Your search keyword '"Ramírez-Lorca, Reposo"' showing total 7 results

1. Impact of aquaporin-4 and CD11c + microglia in the development of ependymal cells in the aqueduct: inferences to hydrocephalus

Author

Mayo, Francisco, González-Vinceiro, Lourdes, Hiraldo-González, Laura, Rodríguez-Gómez, Francisco D., Calle-Castillejo, Claudia, Mayo, Manuel, Netti, Vanina, Ramírez-Lorca, Reposo, and Echevarría, Miriam

Published

2024

2. An immunoassay that distinguishes real neuromyelitis optica signals from a labeling detected in patients receiving natalizumab.

Author

Gomar, Ismael Sánchez, Sánchez, María Díaz, Uclés Sánchez, Antonio José, Casado Chocán, José Luis, Ramírez-Lorca, Reposo, Serna, Ana, Villadiego, Javier, Toledo-Aral, Juan José, and Echevarría, Miriam

Subjects

NEUROMYELITIS optica, IMMUNOASSAY, NATALIZUMAB, DRUG side effects, PHARMACODYNAMICS, DIAGNOSIS

Abstract

Background Cell-based assays for neuromyelitis optica (NMO) diagnosis are the most sensitive and specific methods to detect anti-aquaporin 4 (AQP4) antibodies in serum, but some improvements in their quantitative and specificity capacities would be desirable. Thus the aim of the present work was to develop a sensitive quantitative method for detection of anti- AQP4 antibodies that allows clear diagnosis of NMO and distinction of false labeling produced by natalizumab treatment. Methods Sera from 167 individuals, patients diagnosed with NMO (16), multiple sclerosis (85), optic neuritis (24), idiopathic myelitis (21), or other neurological disorders (13) and healthy controls (8), were used as the primary antibody in an immunofluorescence assay on HEK cells transfected with the M23 isoform of human AQP4 fused with enhanced green fluorescent protein. Cells used were freshly transfected or stored frozen and then thawed just before adding the serum. Results Microscopic observation and fluorescence quantification produced similar results in fresh and frozen samples. Serum samples from patients diagnosed with NMO were 100% positive for anti-AQP4 antibodies, while all the other sera were negative. Using serum from patients treated with natalizumab, a small and unspecific fluorescent signal was produced from all HEK cells, regardless of AQP4 expression. Conclusions Our cell-based double-label fluorescence immunoassay protocol significantly increases the signal specificity and reduces false diagnosis of NMO patients, especially in those receiving natalizumab treatment. Frozen pretreated cells allow faster detection of anti-AQP4 antibodies. [ABSTRACT FROM AUTHOR]

Published

2014

3. The membrane-spanning 4-domains, subfamily A (MS4A) gene cluster contains a common variant associated with Alzheimer's disease.

Author

Antúnez, Carmen, Boada, Mercè, González-Pérez, Antonio, Gayán, Javier, Ramírez-Lorca, Reposo, Marín, Juan, Hernández, Isabel, Moreno-Rey, Concha, Morón, Francisco Jesús, López-Arrieta, Jesús, Mauleón, Ana, Rosende-Roca, Maitée, Noguera-Perea, Fuensanta, Legaz-García, Agustina, Vivancos-Moreau, Laura, Velasco, Juan, Carrasco, José Miguel, Alegret, Montserrat, Antequera-Torres, Martirio, and Manzanares, Salvadora

Subjects

ALZHEIMER'S disease, PRESENILE dementia, CLEAN rooms, META-analysis, GENES

Abstract

Background: In order to identify novel loci associated with Alzheimer's disease (AD), we conducted a genomewide association study (GWAS) in the Spanish population. Methods: We genotyped 1,128 individuals using the Affymetrix Nsp I 250K chip. A sample of 327 sporadic AD patients and 801 controls with unknown cognitive status from the Spanish general population were included in our initial study. To increase the power of the study, we combined our results with those of four other public GWAS datasets by applying identical quality control filters and the same imputation methods, which were then analyzed with a global meta-GWAS. A replication sample with 2,200 sporadic AD patients and 2,301 controls was genotyped to confirm our GWAS findings. Results: Meta-analysis of our data and independent replication datasets allowed us to confirm a novel genomewide significant association of AD with the membrane-spanning 4-domains subfamily A (MS4A) gene cluster (rs1562990, P = 4.40E-11, odds ratio = 0.88, 95% confidence interval 0.85 to 0.91, n = 10,181 cases and 14,341 controls). Conclusions: Our results underscore the importance of international efforts combining GWAS datasets to isolate genetic loci for complex diseases. [ABSTRACT FROM AUTHOR]

