ABSTRACT
Background: Suicide mortality rates are increasing among teenagers. Aim: To study the prevalence and predictive factors of suicide attempts among Chilean adolescents. Material and Methods: A random sample of 195 teenagers aged 16 ± 1 years (53% males) answered an anonymous survey about their demographic features, substance abuse, the Osaka suicidal ideation questionnaire, Smilksten familial Apgar. Beck hopelessness scale, Beck depression scale and Coppersmith self-esteem inventory. Results: Twenty five percent of respondents had attempted suicide at least in one occasion during their lives. These attempts were significantly associated with female gender, absent parents, family dysfunction, drug abuse, smoking, low self-esteem, hopelessness, depression and recent suicidal ideation. A logistic regression analysis accepted female gender, smoking and recent suicidal ideation as significant independent predictors of suicide attempt. Conclusions: Suicide attempted is common among teenagers and its predictors are female sex, smoking and previous suicidal ideation.
Subject(s)
Animals , Female , Humans , Mice , Pregnancy , Acetaldehyde/metabolism , Aldehyde Dehydrogenase/genetics , Aldehyde Dehydrogenase/metabolism , Embryo, Mammalian/metabolism , Ethanol/toxicity , Fanconi Anemia Complementation Group A Protein/genetics , Fanconi Anemia/pathology , Acetaldehyde/toxicity , Animals, Newborn , DNA Damage , Disease Models, Animal , Embryo, Mammalian/embryology , Genome , Hematopoietic Stem Cells/metabolism , Isoenzymes/genetics , Isoenzymes/metabolism , Retinal Dehydrogenase/genetics , Retinal Dehydrogenase/metabolismABSTRACT
En el hombre el consumo excesivo de alcohol está asociado con una disminución en la producción de testosterona y la atrofia testicular. Pudieron observarse consecuencias similares en estudios realizados in vitro en testículos aislados y la producción de testosterona, donde el acetaldehído mostró ser más potente que el alcohol para la supresión de la liberación de la hormona. Estudios previos de este laboratorio reportaron que la fracción microsomal del testículo de rata era capaz de metabolizar el etanol a metabolitos reactivos como el acetaldehído y los radicales libres 1-hidroxietilo. En este trabajo se presenta evidencia de que luego de una dosis única de etanol, el acetaldehído se acumula en el testículo durante las primeras seis horas posteriores al tratamiento para alcanzar concentraciones superiores a las plasmáticas aunque más bajas que en el hígado. Además se encontró que la actividad aldehído deshidrogenasa presente en el testículo es significativamente menor que en el hígado. El consumo de etanol en los animales produjo una susceptibilidad aumentada a la oxidación de los lípidos testiculares, que fue detectada por niveles aumentados de hidroperóxidos de lípidos. Los resultados sugieren que la oxidación in situ del etanol a acetaldehído y a radicales libres y la detoxificación deficiente podrían ser relevantes para explicar los efectos observados.
Excessive alcohol consumption is associated with impaired testosterone production and testicular atrophy. Similar findings were observed in in vitro studies on testosterone production by isolated testes, being acetaldehyde more potent than alcohol in suppressing testosterone release. In previous laboratory studies, it was reported that rat testicular microsomes were able to bioactivate ethanol to reactive metabolites like acetaldehyde and 1-hydroxyethyl free radical. In this work, evidence is shown that after a single ethanol dose, acetaldehyde accumulates in testicular tissue during the first six hours post-treatment to reach concentrations higher than those in blood but lower than those in the liver. In agreement with those findings, it was reported that aldehyde dehydrogenase activity in cytosolic, mitochondrial and microsomal fractions is significantly smaller than in the corresponding liver counterparts. Ethanol drinking led to increased susceptibility of testicular lipids to oxidation as detected by increased levels of microsomal lipid hydroperoxides. Results suggest that in situ oxidation of ethanol to acetaldehyde and free radicals and their poor detoxification would be relevant to the effects observed.
No homem, o consumo excessivo de álcool está associado a uma diminuição da produção de testosterona e atrofia testicular. Efeitos semelhantes foram observados em estudos realizados in vitro em testículos isolados e na produção de testosterona, em que o acetaldeído se mostrou mais potente do que o álcool para a supressão da liberação do hormônio. Estudos anteriores deste laboratório referiram que a fração microssomal do testículo de camundongo era capaz de metabolizar etanol para metabolitos reativos como o acetaldeído e os radicais livres 1-hidroxietil. Este trabalho apresenta evidência de que após uma dose única de etanol o acetaldeído se acumula no testículo durante as primeiras seis horas após o tratamento para atingir concentrações superiores às plasmáticas embora mais baixas que no fígado. Constatou-se também que a atividade aldeído desidrogenase presente no testículo é significativamente menor do que no fígado. O consumo de etanol nos animais produziu uma susceptibilidade aumentada à oxidação dos lipídeos testiculares, que foi detectada por níveis aumentados de hidroperóxidos de lipídeos. Os resultados sugerem que a oxidação in situ de etanol a acetaldeído e a radicais livres e a desintoxicação deficiente poderiam ser relevantes para explicar os efeitos observados.
