Your search keyword '"Gazito, D."' showing total 19 results

1. Screening of Rare Donors Using a Single PCR Multiplex SNaPshot Reaction for Detection of 16 Blood Group Alleles: SP272

Author

Latini, F, Gazito, D, Arnoni, C, Muniz, J G, Person, R, Carvalho, F O, Baleotti, W, Castilho, L, and Barreto, J

Published

2012

2. Alcohol metabolizing gene polymorphisms and their relationship with oral cancer risk and clinicopathological features

Author

Takamori, J. T., Santos, Marcelo dos, Peterle, G. T., Rossi, L., Curioni, O. A., Gazito, D., Maia, L. L., Louro, I. D., Oliveira, M. M. de, Santos, J. G. dos, Moyses, R. A., Cury, P. M., Toporcov, T. N., Kanda, J. L., Silva, A. M. A. da, and Carvalho, M. B. de

Subjects

Lymph node metastasis, Oral cancer, ADH, ALDH, Polymorphism

Abstract

Oral cancer incidence is higher in individuals between the fifth and seventh decades of life, but some studies indicate a decreasing age trend. From the epidemiological point of view, alcohol consumption is associated with the emergence of oral cancer by interfering with mechanisms of DNA synthesis and repair. From a genetic standpoint, variant alleles in genes encoding the enzymes of alcohol (CYP2E1 and ADH) and acetaldehyde (ALDH2) metabolism may play an important role in the genesis of oral cancer. This study aimed to assess the relation of polymorphisms ADH1B (rs1229984 and rs2066702), ADH1C (rs698), ALDH2 (rs671) and CYP2E1 96bp insertion and the risk of squamous cell carcinoma of the mouth floor, as well as its clinicopathological and prognostic characteristics in relation to alcohol consumption. Our sample group was made of 301 patients, with 159 controls without a previous history of cancer and 142 patients with oral cancer. Genomic DNA was extracted from peripheral blood samples and genotypes were determined by PCR-RFLP. Our results suggest that the presence of ALDH2 Lys504 allele and 96bp insertion CYP2E1 were significantly associated with oral cancer risk. ADH1C gene Ile350 allele was associated with the presence of positive lymph nodes, and lymphatic invasion was related to the presence of polymorphic alleles ADH1B*1, ADH1C Ile350 and ALDH2 Lys504. In conclusion, these results reveal potential markers of oral cancer risk and behavior

Published

2017

3. Alcohol metabolizing gene polymorphisms and their relationship with oral cancer risk and clinicopathological features

Author

Takamori, J T, primary, Santos, M, additional, Peterle, G T, additional, Rossi, L, additional, Curioni, O A, additional, Gazito, D, additional, Maia, L L, additional, Louro, I D, additional, Oliveira, M M de, additional, Santos, J G dos, additional, Moyses, R A, additional, Cury, P M, additional, Toporcov, T N, additional, Kanda, J L, additional, Silva, A M A da, additional, and Carvalho, M B de, additional