Published

2011

4. Genetic Structure of the Spanish Population.

Author

Gayán, Javier, Galan, José J., González-Pérez, Antonio, Sáez, María Eugenia, Martínez-Larrad, María Teresa, Zabena, Carina, Rivero, M. Carmen, Salinas, Ana, Ramírez-Lorca, Reposo, Morón, Francisco J., Royo, Jose Luis, Moreno-Rey, Concha, Velasco, Juan, Carrasco, José M., Molero, Eva, Ochoa, Carolina, Ochoa, María Dolores, Gutiérrez, Marta, Reina, Mercedes, and Pascual, Rocío

Subjects

HUMAN population genetics, BIOLOGICAL variation, LINKAGE disequilibrium, POPULATION research

Abstract

Background: Genetic admixture is a common caveat for genetic association analysis. Therefore, it is important to characterize the genetic structure of the population under study to control for this kind of potential bias. Results: In this study we have sampled over 800 unrelated individuals from the population of Spain, and have genotyped them with a genome-wide coverage. We have carried out linkage disequilibrium, haplotype, population structure and copy-number variation (CNV) analyses, and have compared these estimates of the Spanish population with existing data from similar efforts. Conclusions: In general, the Spanish population is similar to the Western and Northern Europeans, but has a more diverse haplotypic structure. Moreover, the Spanish population is also largely homogeneous within itself, although patterns of micro-structure may be able to predict locations of origin from distant regions. Finally, we also present the first characterization of a CNV map of the Spanish population. These results and original data are made available to the scientific community. [ABSTRACT FROM AUTHOR]

Published

2010

5. Interaction between Calpain 5, Peroxisome proliferator-activated receptor-gamma and Peroxisome proliferator-activated receptor-delta genes: a polygenic approach to obesity.

Author

Sáez, María E., Grilo, Antonio, Morón, Francisco J., Manzano, Luis, Martínez-Larrad, María T., González-Pérez, Antonio, Serrano-Hernando, Javier, Ruiz, Agustín, Ramírez-Lorca, Reposo, and Serrano-Ríos, Manuel

Subjects

OBESITY treatment, PEROXISOMES, NUCLEAR receptors (Biochemistry), BODY mass index, GENES

Abstract

Context: Obesity is a multifactorial disorder, that is, a disease determined by the combined effect of genes and environment. In this context, polygenic approaches are needed. Objective: To investigate the possibility of the existence of a crosstalk between the CALPAIN 10 homologue CALPAIN 5 and nuclear receptors of the peroxisome proliferator-activated receptors family. Design: Cross-sectional, genetic association study and gene-gene interaction analysis. Subjects: The study sample comprise 1953 individuals, 725 obese (defined as body mass index ≥ 30) and 1228 non obese subjects. Results: In the monogenic analysis, only the peroxisome proliferator-activated receptor delta (PPARD) gene was associated with obesity (OR = 1.43 [1.04-1.97], p = 0.027). In addition, we have found a significant interaction between CAPN5 and PPARD genes (p = 0.038) that reduces the risk for obesity in a 55%. Conclusion: Our results suggest that CAPN5 and PPARD gene products may also interact in vivo. [ABSTRACT FROM AUTHOR]

Published

2008

6. Calpain-5 gene variants are associated with diastolic blood pressure and cholesterol levels.

Author

Sáez, María E., Martínez-Larrad, María T., Ramírez-Lorca, Reposo, González-Sánchez, José L., Zabena, Carina, Martinez-Calatrava, María J., González, Alejandro, Morón, Francisco J., Ruiz, Agustín, and Serrano-Ríos, Manuel

