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1.
Multiparameter Flow Cytometry Assay for Analysis of Nitrosative Stress Status in Human Spermatozoa.
Uribe, Pamela; Meriño, Juan; Manquemilla, Emilio; Villagrán, Camila; Vega, Etelinda; Zambrano, Fabiola; Schulz, Mabel; Pezo, Felipe; Villegas, Juana V; Boguen, Rodrigo; Sánchez, Raúl.
Cytometry A ; 97(12): 1238-1247, 2020 12.
Artigo em Inglês | MEDLINE | ID: mdl-32530108

RESUMO

Male infertility is an increasing health problem, and oxidative/nitrosative stress plays an important role in the etiology of this condition. Nitrosative stress due to excessive levels of reactive nitrogen species (RNS) is associated with impaired male fertility. Flow cytometry may be a useful tool for semen evaluation, but the availability of multiparameter assays for analysis of sperm quality is limited. The present study standardized a multiparameter flow cytometry analysis for nitrosative stress status in human spermatozoa in a single assay. A suitable multicolor fluorochrome panel was designed and consisted of fluorescein-boronate to detect peroxynitrite, a highly RNS, propidium iodide to analyze viability, tetramethylrhodamine methyl ester perchlorate to detect mitochondrial membrane potential (MMP) and monobromobimane to analyze thiol oxidation. Proper positive and negative controls for each fluorochrome were used to establish the technique, and sperm cells of different qualities and spermatozoa subjected to cryopreservation were analyzed. The results showed that the controls clearly discriminated between the high and low fluorescence intensities for each fluorochrome. The analysis of sperm cells of different quality demonstrated that the assay properly detected differences in all parameters analyzed according to sperm quality. The results may be reported as the mean fluorescence intensity of each fluorochrome and the percentage of cells exhibiting different characteristics. In conclusion, a protocol was standardized to analyze nitrosative stress status, including peroxynitrite production, viability, MMP, and thiol oxidation, in a single analysis using flow cytometry. This protocol may be applied to research approaches and clinical andrology to improve the evaluation of sperm quality and provide a promising tool to increase the use of clinical flow cytometry. © 2020 International Society for Advancement of Cytometry.


Assuntos
Estresse Nitrosativo , Espermatozoides , Criopreservação , Citometria de Fluxo , Humanos , Masculino , Potencial da Membrana Mitocondrial , Espermatozoides/metabolismo
2.
Utilidad del cariotipo y la citometría de flujo en el mieloma múltiple / Utility of karyotype and flow cytometry in multiple myeloma
Martínez Sánchez, Lina María; Álvarez Hernández, Luis Felipe; Ruiz Mejía, Camilo; Villegas Álzate, Juan Diego.
Rev. cuba. hematol. inmunol. hemoter ; 34(3): 1-16, jul.-set. 2018. tab
Artigo em Espanhol | LILACS, CUMED | ID: biblio-985531

Assuntos
Humanos , Cariótipo , Citometria de Fluxo/métodos , Mieloma Múltiplo/diagnóstico , Mieloma Múltiplo/epidemiologia , Mieloma Múltiplo/genética
3.
Multiparametric flow cytometry: a relevant tool for sperm function evaluation
Peña, F. J.
Anim. Reprod. (Online) ; 12(3): 351-355, July.-Sept.2015. graf
Artigo em Inglês | VETINDEX | ID: biblio-1461160

RESUMO

Nowadays in human and animal andrology flow cytometry is recognized as a robust tool for the evaluation of sperm quality and function. However, in this particular field, this technique has not reached the sophistication of other areas of biology and medicine. In recent years more sophisticated flow cytometers are being introduced in andrology laboratories, and the number of tests that can be potentially used in the evaluation of the sperm physiology has increased accordingly. In this review recent advances in the evaluation of sperm will be discussed; representing new techniques in flow cytometry, many of them able to measure simultaneously, in a single test, different degrees of damage in different sperm regions and/or changes in functionality.


