RESUMEN
BACKGROUND: The leaves of Kalanchoe pinnata (Lam.) Pers. (K. pinnata), a succulent plant native to tropical regions, are used as a medicinal alternative against cancer in several countries worldwide; however, its therapeutic potential to fight cancer has been little addressed. In this study, we analyzed the phytochemical content, antioxidant capacity, and selectivity of K. pinnata leaf ethanolic extract against different human cancer cell lines in vitro. METHODOLOGY: This study subjected the ethanolic extract to enzymatic assays to quantify the phytochemical content (phenolics, flavonoids, and anthraquinones) and its radical scavenging and iron-reducing capacities. Also, the phytoconstituents and major phenolic compounds present in the extract's subfractions were identified by GC-MS, HPLC, and NMR. Human cancer (MCF-7, PC-3, HT-29) and normal colon (CoN) cell lines were treated with different concentrations of K. pinnata leaf ethanolic extract, and the changes in cell proliferation (sulforhodamine B assay), caspases activity (FITC-VAD-FMK reporter), mitochondrial membrane potential (MMP, rhodamine 123 assay), chromatin condensation/fragmentation (Hoechst 33342 stain), and ROS generation (DCFH2 probe assay) were assessed. RESULTS: The results showed that the K. pinnata leaf ethanolic extract is rich in phytoconstituents with therapeutic potential, including phenols (quercetin and kaempferol), flavonoids, fatty acid esters (34.6% of the total composition), 1- triacontanol and sterols (ergosterol and stigmasterol, 15.4% of the total composition); however, it presents a poor content of antioxidant molecules (IC50 = 27.6 mg/mL for H2O2 scavenging activity vs. 2.86 mg/mL in the case of Trolox). Notably, the extract inhibited cell proliferation and reduced MMP in all human cell lines tested but showed selectivity for HT-29 colon cancer cells compared to CoN normal cells (SI = 8.4). Furthermore, ROS generation, caspase activity, and chromatin condensation/fragmentation were augmented significantly in cancer-derived cell lines, indicating a selective cytotoxic effect. CONCLUSION: These findings reveal that the K. pinnata leaf ethanolic extract contains several bioactive molecules with therapeutic potential, capable of displaying selective cytotoxicity in different human cancer cell lines.
Asunto(s)
Apoptosis , Kalanchoe , Extractos Vegetales , Hojas de la Planta , Especies Reactivas de Oxígeno , Humanos , Extractos Vegetales/farmacología , Extractos Vegetales/química , Kalanchoe/química , Hojas de la Planta/química , Apoptosis/efectos de los fármacos , Especies Reactivas de Oxígeno/metabolismo , Línea Celular Tumoral , Antineoplásicos Fitogénicos/farmacología , Proliferación Celular/efectos de los fármacos , Antioxidantes/farmacologíaRESUMEN
The aim of this study was to evaluate the sperm head morphometry and chromatin condensation at different regions of the reproductive tract in bulls. Sperm smears of seminiferous tubules (ST), epididymis head (EH), body (EB), and tail (ET), and ductus deferens (DD) were stained with toluidine blue. Afterwards, the sperm head morphometry and chromatin alteration types were evaluated by a computational image analysis. Overall, spermatozoa of ST had lower (P < 0.05) area (A), perimeter (P), width (W), length (L), ellipticity (E), and Fourier harmonics (F0, F1, and F2). The chromatin decondensation (CD) and heterogeneity (CH) were higher (P < 0.05) in the ST region and decreased (P < 0.0001) during the migration along the reproductive tract (ST - DD direction). Considering the factors extracted (Factors 1 and 2) by the principal component analysis, the parameters A, P, W, L, and F0 were responsible for â¼36% of the Factor 1, while the E, F0, F1, and anterior-posterior symmetry (APS) contributed â¼27% to Factor 2. Both, CD and CH were associated with Factor 1 in the EH and ET regions and Factor 2 in the ST. Also, a well-defined difference between sperm heads collected from the ST and DD regions was observed by canonical analysis. The distribution of each chromatin alteration type was recorded. The proportion of normal sperm was lower (P < 0.05) in ST compared to other regions. Moreover, the chromatin influenced the morphometry and sperm heads with whole chromatin alteration type showed a smaller (P < 0.05) A, P, W, L, and E. In summary, the epididymal maturation is important for chromatin compaction and final morphometry of the sperm head. Also, the identification and quantification of the sperm chromatin condensation in different regions of reproductive tract can be used as potential biomarkers to predict the fertility in bulls.
