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4. The trehalose coating effect on the internal protein dynamics

Author

Hackel C., Zinkevich T., Belton P., Achilles A., Reichert D., and Krushelnitsky A.

Abstract

15N and 13C NMR experiments were applied to conduct a comparative study of a cold shock protein (Csp) in two states - lyophilized powder and a protein embedded in a glassy trehalose matrix. Both samples were studied at various levels of rehydration. The experiments used (measuring relaxation rates R 1 and R 1ρ, motionally averaged dipolar couplings and solid state exchange method detecting reorientation of the chemical shift anisotropy tensor) allow obtaining abundant information on the protein structural features and internal motions in a range of correlation times from nanoseconds to seconds. The main results are: (a) the trehalose coating makes the protein structure more native in comparison with the dehydrated lyophilized powder, however, trehalose still cannot remove all non-native hydrogen bonds which are present in a dehydrated protein; (b) trehalose has an appreciable effect on the internal dynamics: the motion of the backbone N-H groups in the nanosecond and microsecond time scales becomes slower while the motional amplitude remains constant; (c) upon adding water to the Csp-trehalose mixture, water molecules accumulate around proteins forming a layer between the protein surface and the trehalose matrix. The protein dynamics become faster, however, not as fast as in the fully hydrated state; (d) the hydration response of dynamics of the NH and CH(CH 2) groups in a protein is qualitatively different: upon increasing protein hydration, the correlation times of the N-H motions become shorter and the amplitude remains stable, and for CH(CH 2) groups the motional amplitude increases and the correlation times do not change. This can be explained by a different ability of the NH and CH(CH 2) groups to form hydrogen bonds. © the Owner Societies 2012.

Published
2012

5. Journal of Molecular Medicine

Author

Silva, D. N., Toralles, Maria Betânia Pereira, Hackel, C., Oliveira, L. E. C., Ferraz, L. F. C., Tonini, Maria Manuela de Oliveira, Stuchi-Perez, Eliana Gabas, and Guerra-Junior, G.

Abstract

Texto completo: acesso restrito. p. 569-576 Submitted by Edileide Reis (leyde-landy@hotmail.com) on 2013-11-20T13:51:39Z No. of bitstreams: 1 D. N. Silva.pdf: 216700 bytes, checksum: 90d6efed1ef96d76c2012845f66c2d3b (MD5) Approved for entry into archive by Rodrigo Meirelles (rodrigomei@ufba.br) on 2013-11-26T12:53:24Z (GMT) No. of bitstreams: 1 D. N. Silva.pdf: 216700 bytes, checksum: 90d6efed1ef96d76c2012845f66c2d3b (MD5) Made available in DSpace on 2013-11-26T12:53:24Z (GMT). No. of bitstreams: 1 D. N. Silva.pdf: 216700 bytes, checksum: 90d6efed1ef96d76c2012845f66c2d3b (MD5) Previous issue date: 2005 Mutations of the steroid 5α-reductase type 2 (SRD5A2) gene in 46,XY subjects cause masculinization defects of varying degrees, due to reduced or impaired enzymatic activity. In this study, sequence abnormalities of the SRD5A2 gene were assessed by polymerase chain reaction with specific primers and automated sequencing analysis in DNA samples from 20 patients with suspected steroid 5α-reductase type 2 deficiency from 18 Brazilian families. Eleven subjects presented SRD5A2 homozygous single-base mutations (two first cousins and four unrelated patients with G183S, two with R246W, one with del642T, one with G196S, and one with 217_218insC plus the A49T variant in heterozygosis), whereas four were compound heterozygotes (one with Q126R/IVS3+1G>A, one with Q126R/del418T, and two brothers with Q126R/G158R). Three patients were heterozygous for A207D, G196S, and R266W substitutions. The V89L polymorphism was found in heterozygosis in one of them (with A207D) and in one case with an otherwise normal gene sequence. The A49T variant was also detected in heterozygosis in the second case without other sequencing abnormalities. Four patients harbor yet non-described SRD5A2 gene mutations: a single nucleotide deletion (del642T), a G158R amino acid substitution, a splice junction mutation (IVS3+1G>A), and the insertion of a cytosine (217_218insC) occurring at a CCCC motif. This is the first report of a single-nucleotide insertion in the coding sequence of the SRD5A2 gene. In addition to these new mutations, this investigation reveals the prevalence of G183S substitution among a subset of African–Brazilian patients and presents evidences of the recurrence of already known mutations.