Subjects

CALPAIN, GENES, BLOOD pressure, BLOOD cholesterol, CARDIOVASCULAR diseases, METABOLIC syndrome

Abstract

Background: Genes implicated in common complex disorders such as obesity, type 2 diabetes mellitus (T2DM) or cardiovascular diseases are not disease specific, since clinically related disorders also share genetic components. Cysteine protease Calpain 10 (CAPN10) has been associated with T2DM, hypertension, hypercholesterolemia, increased body mass index (BMI) and polycystic ovary syndrome (PCOS), a reproductive disorder of women in which isunlin resistance seems to play a pathogenic role. The calpain 5 gene (CAPN5) encodes a protein homologue of CAPN10. CAPN5 has been previously associated with PCOS by our group. In this new study, we have analysed the association of four CAPN5 gene variants(rs948976A>G, rs4945140G>A, rs2233546C>T and rs2233549G>A) with several cardiovascular risk factors related to metabolic syndrome in general population. Methods: Anthropometric measurements, blood pressure, insulin, glucose and lipid profiles were determined in 606 individuals randomly chosen from a cross-sectional population-based epidemiological survey in the province of Segovia in Central Spain (Castille), recruited to investigate the prevalence of anthropometric and physiological parameters related to obesity and other components of the metabolic syndrome. Genotypes at the four polymorphic loci in CAPN5 gene were detected by polymerase chain reaction (PCR). Results: Genotype association analysis was significant for BMI (p ≤ 0.041), diastolic blood pressure (p = 0.015) and HDL-cholesterol levels (p = 0.025). Different CAPN5 haplotypes were also associated with diastolic blood pressure (DBP) (0.0005 ≤ p ≤ 0.006) and total cholesterol levels (0.001 p ≤ 0.029). In addition, the AACA haplotype, over-represented in obese individuals, is also more frequent in individuals with metabolic syndrome defined by ATPIII criteria (p = 0.029). Conclusion: As its homologue CAPN10, CAPN5 seems to influence traits related to increased risk for cardiovascular diseases. Our results also may suggest CAPN5 as a candidate gene for metabolic syndrome. [ABSTRACT FROM AUTHOR]

Published

2007

7. An immunoassay that distinguishes real neuromyelitis optica signals from a labeling detected in patients receiving natalizumab.

Author

Sánchez Gomar, Ismael, Díaz Sánchez, María, Uclés Sánchez, Antonio José, Casado Chocán, José Luis, Ramírez-Lorca, Reposo, Serna, Ana, Villadiego, Javier, Toledo-Aral, Juan José, and Echevarría, Miriam

Abstract

Background: Cell-based assays for neuromyelitis optica (NMO) diagnosis are the most sensitive and specific methods to detect anti-aquaporin 4 (AQP4) antibodies in serum, but some improvements in their quantitative and specificity capacities would be desirable. Thus the aim of the present work was to develop a sensitive quantitative method for detection of anti-AQP4 antibodies that allows clear diagnosis of NMO and distinction of false labeling produced by natalizumab treatment.Methods: Sera from 167 individuals, patients diagnosed with NMO (16), multiple sclerosis (85), optic neuritis (24), idiopathic myelitis (21), or other neurological disorders (13) and healthy controls (8), were used as the primary antibody in an immunofluorescence assay on HEK cells transfected with the M23 isoform of human AQP4 fused with enhanced green fluorescent protein. Cells used were freshly transfected or stored frozen and then thawed just before adding the serum.Results: Microscopic observation and fluorescence quantification produced similar results in fresh and frozen samples. Serum samples from patients diagnosed with NMO were 100% positive for anti-AQP4 antibodies, while all the other sera were negative. Using serum from patients treated with natalizumab, a small and unspecific fluorescent signal was produced from all HEK cells, regardless of AQP4 expression.Conclusions: Our cell-based double-label fluorescence immunoassay protocol significantly increases the signal specificity and reduces false diagnosis of NMO patients, especially in those receiving natalizumab treatment. Frozen pretreated cells allow faster detection of anti-AQP4 antibodies. [ABSTRACT FROM AUTHOR]

Published

2014