Published

2017

4. Global gene expression profiling of oral cavity cancers suggests molecular heterogeneity within anatomic subsites

Author

Severino, Patricia, Alvares, Adriana M., Michaluart, Pedro, Okamoto, Oswaldo K., Nunes, Fabio D., Moreira-Filho, Carlos A., Tajara, Eloiza H., Cury, P. M., Frizzera, A. P.Z., de Carvalho, M. B., Silva, A. M.A., Amar, A., Barbieri, R. B., Bastos, A. U., Carvalho-Neto, P. B., Casemiro, A. F., Chedid, H., Chiappini, P. B.O., Correia, L. A., Costa, A. C.W., Curioni, O. A., Franzi, S. A., Gazito, D., Gutierres, A. P., Lehn, C. N., Martins, A. E., Mercante, A. M.C., Porsani, A. F., Rapoport, A., Rossi, L., Santos, M., Souza, T. B., Takamori, J. T., Dias-Neto, E., Ojopi, E. P.B., Dias, T. H.G., Figueiredo, D. L.A., Mamede, R. C.M., Fukuyama, E. E., Góis-Filho, J. F., Cerione, M., Cicco, R., Settani, F., Valentim, P. J., Yamagushi, F., Cominato, M. L., Mendes, G. S., Paiva, R., Silva, M. J., Leopoldino, A. M., Silva, F. A.M., Moyses, R. A., Arap, S. S., Araújo, N. S.S., Araújo-Filho, V., Brandão, L. G., Cernea, C. R., Durazzo, M., Ferraz, A. R., Gallo, J., Guimarães, P. E.M., Magalhães, R. P., Montenegro, F. L.M., Silva-Filho, G. B., Smith, R. B., Stabenow, E., Tavares, M. R., Turcano, R., Volpi, E. M., Ramos, O., Silva, C., Moreira-Filho, C. A., Nóbrega, F. G. [UNESP], Nóbrega, M. P. [UNESP], Canto, A. L. [UNESP], Macarenco, R. [UNESP], Meneses, C. [UNESP], Correa, P. M.S. [UNESP], Bogossian, A. P. [UNESP], Nunes, F. D., Souza, S. C.O.M., Rodini, C. O., Xavier, F. C.A., Okamoto, O. K., Serafini, L. N., Severino, P., Silva, W. A., Brandão, R. M., Kaneto, C. M., Pinheiro, D. G., Santos, A. R.D., Silva, I. T., Tarlá, M. V.C., Silveira, N. J.F., Tajara, E. H., Rodrigues-Lisoni, F. C., Rodrigues, R. V., Polachini, G. M., Vidotto, A., Cunha, B. R., Carmona-Raphe, J., Wünsch-Filho, V., Costa, A., Figueiredo, R. O., Fortes, C. S., Inamine, R., López, R. V.M., Rodrigues, A. N., Zago, M. A., Instituto Israelita de Ensino e Pesquisa Albert Einstein, Hospital Heliópolis, Universidade de São Paulo (USP), Universidade Federal de São Paulo (UNIFESP), Faculdade de Medicina de São José do Rio Preto, Faculdade de Medicina, Instituto do Câncer Arnaldo Vieira de Carvalho, Universidade Estadual Paulista (UNESP), Instituto de Ensino e Pesquisa Albert Einstein, and UNIVAP

Subjects

Medicine(all), Microarray, Cytoskeleton organization, business.industry, Biochemistry, Genetics and Molecular Biology(all), lcsh:R, Short Report, lcsh:Medicine, General Medicine, Disease, Cell cycle, Bioinformatics, General Biochemistry, Genetics and Molecular Biology, Gene expression profiling, stomatognathic diseases, lcsh:Biology (General), Gene expression, Gene chip analysis, Medicine, lcsh:Science (General), business, lcsh:QH301-705.5, Gene, lcsh:Q1-390

Abstract

Made available in DSpace on 2022-04-29T08:44:18Z (GMT). No. of bitstreams: 0 Previous issue date: 2008-01-01 Background: Oral squamous cell carcinoma (OSCC) is a frequent neoplasm, which is usually aggressive and has unpredictable biological behavior and unfavorable prognosis. The comprehension of the molecular basis of this variability should lead to the development of targeted therapies as well as to improvements in specificity and sensitivity of diagnosis. Results: Samples of primary OSCCs and their corresponding surgical margins were obtained from male patients during surgery and their gene expression profiles were screened using whole-genome microarray technology. Hierarchical clustering and Principal Components Analysis were used for data visualization and One-way Analysis of Variance was used to identify differentially expressed genes. Samples clustered mostly according to disease subsite, suggesting molecular heterogeneity within tumor stages. In order to corroborate our results, two publicly available datasets of microarray experiments were assessed. We found significant molecular differences between OSCC anatomic subsites concerning groups of genes presently or potentially important for drug development, including mRNA processing, cytoskeleton organization and biogenesis, metabolic process, cell cycle and apoptosis. Conclusion: Our results corroborate literature data on molecular heterogeneity of OSCCs. Differences between disease subsites and among samples belonging to the same TNM class highlight the importance of gene expression-based classification and challenge the development of targeted therapies. Centro de Pesquisa Experimental Instituto Israelita de Ensino e Pesquisa Albert Einstein Laboratório de Biologia Molecular Hospital Heliópolis Departamento de Cirurgia de Cabeça e Pescoço Hospital das Clínicas Faculdade de Medicina Universidade de São Paulo Departamento de Neurologia e Neurocirurgia Universidade Federal de São Paulo Departamento de Estomatologia Faculdade de Odontologia Universidade de São Paulo Departamento de Pediatria Faculdade de Medicina Universidade de São Paulo Departamento de Biologia Molecular Faculdade de Medicina de São José do Rio Preto Departamento de Genética e Biologia Evolutiva Instituto de Biociências Universidade de São Paulo Departamento de Patologia Faculdade de Medicina Hospital Heliópolis Departamento e Instituto de Psiquiatria Faculdade de Medicina USP Serviço de Cirurgia de Cabeça e Pescoço Faculdade de Medicina de Ribeirão Preto USP Serviço de Cirurgia de Cabeça e Pescoço Instituto do Câncer Arnaldo Vieira de Carvalho Departamento de Análises Clínicas Toxicológicas e Bromatológicas Faculdade de Ciências Farmacêuticas de Ribeirão Preto USP Departamento de Cirurgia de Cabeça e Pescoço Faculdade de Medicina USP Departamento de Pediatria Faculdade de Medicina USP Departamento de Biociências e Diagnóstico Bucal Faculdade de Odontologia UNESP Departamento de Estomatologia Faculdade de Odontologia USP Departamento de Neurologia e Neurocirurgia UNIFESP Departamento de Patologia Faculdade de Medicina de Ribeirão Preto USP Instituto de Ensino e Pesquisa Albert Einstein Departamento de Genética Faculdade de Medicina de Ribeirão Preto USP Ciências da Computação UNIVAP Departamento de Biologia Molecular Faculdade de Medicina Departamento de Epidemiologia Faculdade de Saúde Pública USP Departamento de Clínica Médica Faculdade de Medicina de Ribeirão Preto USP Departamento de Biociências e Diagnóstico Bucal Faculdade de Odontologia UNESP

