kinetochore positive micronuclel, were not able to induce mutations. Thus, the induction of micronuclei containing wbole chromosomes barborlog a select.able gene is not an early event leadlog to mutations in these cells.
The cytoskeleton and/or membrane skeleton has been implicated in the regulation of N-formyl peptide receptors. The coupling of these chemotactic receptors to the membrane skeleton was investigated in plasma membranes from unstimulated and desensitized human neutrophils using the photoreactive agonist N-formyl-met-leu-phelys-N\(^6\)-[\(^{125}\)I]2(p-azidosalicylamido)ethyl-1,3'-dithiopropionate (fMLFK-[\(^{125}\)I]ASD). When membranes of unstimulated cells were solubilized in Triton-X 100, a detergent that does not disrupt actin filaments, only 50% of the photoaffinity-labeled receptors were solubilized sedimenting in sucrose density gradients at a rate consistent with previous reports. The remainder were found in the pellet fraction along with the membrane skeletal actin. Solubilization of the membranes in the presence of p-chloromercuriphenylsulfonic acid, elevated concentrations of KCI, or deoxyribonuclease I released receptors in parallel with actin. When membranes from neutrophils, desensitized by incubation with fMLFK-e 251]ASD at 15°C, were solubilized, nearly all receptors were recovered in the pellet fraction. lncubation of cells with the Iigand at 4°C inhibited desensitization partially and prevented the conversion of a significant fraction of receptors to the form associated with the membrane skeletal pellet. ln these separations the photoaffinity-labeled receptors not sedimenting to the pellet cosedimented with actin. Approximately 25% of these receptors could be immunosedimented with antiactin antibodies suggesting that N-formyl peptide receptors may interact directly with actin. These results are consistent with a regulatory role for the interaction of chemotactic N-formyl peptide receptors with actin of the membrane skeleton.
Signal transduction via receptors for N-formylmethionyl peptide chemoattractants (FPR) on human neutrophils is a highly regulated process which involves participation of cytoskeletal elements. Evidence exists suggesting that the cytoskeleton and/or the membrane skeleton controls the distributJon of FPR in the plane of the plasma membrane, thus controlling the accessibility of FPR to different proteins in functionally distinct domains. In desensitized cells, FPR are restricted todomains which are depleted of G proteins but enriched in cytoskeletal proteins such as actin and fodrin. Thus, the G protein signal transduction partners of FPR become inaccessible to the agonist-occupied receptor, preventing cell activation. The mechanism of interaction of FPR with the membrane skeleton is poorly understood but evidence is accumulating that suggests a direct binding of FPR (and other receptors) to cytoskeletal proteins such as actin.
Desensitization of N-formyl peptide chemoattractant receptors (FPR) in human neutrophils results in association of these receptors to the membrane skeleton. This is thought to be the critical event in the lateral segregation of receptors and guanyl nucleotide-binding proteins (G proteins) within the plane of the plasma membrane resulting in an interruption of the signaling cascade. In this study we probed the interaction of FPR with G protein in human neutrophils that were desensitized to various degrees. Human neutrophils were desensitized using the photoreactive agonist N-formyl-met-leu-phelys- N\(^\epsilon\)-[\(^{125}\)I]2(p-azidosalicylamido )ethyl-1 ,3 '-dithiopropionate (/MLFK-[\(^{125}\)I]ASD). The interaction if FPR with G protein was studied via a reconstitution assay and subsequent analysis of FPR-G protein complexes in sucrose density gradients. FPR-G protein complexes were reconstituted with solubilized FPR from partially and fully desensitized neutrophils with increasing concentrations of Gi purified from bovine brain. The respective EC\(_{50}\) values for reconstitution were similar to that determined for FPR from unstimulated neutrophils (Bommakanti RK et al., J Bio[ Chem 267: 757~7581, 1992). We conclude, therefore, that the affinity of the interaction of FPR with G protein is not affected by desensitization, consistent with the model of lateral segregation of FPR and G protein as a mechanism of desensitization.
Desensitization of N-fonnyl peptide chemoattractant receptors (FPR) in human neutrophils is thought to be achieved by lateral segregation of receptors and G proteins within the plane of the plasma membrane resulting in an interruption of the signalling cascade. Direct coupling of FPR to membrane skeletal actin appears to be the basis of this process~ however, the molecular mechanism is unknown. In this study we investigated the effect of energy depletion on formation of FPR-membrane skeleton complexes. In addition the effect of the protein kinase C inhibitor stauroporine and the phosphatase inhibitor okadaic acid on coupling of FPR to the membrane skeletonwas studied. Human neutrophils were desensitized using the photoreactive agonist N-formy1-met-leu-phe-1ys-N'[\(^{125}\)I]2(p-azidosalicylamido)ethyl-1,3'-dithiopropionate (fMLFK-[\(^{125}\)I]ASD) after ATP depletion with NaF or after incubation with the respective inhibitors. The interaction of FPR with the membrane skeleton was studied by Sedimentation of the membrane skeleton-associated receptors in sucrose density gradients. Energy depletion of the cells markedly inhibited the formation of FPR-membrane skeleton complexes. This does not appear tobe related to inhibition of protein phosphorylation due to ATP depletion because inhibition of protein kinases and phosphatases bad no significant effect on coupling of FPR to the membrane skeleton. We conclude, therefore, that coupling of FPR to the membrane skeleton is an energy,dependent process which does not appear to require modification of the receptor protein by phosphorylation.
The detection Iimit of the lacl transgenic mouse mutagenicity assay lies, in practice, at approximately a 50-100% increase in mutant frequency in treated animals over controls. The sensitivity of this assay in detecting genotoxins can be markedly improved by subchronic rather than acute application of the test compound. The lac/ transgenic mouse mutagenicity assay was compared quantitatively to rodent carcinogenicity tests and to presently used in vivo mutagenicity assays. With the genotoxic carcinogens tested thus far, a rough correlation between mutagenic potency and carcinogenic potency was observed: on average, to obtain a doubling in lacl mutant frequency the mice bad to be treated with a total dose equal to 50 times the TD50 daily dose Ievel. This total dose could be administered eilher at a high dose rate within a few days or, preferably, at a low dose rate over several weeks. This analysis also indicated that a lacl experiment using a 250-day exposure period would give a detection Iimit approximately equal to that of a long-term carcinogenicity study. In comparison to the micronucleus test or the chromosome aberration assay, acute sturlies with the presently available lacl system offered no increase in sensitivity. However, subchronic lacl sturlies (3-4-month exposure) resulted in an increase in sensitivity over the established tests by 1-2 orders of magnitude (shown with 2-acetylaminofluorene, N-nitrosomethylamine, N-nitrosomethylurea and urethane). 1t is concluded that a positive result in the lacl test can be highly predictive of carcinogenicity butthat a negative result does not provide a large margin of safety.
In addition to its tumor-promoting activity in honnone-receptive tissue, the carcinogenic estrogen diethylstilbestrol (DES) has been found to induce cell transformation, aneuploidy and micronucleus formation in mammalian cells. The majority of these micronuclei contained whole chromosomes and were fonned during mitosis. Here a possible relationship between a disturbance in cell cycle progression and micronucleus fonnation is investigated by exposing Syrian hamster embryo (SHE) cells to DES. Continuous bromodeoxyuridine labeling followed by bivariate Hoechst 33258/ethidium bromide flow cytometry was employed for analysis of cell cycle transit and related to the time course of micronucleus formation. Treatment of SHE cells with DES resulted in delayed and impaired cell activation (exit from the GO/G 1 phase), impaired S-phase transit and, mainly, G2-phase traverse. Cells forming micronuclei, on the other hand, were predominantly in G2 phase during DES treatment. These results suggest that impairment of Sand G2 transit may involve a process ultimately leading to micronucleus formation.
Transgene Mausmodelle zur Charakterisierung der Funktion kardialer beta-adrenerger Rezeptoren
(2001)
In der vorliegenden Arbeit wurde die Funktion kardialer beta-adrenerger Rezeptoren mit Hilfe einer Kombination aus transgenen Mausmodellen und physiologischen und molekularbiologischen Methoden untersucht. Durch gezielte Überexpression des humanen beta1-adrenergen Rezeptors im Herzen transgener Mäuse konnte gezeigt werden, daß die chronische Aktivierung dieses Rezeptors eine trophische Wirkung auf die Herzmuskelzellen hat. Über einen Zeitraum von mehreren Monaten führte dies zur Entwicklung einer Herzinsuffizienz. In der menschlichen Herzinsuffizienz kommt es zu einem ähnlichen Phänomen: Durch deutlich erhöhte Freisetzung von endogenen Katecholaminen kommt es zu einer chronischen Dauerstimulation kardialer beta1-adrenerger Rezeptoren. Daß diese schädlich ist belegen das hier beschriebene Mausmodell und zudem einige neuere klinische Studien, die zeigen daß eine pharmakologische Blockade beta-adrenerger Rezeptoren zu einer Verminderung der Herzinsuffizienzmortalität führt. Dieses Mausmodell erlaubte es erstmals den beta1-adrenergen Rezeptor hinsichtlich seiner spontanen Rezeptoraktivität in einem physiologischen Modell zu untersuchen. Dabei zeigte sich, daß der humane beta1-adrenerge Rezeptor spontane Aktivität aufweist, jedoch in einem deutlich geringeren Ausmaß als der beta2-adrenerge Rezeptor. Dies könnte klinisch relevant sein, da klinisch verwendete beta-Rezeptor-Antagonisten die spontane Aktivität des beta1-adrenergen Rezeptors in unserem Modell unterschiedlich stark unterdrückten. In der vorliegenden Arbeit wurde zudem untersucht, ob sich die beiden kardial exprimierten Beta-Rezeptor-Subtypen Beta1 und Beta2 hinsichtlich ihrer Signaltransduktion unterscheiden. Ausgehend von dem Befund, daß die chronische Aktivierung der beiden Subtypen in transgenen Mausmodellen zu deutlich unterschiedlichen Phänotypen führt, wurden verschiedene intrazelluläre Signalwege auf ihre Aktivierung hin überprüft. Abweichend von publizierten, in vitro nach kurzzeitiger Rezeptorstimulation erhobenen Daten zeigte sich, daß die chronische Aktivierung der Rezeptorsubtypen zu einer unterschiedlichen Aktivierung der kardialen MAP-kinasen (ERK) führt. Die beta1-spezifische Aktivierung dieser Kinasen könnte die beobachtete unterschiedliche Hypertrophieentwicklung in diesen beiden Mausmodellen erklären. Einen weiteren Schwerpunkt bei der Aufklärung des Mechanismus beta-adrenerg induzierter Hypertrophie bildete die Untersuchung der zellulären Calcium-homöostase. Als früheste funktionelle Veränderung in der Entwicklung einer beta-adrenerg induzierten Herzhypertrophie und -insuffizienz trat dabei eine Störung des intrazellulären Calciumtransienten auf. Als möglicher Mechanismus für die Störung des Calciumhaushalts konnte eine zeitgleich auftretende veränderte Expression des Calcium-regulierenden Proteins Junctin beschrieben werden. Einen neuen therapeutischen Ansatz für die Therapie der Herzinsuffizienz könnten schließlich vielleicht die Untersuchungen zum kardialen Na/H-austauscher ergeben: Es konnte erstmals gezeigt werden, daß der kardiale Na/H-Austauscher maßgeblich an der beta-adrenerg induzierten Herzhypertrophie- und Fibrose-entstehung beteiligt ist und daß die pharmakologische Inhibition dieses Proteins sowohl Hypertrophie als auch die Fibrose wirksam unterdrücken kann.
