Your search keyword '"Saad, Sara Teresinha"' showing total 506 results

501. Simple fluorescent PCR method for detection of large deletions in the beta-globin gene cluster.

Author

De Andrade TG, Saad ST, Sonati Mde F, and Costa FF

Subjects

Africa ethnology, Brazil, Fetal Hemoglobin analysis, Fluorescent Dyes, Hematologic Diseases genetics, Humans, Thalassemia genetics, Gene Deletion, Globins genetics, Polymerase Chain Reaction methods

Abstract

We developed a semi-automated approach to detect large deletions in the beta-globin gene cluster, based on the quantitative differences in the amplifications of samples by a fluorescent PCR. With this strategy, we were able to detect the presence of HPFH-2 in an African-Brazilian subject, confirmed by sequencing analysis. Differently from other PCR strategies, GAP-PCR for example, it has the potential to identify new deletions., (Copyright 2003 Wiley-Liss, Inc.)

Published

2003

502. Long-term hydroxyurea therapy in beta-thalassaemia patients.

Author

de Paula EV, Lima CS, Arruda VR, Alberto FL, Saad ST, and Costa FF

Subjects

Adolescent, Adult, Aged, Blood Cell Count, Clinical Enzyme Tests, Creatine blood, Erythrocyte Indices drug effects, Fetal Hemoglobin drug effects, Hemoglobins drug effects, Humans, Hydroxyurea administration & dosage, Hydroxyurea toxicity, Liver enzymology, Male, Reticulocyte Count, Hydroxyurea therapeutic use, beta-Thalassemia drug therapy

Abstract

Objective: The study aimed to investigate the use of hydroxyurea (HU) for the treatment of beta-thalassaemia (beta-thal) patients., Methods: We examined the haematological effects of orally administered HU (10-20 mg/kg/d) in 11 patients, including four beta-thal major and seven beta-thal intermedia patients. Complete blood count and levels of foetal haemoglobin (HbF), liver enzymes and serum creatinine were evaluated before and during HU. Response to therapy was evaluated at 6 months of treatment., Results: A substantial increase in haemoglobin (Hb) level (4.1 g/dL), leading to complete withdrawal from a regular transfusion programme, was observed in one unique beta-thal major patient. In the beta-thal intermedia patients, increases in Hb level of 1.3, 1.9 and 2.0 g/dL were observed in three of seven (42.9%) patients during HU therapy. The mean values of Hb, mean corpuscular haemoglobin (MCH), and HbF were higher during HU treatment than baseline values (8.7 vs. 7.7 g/dL, P = 0.05; 26.7 vs. 22.9 pg, P = 0.05; 57.2 vs. 44.9%, P = 0.04; respectively). In contrast, the mean reticulocyte count measured during therapy decreased (97.0 x 10(9) vs. 632.0 x 10(9)/L, P = 0.03). No correlations were observed between levels of Hb and HbF (r = 0.77, P = 0.10), and levels of Hb and reticulocyte counts (r = 0.26, P = 0.31). No significant toxicity was observed in our patients., Conclusion: These results suggest that HU may improve Hb levels in beta-thal. Thus, we may conclude that a large trial concerning the response to HU in these patients should be carried out to clarify this issue.

Published

2003

503. Progesterone upregulates GATA-1 on erythroid progenitors cells in liquid culture.

Author

da Silva Santos Duarte A, Sales TS, Mengel JO, Costa FF, and Saad ST

Subjects

Cell Culture Techniques methods, DNA-Binding Proteins drug effects, Erythroid-Specific DNA-Binding Factors, GATA1 Transcription Factor, Globins drug effects, Globins genetics, Humans, NF-E2 Transcription Factor, NF-E2 Transcription Factor, p45 Subunit, RNA, Messenger analysis, RNA, Messenger biosynthesis, Transcription Factors drug effects, DNA-Binding Proteins genetics, Erythroid Precursor Cells metabolism, Progesterone pharmacology, Transcription Factors genetics, Up-Regulation drug effects

Abstract

Steroids hormones modify the hematological features of homozygous sickle cell disease, including the levels of fetal hemoglobin. We used semi-quantitative RT-PCR analysis of GATA-1, GATA-2, NF-E2, and gamma-globin mRNA levels in a two-phase liquid culture system of human adult erythroid cells in order to assay the effect of progesterone upon gene expression. The levels of expression of GATA-1 and gamma-globin mRNA were significantly increased in cells treated with progesterone compared to untreated cells (1.7- to 2.0-fold). Progesterone treatment did not produce any stimulatory effect upon GATA-2 and NF-E2 mRNA expression. Differences in the synthesis of HbF protein could not be detected by flow cytometry, although we observed a small difference in mean intensity fluorescence between cells treated and cells untreated with progesterone on days 7 and 9. Using anti-transferrin receptor and anti-glycophorin A antibodies, we verified that addition of progesterone did not cause any change in erythroid proliferation and differentiation. In conclusion, it is possible that the increased expression of gamma-globin mRNA after progesterone treatment observed in this study may be related to the increased GATA-1 mRNA expression. Interactions of the steroid receptors with the basal transcriptional machinery and with transcription factors might mediate their transcriptional effects.