Published

2008

5. A simple approach to screen rare donors in Brazil

Author

Arnoni, C.P., primary, Latini, F.R.M., additional, Muniz, J.G., additional, Person, R.D.M., additional, Vendrame, T.A.P., additional, Gazito, D., additional, and Castilho, L., additional

Published

2015

6. A simple approach to screen rare donors in Brazil

Author

Arnoni, C.P., Latini, F.R.M., Muniz, J.G., Person, R.D.M., Vendrame, T.A.P., Gazito, D., and Castilho, L.

Abstract

Providing blood units for patients with an antibody to a high-prevalence antigen or with multiple common antibodies is a constant challenge to the blood banks. Finding a compatible donor requires extensive screening, which incurs a large amount of investment. In this article, we share our experience of organizing a rare donor inventory with limited resources, we include the strategy used for finding rare donors, and we share the difficulties found during the implementation of the approach and the results obtained. Immunohematology2015;31:20–23.

Published

2019

7. SMIM1 polymorphisms in a donor population from southeast Brazil and their correlation with VEL expression.

Author

Arnoni CP, De Paula Vendrame TA, Muniz JG, Gazito D, De Medeiros Person RD, Pereira Cortez AJ, Latini FRM, and Castilho L

Subjects

Blood Group Antigens genetics, Brazil, Female, Gene Frequency, Humans, Male, Membrane Proteins metabolism, Alleles, Blood Donors, Blood Group Antigens biosynthesis, Gene Expression Regulation, Membrane Proteins genetics, Polymorphism, Single Nucleotide

Abstract

Background: Vel is a high frequency blood group antigen and its alloantibody is involved in haemolytic transfusion reactions. After elucidation of the molecular basis of the Vel-negative phenotype defined by a 17-base pair deletion in SMIM1, genotyping has been the technique of choice to identify the Vel-negative phenotype, and molecular investigations have contributed to explain Vel expression variability. The present study was aimed at screening for Vel negative blood donors and characterising the genetic changes found in Brazilian donors with altered Vel expression., Materials and Methods: Molecular screening for the SMIM1*64_80del allele was performed in 1,595 blood donor samples using a SNaPshot protocol previously standardised in our laboratory. Four hundred donor samples were also submitted to serological screening using a polyclonal anti-Vel from our inventory. Samples with variability in antigen strength were selected for SMIM1 sequencing., Results: No homozygous SMIM1*64_80del allele was found and the SMIM1*64_80del allele frequency was 1.01%. Different patterns of reactivity were observed in serological testing varying from negative to 3+. Through sequencing analysis we highlighted two polymorphisms: rs1175550 and rs6673829. The minor G allele of rs1175550 was found in 16/20 samples reacting 3+, while the major A allele was found in 21/23 samples reacting 2+. Regarding rs6673829, the minor A allele was present in 14/23 and 3/20 samples reacting 2+ and 3+ respectively., Discussion: We included molecular VEL screening in a previously standardised SNaPshot protocol, which besides enabling detection of Vel-negative donors, also searches for eight other rare blood types. Additionally, the present study demonstrated that although the SMIM1*64_80del allele is responsible for some variation of Vel phenotype in this donor population, Vel expression is also controlled by molecular changes in SMIM1 intron 2.