Die Deletion des AT2-Rezeptors (AT2-KO) führt zu erhöhter Blutdruckempfindlichkeit und vaskulärer Hypertrophie durch Aktivitätszunahhme der P70S6-Kinase. Die Vasodilatation von Blutgefäßen wird maßgeblich durch beta1-adrenerge Rezeptoren vermittelt. Die Deletion von alpha2-adrenergen Rezeptoren (alpha2-KO) führt zur Entwicklung einer Herzinsuffizienz nach Aortenstenose. Der Mortalitätanstieg ist mit erhöhten Plasmanoradrenalin-Spiegeln (a2A-KO), bzw. Plasmaadrenalin-Spiegeln (a2C-KO) assoziiert.
Die Plasmamembran Kalzium-ATPase (PMCA) ist ein in den meisten eukaryontischen Zellen exprimiertes Enzym. Sie katalysiert den Transport von Kalziumionen aus der Zelle und besitzt gegenüber Kalzium eine hohe Affinität jedoch geringe Transportkapazität. Trotz der guten biochemischen Charakterisierung der Pumpe ist ihre Funktion in Zellen wie Kardiomyozyten, die zusätzlich über andere Kalzium-Transportsysteme wie den Natrium/Kalzium-Austauscher verfügen, weiterhin unklar. Erste Ergebnisse aus dem eigenen Labor an PMCA-überexprimierenden L6-Myoblasten zeigten einen Einfluss des Enzyms auf deren Wachstum und Differenzierung. Um diese Erkenntnisse auf den Herzmuskel zu übertragen war im Vorfeld ein transgenes Rattenmodel generiert worden, welches die hPMCA4CI unter einem myokardspezifischen Promotor überexprimierte. Dieses Modell stand für die vorliegende Arbeit zur weiteren Charakterisierung zur Verfügung. Untersucht wurde zunächst das Wachstumsverhalten von Primärkulturen neonataler Kardiomyozyten unter Stimulation mit fetalem Kälberserum, Noradrenalin und dem Platelet Derived Growth Factor BB, jeweils im Vergleich zwischen transgenen und Wildtyp-Kardiomyozyten. Dabei zeigte sich ein beschleunigtes Wachstum der PMCA-überexprimierenden Zellen. In einem zweiten Ansatz wurden Untersuchungen angestellt, um die subzelluläre Lokalisation der PMCA innerhalb der Herzmuskelzelle aufzudecken. Dabei wurden im Speziellen die Caveolae als Ort der möglichen Lokalisation untersucht, kleine, ca. 50-100 nm große Einstülpungen der Plasmamembran, mit charakteristischer Lipid- und Proteinzusammensetzung, darunter auch viele Rezeptoren und Signaltransduktionsmoleküle. Insgesamt konnte mit den Methoden der Detergenzextraktion, Doppelimmunfluoreszenz, Präparation Caveolae-reicher Membranen und Immunpräzipitation gezeigt werden, dass die PMCA zu einem großen Teil in Caveolae lokalisiert ist. Zusätzlich konnte in der Immunpräzipitation eine Interaktion der PMCA mit dem Caveolae-assoziierten Zytoskelettprotein Dystrophin dargestellt werden. Zusammenfassend deuten die Ergebnisse darauf hin, dass die PMCA über eine Steuerung der lokalen Kalziumkonzentration im Bereich der Caveolae modulierend in wachstumsregulierende Signaltransduktionswege von Kardiomyozyten eingreifen kann.
Einfluß der Atherosklerose auf den NO:cGMP Signalweg am Modell des cholesteringefütterten Kaninchen
(2002)
Atherosklerose ist Volkskrankheit und Todesursache Nummer Eins in den sogenannten entwickelten Ländern. Ursachen für die meisten Folgeerkrankungen sind Minderperfusion und Gefäßverschluß, verursacht durch Ablagerungen und Verdickung der Gefäßwand und durch einen pathologisch erhöhten Gefäßtonus. Mehrere zelluläre Signalwege, die im Gesunden eine Vasodilatation hervorrufen können, sind in atherosklerotischen Gefäßen gestört, so auch der NO:cGMP-Signalweg. Der Einfluß der Atherosklerose auf den NO-abhängigen Teil des Signalwegs, also NO-Produktion und -Abbau, sowie Diffusion von NO zu den glatten Muskelzellen, ist seit längerem bekannt. In dieser Studie zeigen wir, daß im fortgeschrittenen Stadium der Erkrankung auch der NO-unabhängige Teil des Signalwegs in erheblichen Maße gestört ist. Die Expression und Aktivität der Enzyme lösliche Guanylatzyklase (sGC) und cGMP-abhängige Proteinkinase-I ist vor allem in der neugebildeten Neointima reduziert. P-VASP, ein Indikator der Aktivität des gesamten NO:cGMP-Signalwegs, ist in eindrucksvoller Weise reduziert. Die Enzyme des NO-unabhängigen Teils des NO:cGMP-Signalwegs werden in zunehmenden Maße pharmakologisch beeinflußbar. Die Ergebnisse dieser Studie stellen somit eine wichtige Grundlage für neue Therapieansätze der Atherosklerose dar.
Obwohl radioaktiv markiertes meta-Iodbenzylguanidin (MIBG) häufig in der Diagnose und bei der Behandlung von Neuroblastomen in der Klink Verwendung findet, ist bis heute sehr wenig über seine Pharmakologie bekannt. In der Literatur finden sich öfters Andeutungen, die aber nicht belegt wurden. So fehlten Untersuchungen über indirekt-sympathomimetische Wirkungen von MIBG. Vor diesem Hintergrund untersuchten wir am isoliert perfundierten Kaninchenherzen die Wirkung von MIBG im Vergleich zum Prototyp eines indirekten Sympathomimetikums (Tyramin). Dabei zeigte sich, daß MIBG zwar etwas potenter aber nicht so effektiv wie Tyramin war. Dies zeigte sich sowohl beim Paramter Herzfrequenz als auch beim Parameter Noradrenalin-Freisetzung. Im Gegensatz dazu zeigte sich im Zeitverlauf, daß die Wirkung von MIBG wesentlich länger anhielt als die von Tyramin. Der Unterschied zwischen MIBG und Tyramin bezüglich der Effektivität als indirekte Sympathomimetika konnte mit unterschiedlichen Wirkstärken beider Substanzen als Hemmstoff des vesikulären Monoamin-Transporters erklärt werden. Tyramin und MIBG wurden in Versuchen mit Neuroblastomzellen mit gleicher Geschwindigkeit durch Uptake1 aufgenommen, Tyramin war aber ein wesentlich potenterer Hemmstoff des vesikulären Monoamin-Transporters als MIBG. Da aber MIBG im Gegensatz zu Tyramin kein Substrat der neuronalen Monoaminoxidase ist, hielt seine Wirkung auch deutlich länger an als die von Tyramin. Die indirekt sympathomimetische Wirkung von MIBG wurde anschließend auch in-vivo untersucht. Dort zeigte sich auch, daß MIBG trotz im Vergleich zu klinischen Anwendungen hoher Dosen wesentlich schwächer indirekt-sympathomimetisch wirkt als Tyramin. In diesen Versuchen wurde auch beobachtet, daß die indirekt-sympathomimetische Wirkung auf die Herzfrequenz durch eine Gegenregulation des Nervensystems (nämlich den Barorezeptor-Reflex) maskiert wurde. Obwohl MIBG in der Literatur von Anfang an als adrenerger Neuronenblocker bezeichnet wurde, fand sich in der Literatur kein direkter Beweis für diese Behauptung. Mit Hilfe eines in-vitro Modells konnte in der vorliegenden Arbeit der Beweis erbracht werden, daß MIBG ein adrenerger Neuronenblocker ist. Dazu benutzten wir als Parameter die durch elektrische Stimulation induzierte Freisetzung von Noradrenalin im spontan schlagenden, perfundierten Kaninchenherzen. Die stimulationsbedingte Abgabe von Noradrenalin ins Perfusat wurde durch MIBG zeit- und konzentrationsabhängig blockiert. Da viele adrenerge Neuronenblocker das Enzym Monoaminoxidase (MAO) hemmen, wurde in-vitro untersucht, ob MIBG die beiden Iso-Enzyme MAO-A und MAO-B hemmt. Es konnte gezeigt werden, daß MIBG die MAO kompetitiv hemmt und zwar bevorzugt die Isoform MAO-A. Diese MAO-Hemmung wurde auch in-vivo in den Versuchen mit narkotisierten Kaninchen beobachtet. MIBG verminderte nämlich dosisabhängig die Konzentration des desaminierten Noradrenalin-Metaboliten DOPEG im Blutplasma der Tiere. Die Beobachtung, daß für die Hemmung der MAO-A im perfundierten Herzen eine IC50 von 17 nM, im Gewebehomogenat von Herzen dagegen eine IC50 von 18 µM gefunden wurde, spricht dafür, daß MIBG als Substrat von Uptake1 im Axoplasma der sympathischen Neurone des Herzens um den Faktor 1000 angereichert wird. Somit konnten in der vorliegenden Arbeit einige offene Fragen zur Pharmakologie von MIBG im Bereich des sympathomimetischen Nervensystems beantwortet werden, die auch für den klinischen Einsatz von MIBG wichtig sein könnten.