Published

2002

504. ARHGAP10, a novel human gene coding for a potentially cytoskeletal Rho-GTPase activating protein.

Author

Bassères DS, Tizzei EV, Duarte AA, Costa FF, and Saad ST

Subjects

Base Sequence, Brain metabolism, Cell Differentiation genetics, Cloning, Molecular, Cytoskeletal Proteins metabolism, DNA, Complementary analysis, DNA, Complementary genetics, GTPase-Activating Proteins biosynthesis, HL-60 Cells, Humans, Molecular Sequence Data, Muscles metabolism, Organ Specificity, rhoA GTP-Binding Protein, Cytoskeletal Proteins genetics, GTPase-Activating Proteins genetics, Genome, Human

Abstract

Rho-GTPase activating proteins (Rho-GAPs) are negative regulators of Rho-GTPase signaling pathways related to actin cytoskeleton dynamics, cell proliferation, and differentiation. We have identified a novel human gene, termed ARHGAP10, that codes for a 1957-aminoacid Rho-GAP, containing a PDZ, a PH, and a Rho-GAP domain. The cDNA is 7118 bp long and has an open reading frame of 5874 bp. A computational analysis located this gene on chromosome 10 band 10p12.32 suggesting that it is composed of 25 exons. Northern analysis revealed that it is widely expressed, with high levels in brain and muscle. Real-time quantitative PCR analysis confirmed an increase in ARHGAP10 expression during differentiation of HL-60 cells with all-trans-retinoic acid and hematopoietic stem cells with erythropoietin, suggesting that this gene could play a role in normal hematopoiesis. The fact that this gene is highly expressed in muscle and brain, which are highly differentiated tissues, further supports the hypothesis that ARHGAP10 is important for cell differentiation.

Published

2002

505. Molecular heterogeneity of G6PD deficiency in an Amazonian population and description of four new variants.

Author

Hamel AR, Cabral IR, Sales TS, Costa FF, and Olalla Saad ST

Subjects

Amino Acid Substitution, Brazil epidemiology, DNA Mutational Analysis, Gene Frequency, Genetic Variation, Glucosephosphate Dehydrogenase analysis, Glucosephosphate Dehydrogenase genetics, Glucosephosphate Dehydrogenase Deficiency diagnosis, Haplotypes, Humans, Male, Point Mutation, Genetic Heterogeneity, Glucosephosphate Dehydrogenase Deficiency genetics

Abstract

To characterize the molecular variation in the glucose-6-phosphate dehydrogenase gene (G6PD), 196 asymptomatic and unrelated male G6PD-deficient blood donors from Belém, an Amazonian metropolis (Brazil), were analyzed. This deficiency was detected by horizontal agarose gel electrophoresis and quantitative spectrophotometric assay for enzyme activity. The mutations were searched by PCR/RFLP, SSCP, and direct DNA sequencing. The most frequent G6PD variant was the widespread and common G6PD A- (202G --> A, 376A --> G) observed in 161 subjects (82.1%). Besides this, we found another form of G6PD A- (968T --> C, 376A --> G) in 14 (7.1%) individuals, G6PD Seattle (844G --> C) in 4.6%, G6PD Santamaria (542A --> T, 376A --> G) in 2.5%, and G6PD Tokyo (1246G --> A) in one blood donor. Four novel variants were also identified: G6PD Belém (409C --> T; Pro137His), G6PD Ananindeua (376A --> G, 871G --> A; Asn126Asp, Val291Met), G6PD Crispim with four point mutations (375G --> T, 379G --> T, 383T --> C, and 384C --> T) leading to three amino acid substitutions (Met125Ile, Ala127Ser, and Leu128Pro), and G6PD Amazonia (185C --> A; Pro62His). The reported frequencies do not reflect the real values for blood donors from Belém, since an excess of individuals with "non A-" phenotype was included in this study to enhance the probability to find rare variants. Haplotype analyses were carried out for the less common G6PD variants identified in our study using PCR/RFLP for five polymorphic sites (FokI, PvuII, PstI, BclI, NlaIII). G6PD Crispim and G6PD Amazonia variants presented the most common haplotype found in G6PD B (- - + - -). G6PD Belém presented two haplotypes (- - + + +, - + + + +) and G6PD Ananindeua was found with the + - + - + haplotype. The reported heterogeneity probably is due to the great miscegenation, characteristic of the population of the Amazonian region, besides the apparently common occurrence of recurrent mutations in the G6PD gene.

Published

2002

506. High expression of apoptosis-regulating proteins in Burkitt's lymphomas.

Author

Pagnano KB, Silva MD, Vassallo J, Souza MS, Costa FF, and Saad ST

Subjects

Burkitt Lymphoma etiology, Burkitt Lymphoma pathology, Humans, Immunohistochemistry, Membrane Proteins metabolism, Myeloid Cell Leukemia Sequence 1 Protein, Neoplasm Proteins metabolism, Proto-Oncogene Proteins c-bcl-2 metabolism, bcl-2 Homologous Antagonist-Killer Protein, bcl-2-Associated X Protein, Apoptosis, Burkitt Lymphoma metabolism, Proto-Oncogene Proteins metabolism

Published

2002