Published

2019

8. A novel KEL silencing allele in a Brazilian patient with anti-Ku.

Author

Brunetta D, Carlos LM, Costa TB, Silva VF, Oliveira PN, Gazito D, Arnoni C, and Castilho L

Subjects

Alleles, Brazil, Female, Gene Frequency genetics, Humans, Middle Aged, Kell Blood-Group System genetics

Published

2017

9. Prevalence of IFNL3 gene polymorphism among blood donors and its relation to genomic profile of ancestry in Brazil.

Author

Rizzo SR, Gazito D, Pott-Junior H, Latini FR, and Castelo A

Subjects

Brazil, Female, Genotype, Humans, Interferons, Male, Polymorphism, Single Nucleotide, Prevalence, Black People genetics, Blood Donors statistics & numerical data, Genomics, Interleukins genetics, White People genetics

Abstract

The recent development of interferon-free regimens based on direct-acting antivirals for the treatment of chronic hepatitis C virus infection has benefited many but not all patients. Some patients still experience treatment failure, possibly attributed to unknown host and viral factors, such as IFNL3 gene polymorphism. The present study assessed the prevalence of rs12979860-CC, rs12979860-CT, and rs12979860-TT genotypes of the IFNL3 gene, and its relationship with ancestry informative markers in 949 adult Brazilian healthy blood donors. Race was analyzed using ancestry informative markers as a surrogate for ancestry. IFNL3 gene was genotyped using the ABI TaqMan single nucleotide polymorphisms genotyping assays. The overall frequency of rs12979860-CC genotype was 36.9%. The contribution of African ancestry was significantly higher among donors from the northeast region in relation to southeast donors, whereas the influence of European ancestry was significantly higher in southeast donors. Donors with rs12979860-CC and rs12979860-CT genotypes had similar ancestry background. The contribution of African ancestry was higher among rs12979860-TT genotype donors in comparison to both rs12979860-CC and rs12979860-CT genotypes. The prevalence of rs12979860-CC genotype is similar to that found in the US, despite the Brazilian ancestry informative markers admixture. However, in terms of ancestry, rs12979860-CT genotype was much closer to rs12979860-CC individuals than to rs12979860-TT., (Copyright © 2016 Sociedade Brasileira de Infectologia. Published by Elsevier Editora Ltda. All rights reserved.)

Published

2016

10. Identification of four novel RHD alleles with altered expression of D in Brazilians.

Author

Arnoni CP, Muniz JG, de Paula Vendrame TA, Gazito D, de Medeiros Person R, Latini FR, and Castilho L

Subjects

Brazil, Exons genetics, Gene Frequency genetics, Genotype, Humans, Phenotype, Alleles, Rh-Hr Blood-Group System genetics

Published

2016

11. Novel RHAG allele encoding the Rh(null) phenotype in Brazil.

Author

Arnoni CP, Muniz JG, Gazito D, Person Rde M, Vendrame TA, Castilho L, and Latini FR

Subjects

Brazil, Female, Humans, Pregnancy, Alleles, Blood Proteins genetics, Codon, Terminator, Exons, Membrane Glycoproteins genetics

Abstract

Rhnull is a rare phenotype characterized by the loss of Rh antigen expression. This phenotype can be related to several molecular backgrounds. In this study, we show a novel allele in a Brazilian pregnant woman encoding the Rhnull phenotype due to a change in RHAG exon2 c.310C>T, which leads to a premature stop codon (Gln104Stop)., (© 2015 AABB.)