Assuntos
Masculino , Animais , Citometria de Fluxo/métodos , Citometria de Fluxo/veterinária , Sêmen/citologia , Sêmen/fisiologia
4.
Multiparametric flow cytometry: a relevant tool for sperm function evaluation
Peña, F. J.
Anim. Reprod. ; 12(3): 351-355, July.-Sept.2015. graf
Artigo em Inglês | VETINDEX | ID: vti-26212

RESUMO

Nowadays in human and animal andrology flow cytometry is recognized as a robust tool for the evaluation of sperm quality and function. However, in this particular field, this technique has not reached the sophistication of other areas of biology and medicine. In recent years more sophisticated flow cytometers are being introduced in andrology laboratories, and the number of tests that can be potentially used in the evaluation of the sperm physiology has increased accordingly. In this review recent advances in the evaluation of sperm will be discussed; representing new techniques in flow cytometry, many of them able to measure simultaneously, in a single test, different degrees of damage in different sperm regions and/or changes in functionality.(AU)


Assuntos
Animais , Masculino , Citometria de Fluxo/métodos , Citometria de Fluxo/veterinária , Sêmen/citologia , Sêmen/fisiologia
5.
Galacto-oligosaccharides and lactulose as protectants against desiccation of Lactobacillus delbrueckii subsp. bulcaricus.
Santos, Mauricio I; Araujo-Andrade, Cuauhtémoc; Esparza-Ibarra, Edgar; Tymczyszyn, Elizabeth; Gómez-Zavaglia, Andrea.
Biotechnol Prog ; 30(5): 1231-8, 2014.
Artigo em Inglês | MEDLINE | ID: mdl-25098896

RESUMO

Lactobacillus delbrueckii subsp. bulgaricus CIDCA 333 was dehydrated on desiccators containing silica gel in the presence of 20% w/w of two types of galacto-oligosaccharides (GOS Biotempo and GOS Cup Oligo H-70®) and lactulose, until no changes in water desorption were detected. After rehydration, bacterial growth was monitored at 37°C by determining: (a) the absorbance at 600 nm and (b) the near infrared spectra (NIR). Principal component analysis (PCA) was then performed on the NIR spectra of samples dehydrated in all conditions. A multiparametric flow cytometry assay was carried out using carboxyfluorescein diacetate and propidium iodide probes to determine the relative composition of damaged, viable, and dead bacteria throughout the growth kinetics. The absorbance at 600 nm and the position of the second derivative band at ∼1370 nm were plotted against the time of incubation. The efficiency of the protectants was GOS Biotempo > GOS Cup Oligo H-70® > lactulose. The better protectant capacity of GOS Biotempo was explained on the basis of the lower contribution of damaged cells immediately after rehydration (t = 0). PCA showed three groups along PC1, corresponding to the lag, exponential and stationary phases of growth, which explained 99% of the total variance. Along PC2, two groups were observed, corresponding to damaged or viable cells. The results obtained support the use of NIR to monitor the recovery of desiccated microorganisms in real time and without the need of chemical reagents. The use of GOS and lactulose as protectants in dehydration/rehydration processes was also supported.


Assuntos
Galactanos/farmacologia , Lactobacillus delbrueckii/efeitos dos fármacos , Lactulose/farmacologia , Substâncias Protetoras/farmacologia , Sobrevivência Celular/efeitos dos fármacos , Desidratação , Citometria de Fluxo , Cinética , Lactobacillus delbrueckii/citologia , Lactobacillus delbrueckii/fisiologia , Reprodutibilidade dos Testes , Espectroscopia de Luz Próxima ao Infravermelho
6.
Análisis inmunofenotípico de muestras normales de médula ósea: aplicaciones en el control de calidad en los laboratorios de citometría / Immunophenotypic analysis of normal cell samples from bone marrow: applications in quality control of cytometry laboratories / Análise imunofenotípica de amostras de medula óssea normal: aplicações no controle de qualidade em laboratórios de citometria
Roa-Higuera, Diana Carolina; Fiorentino, Susana; Rodríguez-Pardo, Viviana Marcela; Campos-Arenas, Alba Myriam; Infante-Acosta, Elvira Antonia; Cardozo-Romero, Claudia Cecilia; Quijano-Gómez, Sandra Milena.
Univ. sci ; 15(3): 206-223, sep.-dic. 2010. ilus, tab
Artigo em Espanhol | LILACS-Express | LILACS | ID: lil-637348