Alpha2-Rezeptoren, die weiter in alpha2A, alpha2B und alpha2C unterteilt werden, gehören zur Gruppe der adrenergen Rezeptoren innerhalb der Klasse der G-Protein-gekoppelten Rezeptoren. Sie sind maßgeblich an der Regulation vieler physiologischer Prozesse beteiligt. Vieles, was heute über alpha2-Rezeptoren bekannt ist, wurde mithilfe von alpha2-defizienten Mäusen, sogenannten „Knock-Out“-Mäusen (KO) herausgefunden, von denen bislang drei Einzel-KOs und der Doppel-KO der Subtypen A und C existieren. Im Rahmen dieser Arbeit wurden durch Kreuzung der vorhandenen KO-Linien Mauslinien generiert, die defizient für alpha2A und alpha2B, für alpha2B und alpha2C oder alle drei alpha2-Rezeptoren sind. Während alpha2AB-KO-Mäuse ungefähr entsprechend der Mendelschen Verteilung geboren wurden, zeigte sich, dass alpha2BC-KO-Mäuse teilweise und alpha2ABC-KO-Mäuse sogar komplett embryonal letal waren. Die morphologischen Unter-suchungen legten den Zeitpunkt der embryonalen Letalität der alpha2ABC-KO-Mäuse auf den Tag E10,5 der Embryonalentwicklung fest und konnten zeigen, dass diese Letalität in einem Vaskularisierungsdefekt innerhalb der extraembryonalen Organe Plazenta und Dottersack begründet lag. Diese Organe stellen die Versorgung des Embryos mit Nährstoffen und Sauerstoff sicher und sorgen somit für dessen Entwicklung. Durch RT-PCR-Experimente konnte die mRNS für alle drei alpha2-Rezeptorsubtypen an Tag E10,5 sowohl im Embryo als auch in Plazenta und Dottersack nachgewiesen werden. Autoradiographische Experimente und Radioligandenbindungsstudien an Plazenten machten deutlich, dass der Großteil an alpha2-Rezeptoren im embryonalen Teil der Plazenta exprimiert wird, nämlich in den Riesenzellen und in der sich daran anschließenden Spongiotrophoblastschicht, und dass hierbei alpha2-Rezeptoren vom B-Subtyp vorherrschen. In den genannten Zellen konnte mittels Immunhistochemie eine alpha2-Rezeptor-vermittelte Phosphorylierung der MAP-Kinasen ERK1/2 gezeigt werden, die auch in kultivierten WT-Dottersäcken beobachtet werden konnte. Unter basalen Bedingungen zeigte sich, dass die ERK1/2-Phosphorylierung in Gewebe von alpha2ABC-KO-Embryonen drastisch vermindert war, während andere Signalwege, die von alpha2-Rezeptoren angestoßen werden können, nicht beeinträchtigt waren. Versuche in einem Zellkulturmodell und mit kultivierten WT-Dottersäcken ergaben eine physiologisch relevante Wechselwirkung zwischen dem alpha2B-Rezeptor und dem PDGFbeta-Rezeptor, einer Rezeptortyrosinkinase, als deren Mechanismus sich in Co-Kultur-Experimenten mit alpha2B-Rezeptor-transfizierten Zellen und alpha2ABC-defizienten Dottersäcken die Transaktivierung von Rezeptortyrosinkinasen herausstellte. In dieser Arbeit konnte demonstriert werden, dass a2-Rezeptoren bei der Maus über eine Transaktivierung von ERK1/2 die Vaskularisierung der Plazenta und des Dottersacks bedingen und damit eine normale Embryonalentwicklung sicherstellen.
In einer Population von 304 Männern und Frauen konnte die Frequenz der TA-Duplikation im Promotor der Uridin-Diphosphat-Glukuronyltransferase Isoform 1A1 bestimmt werden. Sie beträgt 0,39 in der Gruppe der Männer und 0,30 in der Gruppe der Frauen, in der Gesamtgruppe kommt das Allel mit einer relativen Häufigkeit von 0,35 vor. Es wurde gezeigt, daß die Höhe der Bilirubinspiegel und die Diagnose "Gilbert Syndrom" nach definierten klinisch-chemischen Kriterien gut mit dem Genotyp korreliert. Dabei lagen die mittleren Bilirubinwerte der Frauen deutlich unter denen der Männer. Die Festlegung neuer Referenzbereiche für Bilirubin von <18µmol/l für Männer und <15µmol/l für Frauen wurde daraus abgeleitet. Ein Unterschied in der Glukuronidierungskapazität von Paracetamol zwischen Probanden mit homozygot wildtypischer, homozygot mutierter und heterozygoter Allelkombination konnte nicht nachgewiesen werden. Deshalb scheint die UGT1A1 nicht das für Para-cet-amol verantwortliche Isoenzym zu sein. Die Bestimmung des Genotyps des UGT1A1 Promotors kann zur Vorhersage zukünf-tiger oder Erklärung vorliegender erhöhter Bilirubinspiegel herangezogen werden. Dies kann in der Klinik zur routinemäßigen Diagnostik des Gilbert Syndroms eingesetzt werden. Für die klinische Forschung bietet die Genotypisierung der UGT1A1 eine Möglichkeit, zwischen dem genetischen Polymorphismus oder einer Reaktion auf die Prüfmedikation als möglichen Ursachen eine Erhöhung der Bilirubinwerte eines Probanden zu unterscheiden. Zur Phäno-typisierung dieses Stoffwechselweges ist Paracetamol nicht geeignet. Personen mit Gilbert Syndrom unterliegen bei der Einnahme von Paracetamol vermutlich keinem erhöhten Risiko toxischer Nebenwirkungen.
In dieser Arbeit wurden die tumorpromovierenden Effekte von 2-Acetylaminofluoren (2-AAF), 2-Nitrosofluoren (2-NOF) und Phenobarbital (PB) auf die Expression des EGF-Rezeptors (EGF-R), der Proteinkinase C (PKC), der Protoonkogene c-FOS und c-JUN in HepG2 Zellen bestimmt. Nur PB hemmte die Expression des EGF-R, wohingegen die PKC, c-FOS und c-JUN nicht beeinflusst wurden. 2-AAF, 2-NOF und PB wirkten konzentrationsabhängig zytotoxisch und antiproliferativ auf HepG2-Zellen. Die PKC scheint an diesem Effekt beteiligt zu sein. Die Bindungsaktivität der Transkriptionsfaktoren AP1 und NFkappa B wurde durch 2-NOF und Phenobarbital erhöht, wohingegen der Effekt von 2-AAF nicht endeutig zu klären war.
Paclitaxel wird als antineoplastisches Agenz hauptsächlich gegen Ovarial- und Brusttumore eingesetzt. Seine Wirkung beruht auf einer Störung der mikrotubulären Dynamik und Struktur des Zytoskeletts, die einen Arrest der Zelle in der G2- und Mitosephase des Zellzykluses bewirkt. Da Zellen, die in der G2/M-Phase des Zellzykluses arretiert sind, eine erhöhte Empfindlichkeit gegenüber ionisierender Strahlung aufweisen, könnte Paclitaxel als Strahlensensibilisierer in einer Kombinationstherapie mit Bestrahlung Vorteile in der Tumortherapie haben. In dieser Arbeit wurden daher die gentoxischer Effekte einer Einzelbehandlung und einer Kombinationsbehandlung von Paclitaxel und Strahlung untersucht. Da eine Tumortherapie stark von der Art des Tumors abhängt, wurden verschiedene Tumorzellinien untersucht. Als gentoxischen Endpunkt wurde die Induktion von Mikrokernen in vitro gewählt. Der in vitro Mikrokerntest ist ein valider und empfindlicher Test, der sensitiv gegenüber Spindelgiften wie Paclitaxel und chromosomenbrechende Agentien, wie ionisiernder Strahlung ist. In der Maus Lymphom Zellinie L5178Y, den Lungenfibroblasten V79, den humanen Cervixkarzinomzellen HeLa und in den humanen Brustkrebszellen MCF-7 konnte keine Radiosensibilisierung durch Paclitaxel detektiert werden. Die Anzahl der induzierten Mikrokerne lag immer im Bereich der theoretischen Addition der Einzelbehandlung mit Paclitaxel und Bestrahlung. In der humanen Lungenkarzinomzellinie A549, die als fünfte Zellreihe untersucht wurde, konnte für eine Kombination von 2,5 nM Paclitaxel und 2 Gy Bestrahlung ein synergistischer Effekt gefunden werden (30 %ige Erhöhung der Mikrokernrate bei Kombinationsbehandlung verglichen mit der Summe der Einzelbehandlungen). Dieser Effekt konnte in Wiederholungsexperimenten, in denen höhere Dosen an Paclitaxel verwendet wurden jedoch nicht reproduziert werden. Insgesamt konnten damit die Ergebnisse des in vitro Mikrokerntestes in fünf verschiedenen Zellinien keine eindeutige Radiosensibilisierung von Paclitaxel zeigen. In Folgestudien sollten daher verschiedene Konzentrationen und Behandlunsdauern von Paclitaxel sowie andere Endpunkte untersucht werden, um eine abschließende Beurteilung, ob Paclitaxel als zelltypabhängiger Radiosensibilisierer fungieren könnte, zu erlauben.