Published

2015

12. Frequency of Wr(a) antigen and anti-Wr(a) in Brazilian blood donors.

Author

Muniz JG, Arnoni CP, Gazito D, de Medeiros Person R, Vendrame TA, Latini FR, and Castilho L

Abstract

Background: Wr(a) is a low-incidence antigen, which is antithetical to the high prevalence red blood cell antigen, Wr(b). Anti-Wr(a) is a naturally occurring antibody that is found in approximately 1-2% of blood donors. The aim of this study was to determine the frequency of Wr(a) and anti-Wr(a) in Brazilian blood donors., Methods: A total of 1662 Brazilian blood donors were molecularly analyzed using the SNaPshot methodology to determine the WR*A/B alleles and to predict the frequency of the Wr(a) antigen. To detect the anti-Wr(a), samples from 1049 blood donors were analyzed using a gel test with Wr(a+) red blood cells. The serum was treated with dithiothreitol (DTT) to determine the immunoglobulin classes. Immunoglobulin (Ig)-G isotype classification was performed in a gel test using the IgG1/IgG3 card. A monocyte monolayer assay was employed to predict the clinical significance of IgG anti-Wr(a)., Results: Of the 1662 donors, only one sample had the DI*02.03 allele in heterozygous predicting the Wr(a+b+) phenotype. Anti-Wr(a) was detected in 34 (3.24%) samples, 64.7% in females and 35.3% in males. Regarding the immunoglobulin class, eight (23.5%) cases of anti-Wr(a) were classified as IgG and 26 (76.5%) as IgM. Of the eight cases of IgG anti-Wr(a), four were IgG1, two were IgG3 and three anti-Wr(a) were not IgG3 or IgG1, and thus probably IgG2 or IgG4. The results of the monocyte monolayer assay showed that IgG anti-Wr(a) might be of clinical significance., Conclusion: This study shows a very low frequency (0.06%) of the Wr(a) antigen in Brazilian blood donors. Additionally, it shows that the frequency of anti-Wr(a) in this population is higher than previously reported., (Copyright © 2015 Associação Brasileira de Hematologia, Hemoterapia e Terapia Celular. Published by Elsevier Editora Ltda. All rights reserved.)

Published

2015

13. Two novel KEL alleles encoding K0 phenotypes in Brazilians.

Author

Arnoni CP, Gazito D, Muniz JG, Person Rde M, Brandão F, Marques MG, Barreto JA, Castilho L, and Latini FR

Subjects

Alternative Splicing, Brazil, Codon, Nonsense, Exons genetics, Female, Genotype, Humans, Molecular Sequence Data, Phenotype, Point Mutation, Sequence Analysis, DNA, White People genetics, Kell Blood-Group System genetics, Membrane Glycoproteins genetics, Metalloendopeptidases genetics

Published

2014

14. How do we identify RHD variants using a practical molecular approach?

Author

Arnoni CP, Latini FR, Muniz JG, Gazito D, Person Rde M, de Paula Vendrame TA, Barreto JA, and Castilho L

Subjects

Algorithms, Blood Donors, Brazil, Gene Frequency, Humans, Molecular Diagnostic Techniques methods, Polymerase Chain Reaction methods, Polymorphism, Restriction Fragment Length, DNA Mutational Analysis methods, Polymorphism, Single Nucleotide, Rh-Hr Blood-Group System genetics

Abstract

Serologic resolution of Rh discrepancies due to partial D or weak D phenotypes is a frequent problem encountered during routine typing that can be solved by RHD genotyping because it provides better characterization of these variants. The objective of the current study was to develop algorithms for identification of D variants in multiethnic populations based on a logic sequence of molecular tests using a large number of atypical RhD specimens. Thus, a total of 360 blood samples with atypical D antigen expression were analyzed. A previously published multiplex polymerase chain reaction (PCR) procedure was performed and depending on multiplex PCR analysis, the associated RHCE allele, and D variant frequency in our population, an algorithm was developed composed of six flow charts using specific PCR-restriction fragment length polymorphism and/or specific exon sequencing. This strategy allowed the identification of 22 different variants with few assays and a much reduced cost. This study describes a simple and practical algorithm that we use to determine RHD genotypes in samples with unknown RHD. This strategy is relatively easy to implement and the algorithm can be adapted to populations with various ethnic backgrounds after an initial assessment of the type and frequency of D variants. Essentially, we demonstrate that sequencing of all RHD exons is not necessary for the identification of the majority of known D variants., (© 2014 AABB.)