RESUMO

Objetivo. Describir un protocolo estandarizado mediante citometría de flujo para cuantificar en términos absolutos y relativos distintas subpoblaciones celulares de médula ósea normal y analizar la expresión de diferentes marcadores celulares específicos de linaje cuya reactividad está asociada a la diferenciación celular para ser usado como parte del control de calidad de rutina en los laboratorios de citometría. Materiales y métodos. El análisis inmunofenotípico de distintas subpoblaciones celulares se realizó en muestras de MO normal empleando un panel de anticuerpos monoclonales y policlonales útiles para la caracterización fenotípica de leucemias agudas en 4 fluorescencias distintas, con un protocolo que combina marcaje celular de antígenos de membrana y de citoplasma. El análisis de expresión se realizó en términos de intensidad media de fluorescencia. Para el cálculo de recuentos absolutos se adicionaron esferas fluorescentes de concentración conocida. Resultados. El panel de anticuerpos utilizado permitió la identificación y cuantificación de las distintas subpoblaciones leucocitarias normales de origen linfoide y mieloide incluyendo células precursoras CD34+, y poblaciones celulares más diferenciadas incluidas en las líneas granulocítica, monocítica y eritroide. Se establecieron los valores de referencia de las poblaciones celulares y los rangos de expresión de los diferentes marcadores celulares importantes como parte del control de calidad de rutina en los laboratorios de citometría. Conclusión. Los patrones inmunofenotípicos identificados y la determinación de los valores absolutos y relativos de referencia de las distintas poblaciones leucocitarias normales en MO podrán ser utilizados por los laboratorios de citometría como modelo para establecer parámetros de referencia en el análisis fenotípico de neoplasias hematológicas.

Objective. To describe a standardized flow cytometry protocol for the relative and absolute quantification of hematopoietic cell subpopulations from normal bone marrow, and to evaluate the expression of different lineage-specific cell markers with a reactivity associated to cell differentiation to be used as part of the routine quality control in cytometry laboratories. Materials and methods. The immunophenotypical analysis of different cell subpopulations was done with samples from normal bone marrow using a panel of monoclonal and polyclonal antibodies useful in the characterization of acute leukemias with four different fluorescences, by means of a protocol that combines cell labeling of membrane and cytoplasm antigens. Expression analysis was done in terms of mean fluorescence intensity (MFI). Fluorescent beads at a known concentration were added for calculating the absolute count of cells. Results. The antibody panel used allowed the identification and quantification of different normal leukocyte subpopulations of lymphatic and myeloid origin, including CD34+ stem cells and more differentiated cell populations in the granulocytic, monocytic, and erythroid cell lines. We established reference values for cell populations and cell marker expression ranges as part of routine quality control of cytometry laboratories. Conclusion. Immunophenotypic patterns identified as well as absolute and relative reference values for the different normal leukocyte populations from bone marrow can be used by cytometry laboratories as a basis for establishing reference parameters in phenotypic analyses of hematologic neoplasia.

Objetivo. Descrever um protocolo padronizado por citometria de fluxo para quantificar em termos absolutos e relativos diferentes subpopulações de células de medula óssea normal e analisar a expressão de diferentes marcadores celulares de linhagem específica, cuja reatividade é associada com a diferenciação celular para ser usado como parte do controle de qualidade de rotina nos laboratórios de citometria de fluxo. Materiais e métodos. A análise imunofenotípica das subpopulações de células foi realizada em amostras de MO normais utilizando um painel de anticorpos monoclonais e policlonais úteis para a caracterização fenotípica de leucemia aguda em quatro fluorescências, com um protocolo que combina rotulagem celular de antígeno de membrana celular e de citoplasma. A análise de expressão foi realizada em termos de intensidade média de fluorescência. Para calcular a recontagem absoluta foram adicionadas esferas fluorescentes de concentração conhecida. Resultados. O painel de anticorpos utilizado permitiu a identificação e quantificação das subpopulações de leucócitos normais de origem linfóide e mielóide incluindo as células precursoras CD34+, e populações de células mais diferenciadas incluídas nas linhas granulocítica, monocítica e eritróide. Foram estabelecidos os valores de referência das populações celulares e os intervalos de expressão dos diferentes marcadores celulares importantes como parte da rotina de controle de qualidade em laboratórios de citometria. Conclusão. Os padrões imunofenotípicos identificados e a determinação dos valores absolutos e relativos de referência das diferentes populações de leucócitos normais em MOM podem ser utilizados pelos laboratórios de citometria como um modelo para estabelecer parâmetros de referencia na análise fenotípica de neoplasias hematológicas.

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