Schon vor mehr als zwei Jahrzehnten wurde eine erhöhte Tumorentstehungsrate bei Patienten mit chronischer Nierenerkrankung unter Dialysebehandlung festgestellt. Eine der wahrscheinlichsten Erklärungen für dieses Phänomen ist die klinische Manifestation eines Immundefektes innerhalb dieses Patientenkollektives. Lymphozyten von Patienten mit chronischen Nierenerkrankungen ohne Dialyse und Dialysepatienten mit einer Behandlungsdauer von mehr als 120 Monaten verfügen nachweislich über eine reduzierte DNA-Reparaturfähigkeit. Zusätzlich weisen sie eine erhöhte Rate von Mikrokernen auf, was für verstärkte gentoxische Einflüsse im Patientenblut spricht. In dieser Arbeit wurde mittels Comet Assay, einem sensiblen Testverfahren zur Quantifizierung von DNA-Schäden auf Einzellzellniveau, aus verschiedenen Gruppen von chronisch Nierenkranken die Zellkern-DNA von peripheren Lymphozyten auf Schäden untersucht. Neben Patienten mit leicht bis stark erhöhten Kreatininspiegeln wurden auch Kollektive mit Hämodialyse und Hämodiafiltrationsbehandlung auf DNA-Schäden untersucht und miteinander verglichen. In den Untersuchungen konnte gezeigt werden, dass in der Gruppe der chronisch Nierenkranken ohne Dialysebehandlung offensichtlich ein Zusammenhang zwischen Höhe des Kreatininspiegels und einer durch den Comet Assay feststellbaren DNA-Schädigung besteht: im Kollektiv der Hämodialysepatienten ist mit der Dauer der Behandlung ein Anstieg des Schadens zu verzeichnen. Bei Patienten mit Hämodiafiltrationsbehandlung hingegen war kein Anstieg der DNA-Schäden mit der Länge der Behandlung feststellbar. Bei gleicher Behandlungsdauer bestehen zwischen Hämodialyse- und Hämodiafiltrationsgruppe nur unwesentliche Schadensdifferenzen. Dies war nicht vorhersehbar, da besonders Patienten mit stärkeren gesundheitlichen Einschränkungen in den Vorzug der Hämodiafiltration gelangen. Insgesamt zeigten jedoch alle untersuchten Gruppen einen signifikanten Anstieg der DNA-Schädigung gegenüber den Kontrollen. Da der Comet Assay derzeit noch mit methodischen und patientenbedingten Ergebniss-Schwankungen behaftet ist, muss jede Interpretation mit Zurückhaltung erfolgen. Insbesondere muss anhand eines Zusammenhanges hinsichtlich Gentoxizität und vorliegender Erkrankung untersucht und kritisch hinterfragt werden, ob ein früherer Beginn der Dialyse-Behandlung für den Patienten von Vorteil sein könnte. Inwieweit eine Umstellung von Hämodialyse auf Hämodiafiltration die Schäden der lymphozytären Zellkern DNA und somit eventuell auch die Tumorentstehungsraten beeinflusst, ist durch weitere Forschungen auf diesem Gebiet zu klären.
Soluble guanylyl cyclase (sGC) is the best established receptor for nitric oxide (NO) and regulates a great number of important physiological functions. Surprisingly, despite the wellappreciated roles of this enzyme in regulation of vascular tone, smooth muscle cell proliferation, platelet aggregation, renal sodium secretion, synaptic plasticity, and other functions, extremely little is known about the regulation of sGC activity and protein levels. To date, the only well-proven physiologically relevant sGC regulator is NO. In the present study, some additional possibilities for sGC regulation were shown. Firstly, we evaluated the ability of different NO donors to stimulate sGC. Significant differences in the sGC stimulation by SNP and DEA/NO were found. DEA/NO stimulated sGC much stronger than did SNP. Interestingly, no correlation between the sGC protein and maximal activity distribution was found in rat brain regions tested, suggesting the existence of some additional regulatory mechanisms for sGC. The failure of SNP to stimulate sGC maximally might be one of the reasons why the lack of correlation between the distribution of sGC activity and proteins in brain was not detected earlier. Prolonged exposure of endothelial cells to NO donors produced desensitization of the cGMP response. This desensitization cannot be explained by increased PDE activity, since PDE inhibitors were not able to prevent the NO donor-induced decrease of the maximal cGMP response in endothelial cells. The failure of SH-reducing agents to improve the cGMP response after its desensitization by NO suggests that a SH-independent mechanism mediates NO effects. Demonstration that the potency of the recently described activator of oxidized (heme-free) sGC, BAY58-2667, to stimulate sGC increases after prolonged exposure of the cells to an NO donor, DETA/NO, suggests that oxidation of heme may be a reason for NOinduced desensitization of sGC and decrease in sGC protein level. Indeed, the well-known heme-oxidizing agent ODQ produces a dramatic decrease in sGC protein levels in endothelial cells and BAY58-2667 prevents this effect. Although the mechanism of sGC activation and stabilization by BAY58-2667 is unknown, this substance is an interesting candidate to modulate sGC under conditions where sGC heme iron is oxidized. Very little is known about regulation of sGC by intracellular localization or translocation between different intracellular compartments. In the present study, an increase in sGC sensitivity to NO under membrane association was demonstrated. Treatment of isolated lung with VEGF markedly increased sGC in membrane fractions of endothelial cells. Failure of VEGF to stimulate sGC membrane association in cultured endothelial cells allows us to propose a complex mechanism of regulation of sGC membrane association and/or a transient character of sGC membrane attachment. A very likely mechanism for the attachment of sGC to membranes is via sGCinteracting proteins. These proteins may participate also in other aspects of sGC regulation. The role of the recently described sGC interaction partner, Hsp90, was investigated. Shortterm treatment of endothelial cells with an Hsp90 inhibitor does not affect NO donor or calcium ionophore-stimulated cGMP accumulation in the cells. However, inhibition of Hsp90 results in a rapid and dramatic decrease in sGC protein levels in endothelial cells. These effects were unrelated to changes in sGC transcription, since inhibition of transcription had much slower effect on sGC protein levels. In contrast, inhibitors of proteasomes abolished the reduction in sGC protein levels produced by an Hsp90 inhibitor, suggesting involvement of proteolytic degradation of sGC proteins during inhibition of Hsp90. All these data together suggest that Hsp90 is required to maintain mature sGC proteins. In conclusion, in the present study it was demonstrated that multiple mechanisms are involved in the regulation of sGC activity and its sensitivity to NO. Oxidation of sGC heme by NO seems to be one of the mechanisms for negative regulation of sGC in the presence of high or prolonged stimulation with NO. Another possible means of regulating sGC sensitivity to NO is via the intracellular translocation of the enzyme. It has been also demonstrated here that attachment of sGC to the membrane fraction results in an apparent increase in the enzyme sensitivity to NO. Additionally, Hsp90 was required to maintain sGC protein in endothelial and other cell types. However, we could not find any acute affect of Hsp90 on sGC activity, as reported recently. All these findings demonstrate that the regulation of sGC activity and protein level is a much more complex process than had been assumed earlier.
Die Gruppe der adrenergen Rezeptoren (AR) umfasst neun Rezeptoren (3 alpha1-, 3 alpha2-, 3 beta-AR), die alle durch die physiologischen Liganden Adrenalin und Noradrenalin aktiviert werden können. Eine Subgruppe der AR bilden die drei alpha2-AR alpha2A, alpha2B und alpha2C. Sie können prä- oder postsynaptisch lokalisiert sein. Präsynaptisch lokalisierte alpha2-AR hemmen die Transmitterfreisetzung im Sinne einer negativen Rückkopplung. Die Hauptrolle bei der präsynaptischen Hemmung der Transmitterfreisetzung spielen alpha2-AR vom Subtyp alpha2A. Es lagen zu Beginn dieser Arbeit auch Hinweise vor, daß noch weitere alpha2-Rezeptorsubtypen an dieser Funktion beteiligt sind. Eine eindeutige Zuordnung dieser alpha2-AR zu den Subtypen alpha2B oder alpha2C gelang aber bisher nicht. In dieser Arbeit sollte deshalb die Frage beantwortet werden, welche alpha2-AR neben dem alpha2A-AR an der präsynaptischen Hemmung der Transmitterfreisetzung im zentralen Nervensystem beteiligt sind. Zur Subtypunterscheidung wurden "knockout"-Mäuse verwendet, die nur einen oder zwei alpha2-Rezeptorsubtypen exprimierten. Gehirnschnitte aus dem Neokortex und den Basalganglien dieser Mauslinien wurden mit radoaktiv markiertem Noradrenalin bzw. Dopamin inkubiert. Anschließend wurde in Transmitterfreisetzungsexperimenten mit den so behandelten Gehirnschnitten Konzentrations-Wirkungskurven mit verschiedenen Liganden erstellt. Auf diese Weise konnte gezeigt werden, daß neben den alpha2A-AR auch alpha2C-AR präsynaptisch die Transmitterfreisetzung von Noradrenalin und Dopamin hemmen. In einem weiteren Schritt wurde die Aktivierungs- und Deaktivierungskinetik der alpha2A- und alpha2C-AR im heterologen Expressionssystem untersucht. Hierzu wurden stabile HEK293-Zellinien generiert, die entweder alpha2A- oder alpha2C-AR unterschiedlich stark exprimierten. Diese Zellinien wurden transient mit GIRK-Kanälen transfiziert, um die durch Stimulation mit Noradrenalin resultierenden Kaliumströme mit der "patch-clamp"-Technik zu messen. Dabei ergab sich kein signifikanter Unterschied zwischen alpha2A- und alpha2C-AR bezüglich der Aktivierungskinetik. Alpha2C-AR deaktivierten jedoch deutlich langsamer als alpha2A-AR. Diese Befunde belegen, daß zwei der drei alpha2-AR-Subtypen, alpha2A und alpha2C, als präsynaptische Autorezeptoren (Noradrenalin) bzw. Heterorezeptoren (Dopamin) die Neurotransmission modulieren. Dies könnte in der Zukunft für die Entwicklung neuer, subtypspezifischer Pharmaka von großer Bedeutung sein.