Published

2014

15. A new strategy to identify rare blood donors: single polymerase chain reaction multiplex SNaPshot reaction for detection of 16 blood group alleles.

Author

Latini FR, Gazito D, Arnoni CP, Muniz JG, de Medeiros Person R, Carvalho FO, Baleotti W Jr, Castilho L, and Barreto JA

Subjects

Alleles, Blood Group Antigens analysis, Blood Grouping and Crossmatching economics, Brazil, Cost-Benefit Analysis, Costs and Cost Analysis, DNA Primers, Donor Selection economics, High-Throughput Nucleotide Sequencing economics, Humans, Polymerase Chain Reaction economics, Polymorphism, Restriction Fragment Length, Blood Donors, Blood Group Antigens genetics, Blood Grouping and Crossmatching methods, Donor Selection methods, Polymerase Chain Reaction methods, Polymorphism, Single Nucleotide

Abstract

Background: As an alternative to phenotyping, large-scale DNA-based assays, which are feasible for high-throughput donor red blood cell typing, were developed for determination of blood group polymorphisms. However, high-throughput genotyping platforms based on these technologies are still expensive and the inclusion of single nucleotide polymorphisms and analysis of the alleles depend on the manufacturer's determination. To overcome this limitation and in order to develop an assay to enable the screening of rare donors, we developed a SNaPshot assay for analysis of nine single nucleotide polymorphisms related to antigens that are difficult to assess using conventional serology., Materials and Methods: The single polymerase chain reaction multiplex SNaPshot reaction was optimized to identify nine single nucleotide polymorphisms determining 16 alleles: KEL*3/KEL*4, KEL*6/KEL*7, DI*1/DI*2, DI*3/DI*4, YT*1/YT*2, CO*1/CO*2, DO*1/DO*2, DO*4, DO*5. We designed a single multiplex PCR with primers encompassing the blood group single nucleotide polymorphisms and performed an internal reaction with probe primers able to discriminate the alleles after fragment analysis. The SNaPshot assay was validated with 140 known alleles previously determined by PCR restriction fragment length polymorphism., Results: We were able to simultaneous detect nine single nucleotide polymorphisms defining 16 blood group alleles on an assay based on a multiplex PCR combined with a single base extension using genomic DNA., Discussion: This study demonstrates a robust genotyping strategy for conducting rare donor screening which can be applied in blood centers and could be an important tool for identifying antigen-negative donors and, therefore, for providing rare blood.

Published

2014

16. An easy and efficient strategy for KEL genotyping in a multiethnic population.

Author

Arnoni CP, Muniz JG, de Paula TA, Person RD, Gazito D, Baleotti W Jr, Barreto JA, Castilho L, and Latini FR

Abstract

Background: The Kell blood group system expresses high and low frequency antigens with the most important in relation to transfusion including the antithetic KEL1 and KEL2; KEL3 and KEL4; KEL6 and KEL7 antigens. Kell is a clinically relevant system, as it is highly immunogenic and anti-KEL antibodies are associated with hemolytic transfusion reactions and hemolytic disease of the fetus and newborn. Although required in some situations, Kell antigen phenotyping is restricted due to technical limitations. In these cases, molecular approaches maybe a solution. This study proposes three polymerase chain reaction genotyping protocols to analyze the single nucleotide polymorphisms responsible for six Kell antithetic antigens expressed in a Brazilian population., Methods: DNA was extracted from 800 blood donor samples and three polymerase chain reaction-restriction fragment length polymorphism protocols were used to genotype the KEL*1/KEL*2, KEL*3/KEL*4 and KEL*6/KEL*7 alleles. KEL*3/KEL*4 and KEL*6/KEL*7 genotyping was standardized using the NlaIII and MnlI restriction enzymes and validated using sequencing. KEL*1/KEL*2 genotyping was performed using a previously reported assay., Results: KEL genotyping was successfully implemented in the service; the following distribution of KEL alleles was obtained for a population from southeastern Brazil: KEL*1 (2.2%), KEL*2 (97.8%), KEL*3 (0.69%), KEL*4 (99.31%), KEL*6 (2.69%) and KEL*7 (97.31%). Additionally, two individuals with rare genotypes, KEL*1/KEL*1 and KEL*3/KEL*3, were identified., Conclusion: KEL allele genotyping using these methods proved to be reliable and applicable to predict Kell antigen expressions in a Brazilian cohort. This easy and efficient strategy can be employed to provide safer transfusions and to help in rare donor screening.