Asunto(s)
Cromatina , Epidídimo , Animales , Bovinos , Masculino , Túbulos Seminíferos , Cabeza del Espermatozoide , Espermatozoides , Conducto DeferenteRESUMEN
DNA damage response (DDR) constitutes a protein pathway to handle eukaryotic DNA lesions in the context of chromatin. DDR engages the recruitment of signaling, transducer, effector, chromatin modifiers and remodeling proteins, allowing cell cycle delay, DNA repair or induction of senescence or apoptosis. An early DDR-event includes the epigenetic phosphorylation of the histone variant H2AX on serine 139 of the C-termini, so-called gammaH2AX. GammaH2AX foci detected by immunolabeling on interphase nuclei have been largely studied; nonetheless gammaH2AX signals on mitotic chromosomes are less understood. The CHO9 cell line is a subclone of CHO (Chinese hamster ovary) cells with original and rearranged Z chromosomes originated during cell line transformation. As a result, homologous chromosome regions have been relocated in different Z-chromosomes. In a first quantitative analysis of gammaH2AX signals on immunolabeled mitotic chromosomes of cytocentrifuged metaphase spreads, we reported that gammaH2AX139 signals of both control and bleomycin-exposed cultures showed statistically equal distribution between CHO9 homologous chromosome regions, suggesting a possible dependence on the structure/function of chromatin. We have also demonstrated that bleomycin-induced gammaH2AX foci map preferentially to DNA replicating domains in CHO9 interphase nuclei. With the aim of understanding the role of gammaH2AX signals on metaphase chromosomes, the relation between 5-ethynyl-2'-deoxyuridine (EdU) labeled replicating chromosome regions and gammaH2AX signals in immunolabeled cytocentrifuged metaphase spreads from control and bleomycin-treated CHO9 cultures was analyzed in the present work. A quantitative analysis of colocalization between EdU and gammaH2AX signals based on the calculation of the Replication Related Damage Distribution Index (RDDI) on confocal metaphase images was performed. RDDI revealed a colocalization between EdU and gammaH2AX signals both in control and bleomycin-treated CHO9 metaphases, suggesting that replication may be involved in H2AX phosphorylation. The possible mechanisms implicated are discussed.
Asunto(s)
Cromatina , Cromosomas/genética , Replicación del ADN , Histonas/metabolismo , Metafase , Animales , Células CHO , Cricetinae , Cricetulus , Daño del ADN , Reparación del ADN , Histonas/genéticaRESUMEN
Na avicultura, a avaliação de fertilidade em machos é de extrema importância, para garantir uma melhor produção de ovos férteis. As técnicas para avaliação de fertilidade em galos são pouco exploradas, sendo que na maioria das vezes, a avaliação é feita por amostragem e levando em consideração, apenas fatores morfofisiológicos, diretamente relacionados com o espermatozóide. Mas é sabido que, em outras espécies, além dos fatores morfofisiológicos, existem problemas intrínsecos ao espermatozóide, como a baixa compactação da cromatina, que pode levar a distúrbios de fertilidade, que na maioria das vezes não são diagnosticados. O objetivo desse trabalho foi a adaptação de técnicas de avaliação da cromatina, já descritas em outras espécies, para aves de linhagem pesada (Gallus gallus, Linnaeus, 1758), correlacionando as alterações cromatínicas com as alterações morfológicas e com a fertilidade. Para tanto, sêmen de galo com diferentes níveis de fertilidade, foram utilizados em diferentes métodos para identificação de alterações na cromatina, utilizando os corantes azul de toluidina e alaranjado de acridina. As avaliações demonstraram que esfregaços de sêmen fresco de galo com posterior fixação geram artefatos que levam a alterações na forma da cabeça e na integridade da cromatina, não sendo indicados em métodos de avaliação de fertilidade. Apesar de todos os métodos testados apresentarem falhas metodológicas e um certo grau de subjetividade, o método que gerou melhores resultados foi a mistura de uma gota de sêmen conservado em formol salina e uma gota do alaranjado de acridina sobre lâmina de microscopia, com posterior secagem e observação em microscopia de fluorescência com filtro de excitação azul. (AU)
In poultry breeding, male fertility has extreme importance to assure a better production of fertile eggs. Evaluation techniques for fertility of fowls are not well explored and in most cases, the evaluation is done through sampling considering only morphophysiological factors directly related with the spermatozoon. It's known that in other species, besides morphophysiological factors, there are intrinsic problems to the spermatozoon such as less chromatin condensation that can lead to fertility problems that in most cases are not diagnosised. The purpose of this work was the adaptation of techniques of chromatin evaluation for chicken (Gallus Gallus, Linnaeus, 1758) which have already been described in other species, correlating the chromatin alterations with the morphological