Ergebnisse vieler epidemiologischer Studien über die Risikoabschätzungen von Tumoren hormonabhängiger Gewebe legen einen deutlichen Zusammenhang zwischen den Hormonen und dem Auftreten dieser Tumoren nahe. Dabei wird der zellproliferationssteigernde Effekt der Hormone im Rahmen des Mehrstufenkonzeptes der Kanzerogenese meist als Promotionsfaktor beschrieben. In der vorliegenden Arbeit soll gezeigt werden, dass die hormonelle Induktion einer erhöhten Zellteilungsrate auch primär zu einer genetischen Instabilität beiträgt, mit dem Ziel einen weiteren Mechanismus in der Pathogenese hormonabhängiger Tumoren aufzuklären. Die östrogenrezeptorpositive Ovarialtumorzellinie BG-1 und die rezeptornegativen UCI-107 Zellen wurden mit 17-ß Östradiol behandelt und anschließend mit Hilfe des Mikrokerntests auf chromosomale Schäden untersucht. Die Bestimmung der Mikrokernrate bei den östrogensensitiven BG-1 Zellen zeigte, dass mit steigender Proliferationsinduktion auch die Mikrokernfrequenz konzentrationsabhängig erhöht war. Bei der Behandlung der BG-1 Zellen mit 17-ß Östradiol in Kombination mit dem spezifischen Östrogenrezeptorantagonisten 4- Hydroxytamoxifen wurde die östradiolinduzierte rezeptorabhängige Proliferationsstimulation durch Hydroxytamoxifen gehemmt. Parallel dazu sank auch die Mikrokernrate. Bei vergleichbaren Versuchen mit der östrogeninsensitiven UCI-107 Zellinie, bei der keine Effekte auf die Proliferation bei Behandlung der Zellen mit 17-ß Östradiol alleine sowie in Kombination mit 4- Hydroxytamoxifen detektiert werden konnte, wurde auch keine Mikrokerninduktion beobachtet. Eine erhöhte Mikrokernfrequenz konnte wiederum ausschließlich in den östradiolstimulierten BG-1 Zellen festgestellt werden, als durch den Einsatz des Zytokineseinhibitors Cytochalasin B die Auswertung der Mikrokerne auf jene Zellen normiert wurde, die genau eine Zellteilung durchgeführt hatten. Die Ergebnisse machten deutlich, dass die östradiolstimulierten Zellen auf Grund der beschleunigten Proliferation eine „andere Art von Zellteilung“ durchführen. In einem weiteren Abschnitt der Arbeit wurde der Einfluss der Östradiolstimulierung auf den Zellzyklus untersucht. Mittels eines FACScans konnten die prozentualen Zellzyklusphasenanteile (G1/ G0-, S- und G2/ M- Phase) der BG-1 Zellen zu verschiedenen Zeiten des Wachstums bestimmt werden. Zum Beispiel war der Anteil an Zellen der östradiolstimulierten Zellpopulation in der G2/ M Phase durchgehend um 6-8 % geringer gegenüber dem Anteil an Zellen, die mit Lösungsmittel behandelt wurden. Möglicherweise ist dies ein Erklärungsansatz für das vermehrte Auftreten von Mikrokernen bei Östradiolstimulierung, da bekannt ist, dass es in der G2/ M-Phase einen wichtigen Kontrollpunkt innerhalb des Zellzyklus zur Detektion und Reparatur chromosomaler Schäden gibt. Bei Berechnung der Zellzyklusphasenzeiten ergab sich ebenso in der G2/M Phase eine deutlich verkürzte Verweildauer der östradiol-behandelten BG-1 Zellen. Zusammengefaßt leitet sich die Hypothese ab: „Die Zellen werden auf Grund der hormonellen Proliferationsstimulierung durch den Zellzyklus „gejagt“, demzufolge werden wichtige „Checkpoints“ im Zellzyklus überlaufen, wodurch eine genetische Instabilität entstehen.kann“.
Zusammenfassung Systeme zur induzierbaren Transgenexpression sind wichtige Werkzeuge, um die Funktion einzelner Gene in vitro und in vivo zu untersuchen. Sie bestehen aus drei Grundkomponenten, einem zu regulierenden Zielgen, einem "Schalter" und einem Liganden, der diesen Schalter bedient. In dieser Arbeit wurden Untersuchungen am Ecdysonsystem durchgeführt, das als Schalter den Insektensteroidhormonrezeptor für das Verpuppungshormon Ecdyson verwendet. Zunächst wurde ein neuer Rezeptor mit der Ligandenbindedomäne des Ecdysonrezeptors (EcR) des Seidenspinners Bombyx mori konstruiert, dessen Eigenschaften in der Zellkultur mit einem DrosophilaEcR-Konstrukt, das für mammalische Expression optimiert ist, verglichen wurden. Mit dem BombyxEcR konnte die Transgenexpression durch den nichtsteroidalen Liganden Tebufenozid gesteuert werden, was beim DrosophilaEcR nicht möglich war. Damit ist man in diesem Expressionssystem nicht wie beim DrosophilaEcR auf teure steroidale Liganden wie Ponasteron angewiesen. Außerdem mußte beim BombyxEcR der Heterodimerisierungspartner RXR nicht kotransfiziert werden. In Bezug auf erreichbaren Induktionsfaktor und Kinetik der Genexpression zeigten sich für die beiden Systeme vergleichbare Ergebnisse. Weiterhin wurden durch Pronukleusinjektion transgene Mäuse erzeugt, die den BombyxEcR unter einem herzspezifischen Promotor (aMHC) exprimieren. Als Zielgen wurde die b2a-Untereinheit des L-Typ-Calciumkanals eingebracht, die mit dem neuen Schaltsystem herzspezifisch gesteuert werden sollte. Die Bioverfügbarkeit des Agonisten Tebufenozid nach intraperitonealer Injektion wurde in einem in-vitro Assay in HEK293-Zellen überprüft. Es ergaben sich hinreichende Wirkstoffspiegel im Serum der Mäuse, um das Reportergen zu induzieren. Auch wenn bei der transgenen Maus nach der Induktion mit Tebufenozid kein immunologischer Nachweis erhöhter Expression der b2a-Untereinheit gelang,konnte doch in Herzkatheteruntersuchungen eine veränderte Herzfunktion nachgewiesen werden. Bei transgenen Mäusen führte die intraperitoneale Applikation von Tebufenozid für bis zu sieben Tage zu einem signifikanten Anstieg des systolischen Blutdrucks und der maximalen linksventrikulären Kontraktionsgeschwindigkeit, der bei nicht-transgenen Kontrolltieren nicht beobachtet wurde. Diese Befunde deuten erstmals in vivo darauf hin, daß die b2a–Untereinheit des L-Typ-Calciumkanals am Herzen eine positiv inotrope Wirkung vermitteln kann. Systeme zur induzierbaren Genexpression müssen weiterentwickelt werden, um die Ideale der präzisen Steuerung ohne Nebenwirkungen sowohl für die Grundlagenforschung als auch für eine in weiterer Zukunft liegende Verwendung in der Gentherapie zu erreichen.
Phytohormone, insbesondere solche mit östrogenem Potential werden heute vermehrt in der postklimakterischen Hormonersatztherapie als natürliche Alternative zu Designeröstrogenen eingesetzt, da sie vermutlich ein besseres Wirkungs-Nebenwirkungsprofil besitzten. Mengenmäßig am bedeutensten sind die Phytoöstrogene aus den Stoffgruppen der Isoflavone, Cumestane und Indol-3-carbinole. Weit über 100 Pflanzen produzieren Phytohormone. Die bekanntesten sind die Sojabohne, Weintrauben, Leinsamen, Haferflocken, Spargel, Traubensilberkerze und roter Klee. Phytohormone können täglich in großer Menge aufgenommen werden (1mg pro kg Körpergewicht), wobei durchaus Plasmaspiegel von über 1µM erreicht werden. Gerade deshalb darf nicht davon ausgegangen werden, daß natürliche Produkte per se gut für die Gesundheit wären. Phytohormone und insbesondere deren Metaboliten, die während der intestinalen Passage entstehen, wurden vielfach nicht den gleichen Prüfbedingungen unterzogen wie sie für andere in Lebensmitteln vorkommenden Substanzen, wie z.B. Konservierungs-, Farb- oder Aromastoffen, heute selbstverständlich ist. Diese Arbeit soll deshalb anhand von in-vitro Tests an Mauslymphomzellen L5178Y für eine Auswahl an Phytohormonen und deren Metaboliten mögliche toxische oder gentoxische Effekte detektieren und die bestehende Datenlage ergänzen. Aus der Gruppe der Isoflavone wurden die Daidzeinmetaboloiten Equol und O-desmethylangolensin und die Glyceteinmetaboliten 3,4,7- und 4,6,7-Trihyroxyisoflavon untersucht. Aus der Gruppe der Flavone wurde Fisetin und aus der Gruppe der Stilbene Resveratrol untersucht. Weiterhin wurden Daten zu den Anthocyanen Delphinidin-, Pelargonidin- und Cyanidin-Chlorid erhoben. Toxische Effekte wurden anhand von Proliferatiosexperimenten, durch die Bestimmung der Zellvitalität (Ethidiumbromid-Flouresceinmethode) und durch die Analyse der Teilungsaktivität nach Behandlung mit Cytocalasin B und anschließender Bestimmung des Anteils mehrkerniger Zellen detektiert. Zur Bestimmung von gentoxischen Effekte wurde auf den Mikrokerntest zurückgegriffen. Ergänzend sollte eine Immunfloureszenzfärbung der Kinetochorproteine in Mikrokernen Aufschluß über aneugene oder klastogene Wirksamkeit der untersuchten Substanzen geben. Die in dieser Arbeit gewonnenen Daten weisen darauf hin, daß erste adverse Effekte der Phytohormone oder deren Metaboliten im Bereich der erreichbaren Plasmakonzentration liegen, so daß eine übertriebene Aufnahme hochdosierter Phytohormonen derzeit als kritisch erachtet und weiterer Forschungsbedarf festgestellt werden muß.