Published

2013

17. Prognostic significance of NDRG1 expression in oral and oropharyngeal squamous cell carcinoma.

Author

Dos Santos M, da Cunha Mercante AM, Nunes FD, Leopoldino AM, de Carvalho MB, Gazito D, López RV, Chiappini PB, de Carvalho Neto PB, Fukuyama EE, Tajara EH, Louro ID, and da Silva AM

Subjects

Adult, Aged, Biomarkers, Tumor genetics, Biomarkers, Tumor metabolism, Carcinoma, Squamous Cell mortality, Carcinoma, Squamous Cell secondary, Cell Cycle Proteins genetics, Female, Humans, Intracellular Signaling Peptides and Proteins genetics, Kaplan-Meier Estimate, Lymphatic Metastasis, Male, Middle Aged, Mouth Neoplasms mortality, Mouth Neoplasms pathology, Oropharyngeal Neoplasms mortality, Oropharyngeal Neoplasms pathology, Prognosis, Proportional Hazards Models, Tissue Array Analysis, Carcinoma, Squamous Cell metabolism, Cell Cycle Proteins metabolism, Gene Expression, Intracellular Signaling Peptides and Proteins metabolism, Mouth Neoplasms metabolism, Oropharyngeal Neoplasms metabolism

Abstract

Human N-myc downstream-regulated gene 1 (NDRG1) is a metastasis suppressor gene with several potential functions, including cell differentiation, cell cycle regulation and response to hormones, nickel and stress. The purpose of this study was to investigate the immunoexpression of NDRG1 in oral and oropharyngeal squamous cell carcinomas searching for its role in the clinical course of these tumors. We investigated immunohistochemical expression of NDRG1 protein in 412 tissue microarray cores of tumor samples from 103 patients with oral and oropharyngeal squamous cell carcinomas and in 110 paraffin-embedded surgical margin sections. The results showed NDRG1 up-regulation in 101/103 (98.1 %) tumor samples, but no expression in any normal tissue sample. Western blot assays confirmed the immunohistochemical findings, suggesting that lower levels of NDRG1 are associated with a high mortality rate. NDRG1 overexpression was related to long-term specific survival (HR = 0.38; p = 0.009), whereas the presence of lymph-node metastasis showed the opposite association with survival (HR = 2.45; p = 0.013). Our findings reinforce the idea that NDRG1 plays a metastasis suppressor role in oral and oropharyngeal squamous cell carcinomas and may be a useful marker for these tumors.

Published

2012

18. FGFR4 profile as a prognostic marker in squamous cell carcinoma of the mouth and oropharynx.

Author

Dutra RL, de Carvalho MB, Dos Santos M, Mercante AM, Gazito D, de Cicco R, Group G, Tajara EH, Louro ID, and da Silva AM

Subjects

Carcinoma, Squamous Cell genetics, Carcinoma, Squamous Cell pathology, Female, Gene Expression Regulation, Neoplastic, Genetic Predisposition to Disease genetics, Humans, Male, Middle Aged, Mouth Neoplasms genetics, Mouth Neoplasms pathology, Oropharyngeal Neoplasms genetics, Oropharyngeal Neoplasms pathology, Polymorphism, Single Nucleotide, Prognosis, Biomarkers, Tumor genetics, Carcinoma, Squamous Cell diagnosis, Mouth Neoplasms diagnosis, Oropharyngeal Neoplasms diagnosis, Receptor, Fibroblast Growth Factor, Type 4 genetics

Abstract

Background: Fibroblast growth factor receptor 4 (FGFR4) is a member of a receptor tyrosine kinase family of enzymes involved in cell cycle control and proliferation. A common single nucleotide polymorphism (SNP) Gly388Arg variant has been associated with increased tumor cell motility and progression of breast cancer, head and neck cancer and soft tissue sarcomas. The present study evaluated the prognostic significance of FGFR4 in oral and oropharynx carcinomas, finding an association of FGFR4 expression and Gly388Arg genotype with tumor onset and prognosis., Patients and Methods: DNA from peripheral blood of 122 patients with oral and oropharyngeal squamous cell carcinomas was used to determine FGFR4 genotype by PCR-RFLP. Protein expression was assessed by immunohistochemistry (IHC) on paraffin-embedded tissue microarrays., Results: Presence of allele Arg388 was associated with lymphatic embolization and with disease related premature death. In addition, FGFR4 low expression was related with lymph node positivity and premature relapse of disease, as well as disease related death., Conclusion: Our results propose FGFR4 profile, measured by the Gly388Arg genotype and expression, as a novel marker of prognosis in squamous cell carcinoma of the mouth and oropharynx.