alterations and the fertility. Fowl semen samples with different levels of fertility were used for test different methods to identify chromatin alterations using toluidine blue and acridine orange die. Evaluations have shown that smears of fresh semen with posterior fixation generate artfacts that change the head shape and the chromatin integrity not being indicated in methods of fertility evaluation. Although all the tested methods have presented methodology imperfections and some certain degree of subjectivity, the method that has generated best results was the mixture of one semen drop conserved in buffered phormol and a drop of acridine orange on microscopy slide with posterior staining and observation in fluorescence microscopy with blue excitation filter. Through this method it was verified that alterations in the chromatin condensation of fowl spermatozoa are generally not followed by morphological alterations and that generally the morphologic alterations of fowl spermatozoa are generally followed by alterations in chromatin condensation. This is an important factor in the determination of the fowl fertility.(AU)
Asunto(s)
Fertilidad/fisiología , Espermatozoides/fisiología , Técnicas y Procedimientos Diagnósticos/veterinaria , Semen/fisiología , AvesRESUMEN
O espermograma é um dos principais métodos de avaliação da fertilidade em mamíferos, contudo, algumas alterações do sêmen como a compactação da cromatina dos espermatozóides, não são identificadas nessa rotina, podendo interferir significativamente na fertilidade de reprodutores. Na avicultura, geralmente a avaliação de reprodutores é feita por amostragem e os parâmetros avaliados são em menor número que em mamíferos, sendo que a compactação da cromatina dos espermatozóides de galo nunca foi explorada. Este trabalho teve como objetivo verificar através da microscopia eletrônica de transmissão, se existe diferentes intensidades de compactação de cromatina em espermatozóides de galo. Para isto, foram coletadas 20 amostras de sêmen de galo, que foram fixadas por 48 horas em glutaraldeído 4% tamponado em cacodilato de sódio 0,1M a pH 7,2, após centrifugado e lavado em tampão cacodilato o sêmen foi pós-fixados em tetróxido de ósmio a 1% mais ferrocianeto de potássio a 1,25%. O sedimento foi incluído, cortado e posteriormente contrastado. Os cortes foram examinados e documentados em microscópio eletrônico Zeiss EM-109. Geralmente, os espermatozóides de galo possuem acrossoma com material homogêneo ou levemente granular e de densidade moderada, o núcleo com cromatina densa e levemente granular, varia as tonalidades de cinza, ou seja, os graus de compactação. Observou-se também o perforatorium, estrutura que une o núcleo ao acrossoma. A inserção da cauda é por meio de dois centríolos, sendo um transversal e o outro longitudinal ao eixo. A peça intermediária possui axonema típico envolto por mitocôndrias aparentemente dispostas longitudinalmente. A transição entre as peças intermediária e principal da cauda é marcada pela ausência das mitocôndrias. A peça principal é formada pelo axonema envolto por uma camada de citoplasma granular.(AU)
The spermiogram is one of the principal methods of evaluation of the fertility in mammals; however some semen modifications as the spermatozoa chromatin condensation, are not identified in this routine, and can expressively interfere in the fertility of reproducers. In poultry breeding, generally the evaluation of reproducers is made by sampling and the evaluated parameters are in fewer quantities than in mammals, considering the spermatozoa chromatin condensation of the fowl has never been exploited. The objective of this work is verifying through the transmission electron microscopy, whether there are different intensities of spermatozoa chromatin condensation of fowl. So that, have been collected 20 samples of fowl semen, which were placed in 4% glutaraldehyde buffered in 0.1M sodium cacodilate to pH 7.2 for 48 hours, after being centrifugated and rinsed in cacodilate tampon, the semen was post-fixed in 1 % osmium tetroxide plus 1.25% potassium ferrocyanide. The sediment was embedded, cut and contrasted. The thin sections were examined and documented in transmission electronic microscopy Zeiss EM -109. Generally the fowl spermatozoon has acrosome with homogenic or slightly granular and of moderate density material, the nucleus with dense or slightly granular chromatin, varies the gray scales, that is, the grades of condensation. It was also observed the "perforatorium", structure that links the nucleus to the acrosome. The insertion of the tail is made through two cetriules, being one transversal and the other longitudinal to the axle. The intermediate piece has typical axoneme involved by mitochondrias, apparently displayed longitudinally. The transition between the principal and the intermediate pieces of the tail is marked by the absence of the mitochondrias. The principal piece is formed by axoneme involved by a granular cytoplasm layer.(AU)