Mechanisms of apoptosis modulation and their contribution to genomic instability in tumor cells
(2004)
The concept of programmed cell death has been increasingly considered from various aspects since early 1970’s. Primarily, knowledge of apoptosis referred to morphological changes in which chromatin is condensed and increasingly fragmented, revealed as small structure in the nucleus. The membrane shrinks and the cell becomes dense as can be seen by flow cytometry. Interestingly, similar modes of cell deletion were observed in nematodes indicating that apoptosis is a highly conserved machinery. Three Caeonorhabditis elegans gene products are found to have high homology with mammalian apoptotic genes: CED-9 inhibits apoptosis and is related to bcl-2; CED-3 and CED-4 promote apoptosis and are related to caspase 9 and APAF-1. Apoptosis is not accidental death, but a highly controlled and medically important molecular process. More general terms such as ‘physiological’ or ‘regulated’ cell death cover different morphologies and sequences. Programmed suicide of cells that were subjected to toxic exogenous and endogenous stimuli plays a key role in understanding cancer development and its treatment. Apoptosis involves sequences of events that may overlap and play contradictory or antagonistic roles in cell death. Generally, the ability to trigger apoptotic processes in cancer cells would benefit an organism by keeping homeostasis intact. Programmed cell death is a regularly present mechanism, for instance, in lymphocyte recruitment in the thymus where immature lymphocytes may recognize host antigens. Therefore, such lymphocytes become apoptotic and are removed by macrophages. Removal prevents possible autoimmune diseases. Unlike apoptosis, necrosis is a passive process of cell death recognizable by membrane morphological changes and accompanied by leakage of intracellular material into intercellular space that may cause inflammation in the organism. Signals that may initiate apoptosis are generally classified into two groups: signals that launch extrinsic apoptotic pathways starting with aggregation of death receptors and intrinsic apoptotic pathways starting with disruption of intracellular homeostasis such as the release of mitochondrial factors or DNA degradation. Early in the process, apoptotic signals may lead to a broad range of signaling mechanisms such as DNA repair and assessment of DNA damage (check points). Thus, failure in any of these steps can cause a defective apoptotic response that plays a decisive role in both tumorigenesis and drug resistance in tumor treatment. More distinctly, the capability of cancer cells to go into apoptosis prevents further neoplastic changes. Generally, the purpose of this study is to investigate the balance between formation of genomic damage and induction of apoptosis under genotoxic stress. After genotoxic insult there are different possibilities for the fate of a cell (Figure 1). The genomic integrity is analyzed at cellular checkpoints, usually leading to a delay in cell cycle progression if DNA was damaged. Mutations in genes such as p53 and p21 change the cellular response to genotoxic stress and may alter the balance between apoptosis and genomic damage. However, p53 is usually mutated or not expressed in 70% of human tumors. Alterations in p53 states that reflect distinct apoptotic response upon induction of DNA damage were examined. In this study, three cell lines with distinct p53 states were used: TK6 harboring wild-type p53, WTK1 with mutated p53 and NH32 with knocked out p53. In the present work we applied different approaches to investigate the correlation between DNA damage and apoptotic responsiveness in cancer cell lines with different p53 states or in hormone responsive cell lines with over expressed bcl-2 gene. We were focused on effects caused by temporary down regulation of the p53 and Bcl-2 activity in human lymphoblastoid cell lines. In addition, we investigated the impact of estradiol-induced proliferation on apoptosis and DNA damage in stably transfected cells with bcl-2gene.
Die vorliegende Arbeit beschäftigt sich im Gegensatz zu bisherigen Studien (überwiegend im Rahmen von Querschnittsstudien) v.a. prospektiv mit der Untersuchung der Auswirkung verschiedener Faktoren (1. Prädialysephase, 2. Wechsel von der Hämodialyse zu HDF-Behandlung, 3. Einfluß einer Angiotensin IIAntagonistentherapie sowie (durch einmalige Erhebung) „Langzeit“-HDF-Behandlung)auf den relativen genetischen Schaden, ermittelt durch den Comet-Assay und den Mikrokern-Test in peripheren Lymphozyten bei Dialysepatienten bzw. Prädialysepatienten.
The biotransformation of 1,1,1,3,3-pentafluoropropane was investigated in rats and in in vitro systems. First, the metabolites were identified in vivo using GC/MS and 19F NMR analysis. The main metabolite was identified as trifluoroacetic acid, the minor metabolite as 3,3,3-trifluoropropionic acid and as a cleavage product, inorganic fluoride was found. As the in vitro system, liver microsomes from rat and human samples and rat liver homogenates were used. Trifluoroacetic acid and 3,3,3 trifluoropropionic acid were confirmed in vitro as metabolic intermediates, following biotransformation of 1,1,1,3,3-pentafluoropropane by the cytochrome P-450-system. Studies, designed for clarifying the cardiotoxicity of 1,1,1,3,3-pentafluoropropane were driven by the hypothesis that 3,3,3-trifluoropropionic acid is the toxic agent. This was based on the lethal toxicity, which was observed in previous in vivo experiments. In addition, the point of its structural similarity to toxic agents as for example monofluoroacetic acid or of possible metabolic intermediates like difluoroacrylic acid with known toxicity were considered to support this assumption. However, trifluoroacetic acid was neglected as the sought-after toxic agent because of its different toxic effects, known from literature. Investigations on the biotransformation of 3,3,3-trifluoropropionic acid were performed and resulted in no metabolic activity and in poor elimination of 3,3,3-trifluoropropionic acid in vivo. The histopathological effects on the heart, which were observed in the 90-day oral toxicity study of 1,1,1,3,3-pentafluoropropane in rats, namely mononuclear inflammatory cell infiltrations and degenerated myocardial fibers, were not observed after a 28 day repeated exposure of up to 10 mg/kg b.w. of 3,3,3-trifluoropropionic acid. However, a single high dose of 3,3,3-trifluoropropionic acid lead to severe toxicological effects. The difference in the observed toxic effects after a single and repeated administration may be due to adaptive mechanisms in rats. The toxicological effects included clinical signs like ataxia, coma and cramps. The conditions of the rats suggested possible inhibition of the energy supply to the organism. Furthermore, the interference of 3,3,3-trifluoropropionic acid in the functionality of the organism was investigated. Experiments were performed in vitro in rat liver and heart mitochondria to investigate effects on the mitochondrial ß-oxidation. However, the transformation of the substrate [U14C] palmitic acid in the ß oxidation pathway was not inhibited by 3,3,3-trifluoropropionic acid. In addition, no cytotoxicity of 3,3,3 trifluoropropionic acid was observed in the cell culture systems. The main effect after a single dose of 3,3,3-trifluoropropionic acid was seen in clinical pathology and metabonomic analysis. The decrease in blood glucose is considered to have the most far-reaching consequences for the toxicity of 3,3,3-trifluoropropionic acid. If considering this change as the primary effect after a single dose, secondary effects, for example, the above-mentioned clinical signs could be explained. In addition, the observed high level of ketone bodies might have been responsible for life-threatening possible ketoacidosis. In general, ketoacidosis occurs after an imbalance between glycolysis, lipolysis, TCA cycle activity and respiratory function. Based on the results, ß-oxidation of fatty acids was not affected, and due to the decrease in glucose levels and the high levels of acetyl CoA, glycolysis was considered not to be impaired. Increased amounts of acetyl CoA might be a result of insufficient activity of the TCA cycle. However, the inhibition of the TCA cycle can be based on the impairment of specific enzymes and/or on the involvement of messenger substrates like insulin. Supporting the first mentioned aspect are decreased levels of TCA cycle intermediates, like α-ketoglutarate or citrate, as seen in 1H-NMR spectra of urine. However, the second aspect would explain the drop in blood glucose with the impairment of glucose transporters or the impairment of the insulin balance. If a single dose of 3,3,3-trifluoropropionic acid had stimulated the insulin release, glycolysis would be activated, and high amounts of acetyl CoA would be produced. In case of impaired use by the TCA cycle, levels of ketone bodies would be increased. Experiments were designed to characterize the direct effect of 3,3,3-trifluoropropionic acid on rat insulinoma-derived INS-1 cells as possible increase in insulin release. Further investigations are necessary to answer in which step of the metabolic pathway 3,3,3-trifluoropropionic acid interferes or finally which specific enzyme is inhibited or activated by 3,3,3-trifluoropropionic acid, leading to the drop in blood glucose and finally in lethal toxicity.
The cyclic nucleotides cAMP and cGMP are two ubiquitous important second messengers, which regulate diverse physiological responses from vision and memory to blood pressure and thrombus formation. They act in cells via cAMP- and cGMP-dependent protein kinases (PKA and GK), cyclic nucleotide-gated channels and Epac. Although the concept of cyclic nucleotide signalling is well developed based on classical biochemical studies, these techniques have not allowed to analyze cAMP and cGMP in live cells with high temporal and spatial resolution. In the present study fluorescence resonance energy transfer was used to develop a technique for visualization of cAMP and cGMP in live cells and in vitro by means of fluorescent biosensors. Ligand-induced conformational change in a single nucleotide-binding domain flanked with green fluorescent protein mutants was used for dynamic, highly sensitive measurements of cAMP and cGMP. Such biosensors retained binding properties and chemical specificity of unmodified domains, allowing to image cyclic nucleotides in a physiologically relevant range of concentrations. To develop cAMP-sensors, binding domains of PKA, Epac and cAMP-gated HCN-channel were used. cGMP-sensors were based on single domains of GK and phosphodiesterases (PDEs). Sensors based on Epac were used to analyze spatio-temporal dynamics of cAMP in neurons and macrophages, demonstrating that cAMP-gradients travel with a high speed (~ 40 μm/s) throughout the entire cytosol. To understand the mechanisms of cAMP-compartmentation, kinetics properties of phosphodi-esterase (PDE2) were, next, analyzed in aldosterone producing cells. PDE2 is able to rapidly hydrolyze extensive amounts of cAMP, so that the speed of cAMP-hydrolysis is much faster than that of its synthesis, which might serve as a basis of compartmentation. cAMP-sensors were also used to develop a clinically relevant diagnostic method for reliable detection of β1-adrenergic receptor autoantibodies in cardiac myopathy patients, which has allowed to significantly increase the sensitivity of previously developed diagnostic approaches. Conformational change in a single binding domain of GK and PDE was, next, used to create novel fluorescent biosensors for cGMP. These sensors demonstrated high spatio-temporal resolution and were applied to analyze rapid dynamics of cGMP production by soluble and particulate guanylyl cyclases as well as to image cGMP in mesangial cells. In summary, highly sensitive biosensors for cAMP and cGMP based on single cyclic nucleotide-binding domains have been developed and used in various biological and clinically relevant applications.