Subject(s)
Animals , Rats , Oxidative Stress , Acetaldehyde/adverse effects , Acetaldehyde/toxicity , Testicular Diseases , Testis , Alcohol Drinking , AcetaldehydeABSTRACT
O acetaldeído é um comprovado agente mutagênico e carcinogênico, pode ser produzido endogenamente pela oxidação do álcool ingerido em bebidas alcoólicas e alimentos ou exogenamente, inalado como poluente, advindo da oxidação de combustíveis fósseis e etanol. O efeito do acetaldeído foi avaliado em modelos celulares e animais com o propósito de avaliarmos o aumento do estresse oxidativo, por lipoperoxidação, fragmentação do DNA, e a formação de adutos DNA, tais como 8-oxo-7,8-dihidro-2-desoxiguanosina, além de, 1,N2-eteno-2-desoxiguanosina e 1,N2-propano-2-desoxiguanosina que foram analisados por HPLC acoplado a espectrometria de massa com a utilização de metodologia ultra-sensível e reprodutiva. O tratamento de fibroblastos pulmonares humanos normais (IMR-90) com diversas concentrações de acetaldeído (58 µM a 711 µM) resultou em aumentos de morte celular, lipoperoxidação, fragmentação do DNA, cálcio intracelular e adutos de DNA. O efeito protetor do licopeno (20 µM) foi comprovado minimizando todos os efeitos deletérios promovidos pelo acetaldeído. O tratamento dos ratos Wistar por 8 e 30 dias com 150 mg/kg e 60 mg/kg via intra-peritoneal ou gavage, evidenciaram os efeitos tóxicos provocados pelo acetaldeído, como aumento significativo de lipoperoxidação, adutos e fragmentação de DNA no fígado e cérebro destes animais. A detecção dos adutos de DNA se mostrou uma ferramenta importante para a detecção dos efeitos provocados por exposição ao aldeído. No tratamento de animais por inalação com variadas concentrações de acetaldeído, que expôs os animais a quantidades do aldeído similares às encontradas em atmosferas poluídas, foi observado aumento de lipoperoxidação, sendo este dose dependente no fígado e pulmão. Já no cérebro, os níveis de MDA foram significativamente maiores em 10 ppb e 30 ppb em relação a 0 ppb e controle, e diminuíram significativamente em 90 ppb. Em relação aos níveis de fragmentação do DNA, observamos no pulmão aumento foi dose dependente...
Acetaldehyde is a known mutagen and carcinogen that can be produced endogenously by ethanol oxidation or directly inhaled as an air pollutant produced by fuel oxidation. The toxicity of acetaldehyde was evaluated in vitro and in vivo models, by means of oxidative stress parameters such as lipid peroxidation (measured as malonaldialdehyde -MDA), DNA fragmentation and DNA adducts such as 8-oxo-7,8-dihydro-2-desoxiguanosine, 1,N2-eteno-2-desoxiguanosine and 1,N2-propano-2-desoxiguanosine, this adducts were analyzed by an ultra-sensible and reproducible HPLC coupled to mass spectrometry assay. Treatment of human normal fibroblast (IMR-90) with a wide range of concentrations (58 µM to 711 µM) resulted in an increase in citotoxicity, lipid peroxidation, DNA fragmentation, intracellular calcium release and DNA adducts. Furthermore, lycopene (20 µM) presented a protective effect against the cellular deleterious properties of acetaldehyde. Treatment of Wistar rats for 8 and 30 days with 150 mg/kg and 60 mg/kg intra-peritonially or by gavage resulted in increased toxicity, measured by lipid peroxidation and DNA damage in liver and brain. The detection of DNA adducts was shown an important tool for the identification of deleterious effects induced by exposure to the aldehyde. Animals treated by inhalation, of amounts commonly found in polluted air samples, presented increased levels of lipid peroxidation in a dose dependent manner in liver and lungs. Nevertheless, in the brain of those animals the higher concentration was devoid of toxic effect measured as MDA levels. Lung tissue presented increased levels of DNA fragmentation. Furthermore, increased levels of 1,N2-εdGuo and 1,N2-propanodGuo was also observed in lungs of all animals. In DNA from livers, 1,N2-propanodGuo presented increased levels. Formation of 8-oxo-7,8-dihydro-2-desoxiguanosine, 1,N2-eteno-2-desoxiguanosine and 1,N2-propano-2-desoxiguanosine in urine samples of people living in the city of São Paulo
Subject(s)
Humans , Animals , Male , Adult , Rats , Acetaldehyde/toxicity , DNA Damage , Biomarkers/analysis , Environmental Pollution/statistics & numerical data , Chemical Pollutants , Carcinogens/analysis , Carcinogens/toxicity , Mutagens/analysis , Mutagens/toxicityABSTRACT
In order to clarify the effect of chronic oral administration of acetaldehyde, 24 adult albino rats of both sexes divided into four groups were used in this study. The stomach was dissected and prepared for staining by Hx and E, periodic acid Schiff, alcian blue- PAS and Pritchard technique. Acetaldehyde induced hyperkeratosis in the forestomach. In glandular stomach, it induced focal discontinuity in the surface mucous cells with exfoliation and shedding of the cells into the lumen. Dilatation and irregularity of many glandular tubules were observed with vacuolation and destruction of some parietal cells. Groups of chief cells were destroyed loosing their eosinophilic granules with pyknotic nuclei. Histochemical observation has revealed increased PAS reaction in the surface and mucous neck cells. Decreased reactivity to AB stain in the mucous neck cells was evident. These findings have suggested that acetaldehyde has a toxic effect even in small dose when taken orally for a long period. It is recommended to restrict its use as a flavoring agent as far as possible