Published

2012

19. Genomics and proteomics approaches to the study of cancer-stroma interactions.

Author

Rodrigues-Lisoni FC, Peitl P Jr, Vidotto A, Polachini GM, Maniglia JV, Carmona-Raphe J, Cunha BR, Henrique T, Souza CF, Teixeira RA, Fukuyama EE, Michaluart P Jr, de Carvalho MB, Oliani SM, Tajara EH, Cury PM, de Carvalho MB, Dias-Neto E, Figueiredo DL, Fukuyama EE, Góis-Filho JF, Leopoldino AM, Mamede RC, Michaluart-Junior P, Moyses RA, Nóbrega FG, Nóbrega MP, Nunes FD, Ojopi EF, Serafini LN, Severino P, Silva AM, Silva WA Jr, Silveira NJ, Souza SC, Tajara EH, Wünsch-Filho V, Amar A, Bandeira CM, Braconi MA, Brandão LG, Brandão RM, Canto AL, Cerione M, Cicco R, Chagas MJ, Chedid H, Costa A, Cunha BR, Curioni OA, Fortes CS, Franzi SA, Frizzera AP, Gazito D, Guimarães PE, Kaneto CM, López RV, Macarenco R, Magalhães MR, Meneses C, Mercante AM, Pinheiro DG, Polachini GM, Rapoport A, Rodini CO, Rodrigues-Lisoni FC, Rodrigues RV, Rossi L, Santos AR, Santos M, Settani F, Silva FA, Silva IT, Souza TB, Stabenow E, Takamori JT, Valentim PJ, Vidotto A, Xavier FC, Yamagushi F, Cominato ML, Correa PM, Mendes GS, Paiva R, Ramos O, Silva C, Silva MJ, and Tarlá MV

Subjects

Annexin A5 metabolism, Apoptosis, Cell Proliferation, Down-Regulation, Electrophoresis, Gel, Two-Dimensional, Fibroblasts metabolism, Genomics, Hep G2 Cells, Humans, Keratins metabolism, Mouth Neoplasms genetics, Nucleic Acid Hybridization, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Stromal Cells metabolism, Vimentin metabolism, Gene Expression Regulation, Neoplastic, Mouth Neoplasms metabolism, Proteome metabolism

Abstract

Background: The development and progression of cancer depend on its genetic characteristics as well as on the interactions with its microenvironment. Understanding these interactions may contribute to diagnostic and prognostic evaluations and to the development of new cancer therapies. Aiming to investigate potential mechanisms by which the tumor microenvironment might contribute to a cancer phenotype, we evaluated soluble paracrine factors produced by stromal and neoplastic cells which may influence proliferation and gene and protein expression., Methods: The study was carried out on the epithelial cancer cell line (Hep-2) and fibroblasts isolated from a primary oral cancer. We combined a conditioned-medium technique with subtraction hybridization approach, quantitative PCR and proteomics, in order to evaluate gene and protein expression influenced by soluble paracrine factors produced by stromal and neoplastic cells., Results: We observed that conditioned medium from fibroblast cultures (FCM) inhibited proliferation and induced apoptosis in Hep-2 cells. In neoplastic cells, 41 genes and 5 proteins exhibited changes in expression levels in response to FCM and, in fibroblasts, 17 genes and 2 proteins showed down-regulation in response to conditioned medium from Hep-2 cells (HCM). Nine genes were selected and the expression results of 6 down-regulated genes (ARID4A, CALR, GNB2L1, RNF10, SQSTM1, USP9X) were validated by real time PCR., Conclusions: A significant and common denominator in the results was the potential induction of signaling changes associated with immune or inflammatory response in the absence of a specific protein.

Published

2010