In der vorliegenden Arbeit wurden die kardial differenzierten embryonalen Stammzellen (ES-Zellen) mittels der von Wobus et al. entwickelten Tröpfchentechnik gewonnen. Eine Optimierung der kardialen Ausbeute konnte durch eine Selektionsmethode erreicht werden, die auf der Expression eines Resistenzgens in den kardial differenzierten ES-Zellen beruht. Hierdurch wurde eine reproduzierbar hohe Anreicherung von ES-Kardiomyozyten erzielt. Die erstmalig durchgeführte quantitative Bestimmung der endogenen β-adrenergen Rezeptorexpression in ES-Kardiomyozyten zeigte eine Subtyp-Verteilung, die mit derjenigen in adulten Maus-Kardiomyozyten übereinstimmt, wobei eine höhere endogene Expression in ES-Kardiomyozyten vorlag. Ferner konnte durch eine β-adrenerge Stimulation in 16 Tage alten ES-Kardiomyozyten eine positive chronotrope Reaktion sowie eine Aktivierung der Adenylatzyklase-Aktivität hervorgerufen werden. Diese Ergebnisse zeigen, dass ES-Kardiomyozyten am 16. Differenzierungstag einen vollständig ausgereiften β-adrenergen Signalweg aufweisen und hinsichtlich der physiologischen Effekte vergleichbare Merkmale mit adulten Maus-Kardiomyoyzten haben. Ein weiteres Ziel dieser Arbeit war es, die Fähigkeit eines adenoviralen Gentransfers in ES-Kardiomoyzten zu untersuchen. Dabei zeigte sich, dass der Gentransfer mittels rekombinanten Adenoviren eine sehr effiziente und durchführbare Methode zur Expression von Transgenen in ES-Kardiomyozyten ist. Weiterhin konnte die funktionelle Kopplung der adenoviral überexprimierten β1-adrenergen Rezeptoren nachgewiesen werden. Die Überexpression hatte eine ausgeprägte Sensitivierung der Rezeptorantwort zur Folge, während die maximale Isoprenalin-induzierte cAMP-Produktion nur wenig erhöht wurde. Dies entspricht Befunden an transgenen Mausmodellen mit einer β1-adrenergen Rezeptor-überexpression. Eine Sensitivierung des chronotropen Effektes konnte dagegen nicht gezeigt werden. Möglicherweise führte die Transfektion der ES-Kardiomyozyten-Zellverbände nur zu einem oberflächlich begrenzten Gentransfer, der keinen Einfluss auf die Gesamtheit des funktionellen Synzytiums hatte. Außerdem wurde in dieser Arbeit der Einfluss einer unterschiedlichen Phosducin-Expression auf die kardiale Differenzierungsfähigkeit in transgenen ES-Zellen untersucht. Dabei konnte kein signifikanter Unterschied in der kardialen Differenzierung sowie in der Basalfrequenz von homozygoten und heterozygoten Phosducin Knock-out Klonen beziehungsweise von Phosducin überexprimierenden Zellklonen festgestellt werden.
Hormone spielen bei der Kanzerogenese eine wichtige Rolle, indem sie vor allem auf die Phase der Promotion einwirken und die Proliferation bereits initiierter Zellen steigern können. In dieser Arbeit wurden humane Ovarialkarzinomzellen mit Östrogen, Insulin, IGF und EGF zur Proliferation angeregt, woraus eine erhöhte Mikrokernrate resultierte. Mikrokerne sind chromatinhaltige Strukturen, die außerhalb des Zellkerns liegen. Somit lag nahe, dass durch die Steigerung der Proliferation eine genetische Instabiltät erzeugt wurde. Weitere Experimente zeigten eine Forcierung der genetisch geschädigten Zellen durch den Zellzyklus, so dass vermutet werden kann, dass schnell proliferierende Zellen durch Verringerung der zellulären Reparaturmechanismen eine erhöhte Rate an genetischer Instabilität aufweisen. Unterstützt wird diese Hypothese durch Analyse diverser Zellzyklusregulationsproteine mittel Wester-Blot.
Hintergrund: Passivrauchen ist nicht nur als kanzerogen für den Menschen eingestuft, sondern verursacht auch verschiedene andere Erkrankungen. Oft wird dabei der Passivrauchbelastung von Kindern im häuslichen Bereich zu wenig Beachtung geschenkt. In dieser Arbeit wurde deswegen der Zusammenhang zwischen Passivrauchen auf der einen Seite und atopischen Erkrankungen, Erkrankungen der oberen Atemwege und Gentoxizität auf der anderen Seite untersucht. Methoden: Die Daten von über 100 Kindern zwischen 1 und 15 Jahren wurden mit Hilfe eines Fragebogens erhoben und zusammen mit den Krankenakten ausgewertet. Zur Prüfung der Gentoxizität wurden Mikrokernraten und Schwesterchromatidenaustausche in peripheren Lymphozyten bestimmt. Der Erfassung der inneren Exposition dienten Hämoglobinaddukte von 4-Aminobiphenyl, welches in Zigarettenrauch vorkommt und als krebserzeugend für den Menschen eingestuft ist. Ergebnisse: Bei Untersuchung der Mikrokernraten zeigten die rauchbelasteten Kinder höhere Mikrokernraten (Mittelwert: 12,7/1000 zweikernige Lymphozyten) als die unbelasteten (Mittelwert: 11,7 Mikrokerne/1000 zweikernige Lymphozyten). Der Unterschied war aber nicht signifikant (p = 0,344). Außerdem hatten die Vorschulkinder mit rauchenden Eltern signifikant höhere Mikrokernraten (Mittelwert: 14,2/1000 zweikernige Lymphozyten) als die Schulkinder (Mittelwert: 9,2/1000 zweikernige Lymphozyten; p = 0,031). Die Analyse der 4-Aminobiphenyl-Hämoglobinaddukte der 1,25- bis 4,0-Jährigen ergab leicht höhere Werte für Kinder mit rauchenden Eltern (Mittelwert: 66,52 pg/g Hb) als für Kinder, deren Eltern nicht zu Hause rauchten, und deren Werte (Mittelwert: 56,18 pg/g Hb) waren höher als die der unbelasteten Kinder (Mittelwert: 49,60 pg/g Hb). Der Unterschied war nicht signifikant. Bei Betrachtung der atopischen Erkrankungen war der Anteil der Atopiker bei der rauchexponierten Gruppe höher (31,3 %) als bei der nicht exponierten (16,3 %), obwohl die genetische Vorbelastung in der rauchbelasteten Gruppe etwas geringer war als in der unbelasteten. Bei den Kindern mit Erkrankungen der oberen Atemwege zeigte sich ein höherer Anteil rauchexponierter Kinder (61,3 %) als in der Gruppe der Kinder mit Erkrankungen, die wahrscheinlich nicht mit postnataler Passivrauchexposition in Zusammenhang stehen (44,8 %). Schlussfolgerung: Diese Arbeit unterstreicht die Bedeutung von Passivrauchen im Hinblick auf atopische Erkrankungen und Erkrankungen der oberen Atemwege bei Kindern. Gerade die häusliche Passivrauch-Belastung im Vorschulalter und ihre Auswirkung auf das Erbgut sollten hinsichtlich der erhöhten Mikrokernraten mehr Beachtung finden.
Ein Problem der Therapie maligner Tumore ist die Resistez gegenüber Chemotherapeutika. Diskutiert wird ein Zusammenhang zur Expression von Hitzeschockproteinen (HSP). Insbesondere das in Mamma-Karzinomen stark exprimierte HSP27 und HSP70 scheinen hier beteiligt. Hitzeschockproteine sind Teil eines durch Noxen induzierten Mechanismus, welcher Schutz vor weiterer Noxenexposition verleiht, also die entsprechenen Zellen im Unterschied zu nicht exponierten Kontrollzellen zu überleben befähigt. Es kommt nach einem Streßereignis zu einer Veränderung von Zelltod unter nachfolgenden Bedingungen, z.B. Verhütung von Apoptose (physiologischer Zelltod). Tumortherapie mittels Zytostatika stellt eine „kontrollierte Apoptose“ dar. Ziel dieser Therapie muß es also folglich sein, eine HSP-Induktion zu vermeiden, da eine solche den Therapieerfolg und Benefit für den Patienten schmälert. Die Exposition einer Tumorzelle mit einem chemotherapeutisch wirksamen Medikament bedeutet für diese Zelle toxischen/oxidativen Streß, den sie nur durch Induktion entsprechender Abwehrmechanismen überleben kann. Diese Mechanismen haben letztlich einen wesentlichen Einfluß auf die Wirksamkeit des Medikamentes und Profit des Patienten durch die ihm angebotene Therapie. Eine frühe adaptive Zellantwort von Säugerzellen auf toxische Einflüsse stellt die Expression von Hitzeschockproteinen dar. Den Fokus der vorliegenden Untersuchungen stellen einerseits diejenigen Substanzen dar, welche heutzutage in der Therapie des Mamma-Karzinoms eingesetzt werden, den drei Einzelsubstanzen des CMF-Protokolls Methotrexat, 5-Fluorouracil und Cyclophosphamid, andererseits die Hitzeschockproteine mit der höchsten bekannten Bedeutung für Tumorwachstum. In einem ersten Schritt wurde in vitro mit einem Zellsystem, welches durch Transfektion mit dem humanen hsp27-Gen bei bekannter HSP70-Induzierbarkeit als einfaches isoliertes Zellsystem ein gutes Werkzeug zur spezifischen Untersuchung dieser beiden Proteine darstellt, untersucht werden, inwieweit sich diese speziellen Proteine durch die unterschiedlichen Substanzgruppen des CMF-Protokolls induzieren lassen. Es wurde also nach einer adaptiven Zellantwort in Form einer Induktion von HSP27 und HSP70 nachfolgend einer Noxenexposition gesucht werden. In einem zweiten Schritt wurde untersucht, ob die für diese beiden HSPs postulierte zytoprotektive Eigenschaften auch für Zytostatika gelten. Es wurde überprüft , inwieweit Chemotherapeutika unter dem Einfluß von HSP70 und HSP27 stehen, also inwieweit die Expression von HSP27 und HSP70 einen Zellschutz gegen toxischen Streß (durch CMF) in den verwendeten L929-Mausfibroblasten darstellen kann.