Published
2005
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6. A transcript finishing initiative for closing gaps in the human transcriptome

Author

Sogayar, M. C., Camargo, A. A., Bettoni, F., Carraro, D. M., Pires, L. C., Parmigiani, M. B., Ferreira, E. N., Moreira, E. S., Latorre, MRDO, Simpson, AJG, Cruz, L. O., Degaki, T. L., Festa, F., Massirer, K. B., Camargo, F., Camargo, L. P., Cunha, MAV, De Souza, S. J., Faria, M., Giuliatti, S., Kopp, Oliviera, PSL, Paiva, P. B., Pereira, A. A., Pinheiro, D. G., Puga, R. D., Souza, JES, Albuquerque, D. M., Andrade, LEC, Baia, G. S., Briones, MRS, Cavaleiro-Luna, AMS, Cerutti, J. M., Costa, F. F., Constanzi-Strauss, E., Espreafico, E. M., Ferrasi, A. C., Ferro, E. S., Fortes, MAHZ, Furchi, JRF, Gianella-Neto, D., Goldman, G. H., Goldman, MHS, Gruber, A., Guimaraes, G. S., Hackel, C., Henrique-Silva, F., Kimura, E. T., Leoni, S. G., Macedo, C., Malnic, B., Manzini, C. V., Marie, SKN, Martinez-Rossi, N. M., Menossi, M., Miracca, E. C., Nagai, M. A., Nobrega, F. G., Nobrega, M. P., Oba-Shinjo, S. M., Oliviera, M. K., Orabona, G. M., Otsuke, A. Y., Paco-Larson, M. L., Paixao, BMC, Pandolfi, JRC, Pardini, MIMC, Passos-Bueno, M. R., Passos, GAS, Pesquero, J. B., Pessoa, J. G., Rahal, Paula [UNESP], Rainho, C. A., Reis, C. P., Ricca, T. I., Rodriguez, V, Rogatto, Silvia Regina [UNESP], Romano, C. M., Romeiro, J. G., Rossi, A., Sa, R. G., Sales, M. M., SantAnna, S. C., Santarosa, P. L., Segato, F., Silva, W. A., Silva, IDCG, Silva, N. P., Soares-Costa, A., Sonati, M. F., Strauss, B. E., Tajara, E. H., Valentini, Sandro Roberto [UNESP], Villanova, F. E., Ward, L. S., Zanette, D. L., Universidade de São Paulo (USP), Ludwig Inst Canc Res, Univ Ribeirao Preto, Inst Ludwig, Universidade Federal de São Paulo (UNIFESP), Universidade Estadual de Campinas (UNICAMP), Universidade Estadual Paulista (Unesp), Universidade Federal de São Carlos (UFSCar), and Univ Vale Paraiba

Subjects
Transcription, Genetic, Software Validation, Molecular Sequence Data, Biology, Cell Line, Open Reading Frames, Exon, Software Design, Cell Line, Tumor, Complementary DNA, Consensus Sequence, Databases, Genetic, Methods, Genetics, Consensus sequence, Humans, Gene, Genetics (clinical), Expressed Sequence Tags, Expressed sequence tag, Genome, Human, Alternative splicing, Computational Biology, DNA, Neoplasm, U937 Cells, HISTOLOGIA, Alternative Splicing, Open reading frame, Genes, Human genome, Software, HeLa Cells
Abstract