Azoles are important chemicals used as antifungal agents in agriculture and human medicine, but also as cytostatic drugs in tumour chemotherapy. Antifungal activities are based on inhibition of lanosterol-14α-demethylase (CYP51). CYP51 catalyses the oxidative removal of the methyl group # 32 of lanosterol to produce follicular fluid meiosis activating steroid (FF-MAS). For fungi the later resulting ergosterol is an essential compound of the cell membrane. Exposed fungi lack ergosterol, which leads to a collapse of the cell membrane. In mammals cholesterol, the downstream product of lanosterol-14α-demethylation necessary for the synthesis of bile acids, mineral corticoids, glucocorticoids and sex steroids, can be supplemented with food intake. However FF-MAS and the resulting T-MAS (testis meiosis activating steroids), the direct products of the CYP51 reaction, act as meiosis-activating steroids on ovaries and testes and are not supplemented with food intake. Inhibition of CYP51 in humans may therefore affect the endocrine system and is an unwanted side effect of azoles. Aromatase (CYP19) catalyses the demethylation of testosterone to estradiol and is inhibited by azoles. Reduction of estrogen levels by CYP19 inhibition is the working principle of cytostatic drugs used in breast cancer therapy but is considered an unwanted side effect for azoles used to treat fungal infections. A favourable fungicide or antifungal drug should be a strong inhibitor of fungal CYP51. In contrast human CYP51 and human CYP19 should not be inhibited by an azole fungicide or antifungal agent. The favourable cytostatic drug should show a high potency towards human CYP19. Neither human CYP51 nor fungal CYP51 should be inhibited by a cytostatic drug. The aim of this work was to assess: are fungicides and antifungal drugs strong inhibitors of fungal CYP51? In return do they not inhibit human CYP51 and human CYP19? Do cytostatic drugs strongly inhibit human CYP19? And in return do they not inhibit human CYP51 or fungal CYP51? Inhibitory potencies of 22 azole compounds used for the three purposes were tested in four inhibition assays: i) on commercially available human CYP19 utilising a fluorescent pseudo substrate dibenzylfluorescein (DBF) ii) on CYP19 utilising testosterone as substrate iii) on human CYP51 and iv) Candida albicans CYP51 utilising lanosterol as substrate. Product formation was measured by liquid chromatography – tandem mass spectrometry utilising photospray ionisation (APPI). A functional human CYP51 was available from BD Gentest Cooperation. A functional enzyme complex comprising of the Candida albicans lanosterol-14α-demethylase and the Candida tropicalis oxidoreductase was expressed in the baculovirus system. When comparing inhibitory potencies on CYP19, human CYP51 and Candida albicans CYP51 a number of agents show desirable patterns of inhibition e.g. the two cytostatic drugs, or two antifungal agents used in human medicine, fluconazole and itraconazole, and a wide variety of the fungicides, e.g. cyproconazole and hexaconazole. Undesirable patterns of inhibition were exhibited by a number of compounds, e.g. prochloraz, bifonazole, ketoconazole and miconazole. Seven compounds show a more complex picture of inhibitory potencies though. To get a picture of residue levels of azoles in food in a model case an LC-ESI-MS/MS method was developed for the determination of azole compounds in wine. All residues were below the maximum residue levels set by authorities. To classify the inhibitory potencies on the different enzyme systems IC50 values obtained were compared to exposure levels measured in farmers, maximum plasma concentrations in humans reported after exposure to antifungal drugs and to acceptable daily intake levels set by authorities. Based on the findings presented, the following conclusions can be drawn. The risk for agricultural workers set by exposure to azole fungicides with respect to human CYP51 and CYP19 can be regarded as negligible when safety measures are adhered to. As a matter of principle however, the usage of bifonazole, miconazole and ketoconazole has to be viewed with caution in respect to the high level of inhibition of human CYP51 and/or CYP19. Under the assumption that the acceptable daily intake amounts set by authorities for azole compounds are not exceeded the residues do not pose a threat to consumer safety judged by our findings. Inhibition of CYP19 with the consequence of a reduction of estradiol levels has to be regarded as a possible disrupting effect of the hormone balance. The relevance of FF-MAS and T-MAS in the endocrine system however still has to be evaluated completely bringing with it the question of how much importance has to be attached to the inhibition of human CYP51.
Seit langem werden auf das β-adrenerge System wirkende Pharmaka, v.a. β1-Antagonisten und β2-Agonisten, therapeutisch eingesetzt, allerdings sind die pharmakologischen Eigenschaften dieser Stoffe an den drei bekannten β-adrenergen Subtypen teilweise nur unzureichend untersucht. Ein Ziel dieser Arbeit war es daher, vergleichbare pharmakologische Daten für Agonisten (Adrenalin, Noradrenalin, Isoprenalin, Fenoterol, Salbutamol, Salmeterol, Terbutalin, Formoterol, Broxaterol) und Neutrale und Inverse Antagonisten (Propranolol, Alprenolol, Atenolol, Metoprolol, Bisoprolol, Carvedilol, Pindolol, BRL 37344, CGP 20712, SR 59230A, CGP 12177, ICI 118551) an allen drei Subtypen von adrenergen Rezeptoren in einem zellbiologisch identischen Hintergrund zu gewinnen. Dazu stellten wir stabil transfizierte CHO-Zelllinien her, die die einzelnen humanen β-adrenergen Subtypen in vergleichbarer Menge exprimierten. Nach der pharmakologischen Charakterisierung der einzelnen Rezeptorsubtypen erfolgte die Affinitätsmessung von klinisch häufig eingesetzten wie auch experimentell verwendeten Substanzen mit dem unselektiven β-adrenergen Antagonisten 125I-CYP als Radioligand. Darüber hinaus untersuchten wir die β-adrenerg vermittelte Stimulation der Adenylylcyclase in isolierten Membranen dieser Zelllinien. Alle untersuchten Substanzen zeigten charakteristische Bindungs- und funktionale Eigenschaften. Wir konnten nachweisen, dass einige β2- bzw. β3-Agonisten an den anderen Subtypen inversen Agonismus zeigen. Zusätzlich konnten β1-Antagonisten mit agonistischer Aktivität an β2- und β3-AR gefunden werden. Die gewonnenen Daten können somit helfen, klinisch beobachtete Effekte, wie z.B. die unerwünschten Wirkungen der entsprechenden Medikamente, besser zu verstehen. Insbesondere die Ergebnisse am β3-AR sind als Referenz und Ausgangspunkt weiterer Studien an diesem noch relativ wenig untersuchten Rezeptor wertvoll.
Die karzinogene Aktivität von Östradiol wurde bereits in mehreren Studien nachgewiesen und scheint das Ergebnis einer Kombination von hormonellen und genotoxischen Mechanismen zu sein. In der vorliegenden Arbeit konnte ein weiterer Mechanismus der Induktion chromosomaler Schäden durch Östradiol festgestellt werden. Es kam in der östrogenrezeptorpositiven Zelllinie MCF-7 zu einer konzentrationsabhängigen Steigerung der Zellproliferation und Mikrokernsteigerung, als Maß für die chromosomale Schädigung. In der östrogenrezeptornegativen Zelllinie MDA-MB231 konnte weder einer Steigerung der Zellproliferation, noch eine vermehrte Mikrokerninduktion nachgewiesen werden. Die Vermutung ist, dass die Zellen, durch den Proliferationsdruck den Zellteilungszyklus schneller durchlaufen und infolgedessen vermehrt Fehler im Replikationsablauf entstehen können. Zudem können wichtige Reparaturmechanismen oder Zellzykluskontrollpunkte nicht mehr adäquat agieren.
Conjugation of reactive intermediates of drugs with proteins or DNA may result in toxic effects such as hepatotoxicity, agranulocytosis, allergies, tumors, etc. From 1975 to 1999, 2.9% of drugs were withdrawn from the market due to such severe adverse drug reactions. Thus, formation of chemically reactive intermediates is a widely discussed problem in drug development processes. Early detection of potentially toxic compounds is required for drug discovery and drug development. Conjugation of such electrophilic compounds with glutathione (GSH) is one of the most important detoxifying reactions in vivo. Processing of these GSH-conjugates ultimately leads to the formation of renally cleared mercapturic acids, which may also be oxidized to sulfoxides. Thus, mercapturic acids may be generated and detected in vitro and non-invasively in vivo in urine to assess the reactivity of a compound in early stages of drug development processes. Therefore, the aim of this work was to develop and evaluate a HPLC-MS/MS screening method for simple and rapid detection and characterization of known and unknown mercapturic acids and application of the method to several different matrices. Based on the common constant neutral loss (CNL) of 129 Da of all mercapturic acids tested (in negative ion mode), a CNL survey scan was performed using a linear ion trap instrument and was combined with two enhanced product ion (EPI) scans with different collision energies to characterize the detected signals. The CNL resulted from the cleavage between the sulfur and the carbon atom in the N-acetyl-L-cysteine moiety. After optimization of the experimental parameters, the detection limits of the reference substances in rat urine ranged from 0.3 to 15.5 pmol on column (i.e. 20 ng/ml to 800 ng/ml). For in vitro evaluation of the method, the model compounds acetaminophen, diclofenac, bifonazole, clozapine, troglitazone, carbamazepine, and bisphenol A were screened for formation of reactive intermediates and, hence, detection of the corresponding mercapturic acids. To determine possible species- and tissue-specific toxicities, the model compounds were incubated with stimulated neutrophils and with liver microsomes from rats and humans. Species-specific differences were observed in incubations of acetaminophen and diclofenac with rat and human hepatic microsomes. Tissue-specific differences in biotransformation of the model compounds in incubations with human neutrophils and human liver microsomes were observed for diclofenac, carbamazepine, clozapine, and bifonazole. The developed HPLC-MS/MS method was also evaluated in vivo by analysis of rat and human urine. Drug-related mercapturic acids were detected in urine of rats orally treated with acetaminophen (20 mg/kg and 640 mg/kg b.w.) or diclofenac (10 mg/kg and 20 mg/kg b.w.). Human urine samples were analyzed before and after oral administration of a clinically used dose of 500 mg and 50 mg of acetaminophen. Besides detection of the mercapturic acid of N-acetylbenzoquinoneimine (AAP-MA), a second mercapturic acid with m/z 327 occurred dose-dependently in rat and human urine samples after administration of acetaminophen. Further investigations on identification of this metabolite using authentic compounds and comparing their MS/MS mass spectra demonstrated oxidation of AAP-MA to stereoisomeric sulfoxides in vivo. For diclofenac, a novel mercapturic acid with m/z 441 was detected in rat urine samples that was identical to a metabolite obtained in incubations with human neutrophils before. The in vivo formation of this diclofenac metabolite is described here for the first time. In addition, three endogenously formed mercapturic acids were detected and identified. In conclusion, the results of the in vitro and in vivo evaluation demonstrate the advantages of the rapid and generic HPLC-MS/MS screening method for the detection of mercapturic acids, that can be obtained with a minimum of sample preparation and a high throughput in diverse matrices.