Submitted by Guilherme Lemeszenski (guilherme@nead.unesp.br) on 2014-02-26T17:19:33Z No. of bitstreams: 1 WOS000222434200023.pdf: 392582 bytes, checksum: eb50adacff00ab5cc37867f0de853492 (MD5) Made available in DSpace on 2014-02-26T17:19:33Z (GMT). No. of bitstreams: 1 WOS000222434200023.pdf: 392582 bytes, checksum: eb50adacff00ab5cc37867f0de853492 (MD5) Previous issue date: 2004-07-01 Submitted by Vitor Silverio Rodrigues (vitorsrodrigues@reitoria.unesp.br) on 2014-05-20T13:50:12Z No. of bitstreams: 1 WOS000222434200023.pdf: 392582 bytes, checksum: eb50adacff00ab5cc37867f0de853492 (MD5) Made available in DSpace on 2014-05-20T13:50:12Z (GMT). No. of bitstreams: 1 WOS000222434200023.pdf: 392582 bytes, checksum: eb50adacff00ab5cc37867f0de853492 (MD5) Previous issue date: 2004-07-01 We report the results of a transcript finishing initiative, undertaken for the purpose of identifying and characterizing novel human transcripts, in which RT-PCR was used to bridge gaps between paired EST Clusters, mapped against the genomic sequence. Each pair of EST Clusters selected for experimental validation was designated a transcript finishing unit (TFU). A total of 489 TFUs were selected for validation, and an overall efficiency of 43.1% was achieved. We generated a total of 59,975 bp of transcribed sequences organized into 432 exons, contributing to the definition of the structure of 211 human transcripts. The structure of several transcripts reported here was confirmed during the course of this project, through the generation of their corresponding full-length cDNA sequences. Nevertheless, for 21% of the validated TFUs, a full-length cDNA sequence is not yet available in public databases, and the structure of 69.2% of these TFUs was not correctly predicted by computer programs. The TF strategy provides a significant contribution to the definition of the complete catalog of human genes and transcripts, because it appears to be particularly useful for identification of low abundance transcripts expressed in a restricted Set of tissues as well as for the delineation of gene boundaries and alternatively spliced isoforms. Univ São Paulo, Inst Quim, BR-05513970 São Paulo, Brazil Ludwig Inst Canc Res, BR-01509010 São Paulo, Brazil Univ São Paulo, Dept Epidemiol, Sch Publ Hlth, BR-01246904 São Paulo, SP, Brazil Univ Ribeirao Preto, Dept Quim Informat Bioinformat, BR-14096380 Ribeirao Preto, Brazil Univ São Paulo, Fac Med Ribeirao Preto, Centro Terapia Celular, Hemocentro, BR-14051140 Ribeirao Preto, SP, Brazil Univ São Paulo, Fac Med Ribeirao Preto, Dept Clin Med, BR-14051140 Ribeirao Preto, SP, Brazil Inst Ludwig, Lab Biol Computacional, BR-01509010 São Paulo, SP, Brazil Univ São Paulo, Lab Genet Cardiol Mol, Inst Coracao, BR-05403000 São Paulo, SP, Brazil Univ Fed São Paulo, Bioinform Lab, Hlth Informatics Dept, BR-04039032 São Paulo, Brazil Univ Estad Campinas, Dept Clin Med, Fac Ciências Med, BR-13083970 Campinas, SP, Brazil Univ Fed São Paulo, Rheumatol Div, BR-04113001 São Paulo, Brazil Univ São Paulo, Dept Histol Embriol, Inst Ciências Biomed, BR-05508900 São Paulo, Brazil Univ Fed São Paulo, Dept Microbiol Immunol Parasitol, BR-04023062 São Paulo, Brazil Univ São Paulo, Lab Cellular Mol Endocrinol, Sch Med, BR-01246903 São Paulo, Brazil Univ Fed São Paulo, Dept Med, Disciplina Endocrinol, Lab Endocrinol Mol, BR-04039002 São Paulo, Brazil Univ São Paulo, Inst Ciências Biomed, Lab Transferencia Genica, BR-05508900 São Paulo, Brazil Univ São Paulo, Fac Med Ribeirao Preto, Dept Biol Celular Mol Bioagentes Patogenicas, BR-14049900 Ribeirao Preto, SP, Brazil Univ Estadual Paulista, Lab Biol Mol, Hemocentro, Fac Med, BR-18618970 Botucatu, SP, Brazil Univ Fed Sao Carlos, Dept Genet Evol, BR-13565905 Sao Carlos, SP, Brazil Univ São Paulo, Fac Ciências Farmaceuticas Ribeirao Preto, BR-14040903 Ribeirao Preto, SP, Brazil Univ São Paulo, Fac Filosofia Ciências Letras Ribeirao Preto, Ribeirao Preto, SP, Brazil Univ São Paulo, Dept Patol, Fac Med Vet Zootecnia, BR-05508000 São Paulo, Brazil Univ Estadual Campinas, Dept Genet Med, Fac Ciências Med, BR-13081970 Campinas, SP, Brazil Univ São Paulo, Fac Med Ribeirao Preto, Dept Genet, BR-14040900 Ribeirao Preto, SP, Brazil Univ São Paulo, Dept Bioquim, Inst Quim, BR-05599970 São Paulo, Brazil Univ São Paulo, Dept Neurol, Fac Med, BR-01246903 São Paulo, Brazil Univ Estadual Campinas, Lab Genoma Funcional, Centro Biol Mol Engenharia Genet, BR-13083970 Campinas, SP, Brazil Univ Estadual Campinas, Dept Genet Evol, Inst Biol, Campinas, SP, Brazil Univ São Paulo, Dept Radiol, Disciplina Oncol, Fac Med, BR-01246903 São Paulo, Brazil Univ Vale Paraiba, Inst Pesquisa Desenvolvimento, BR-12244000 Sao Jose Dos Campos, SP, Brazil Univ São Paulo, Inst Biociencias, Centro Estudios Genoma Humano, Dept Biol, BR-055508900 São Paulo, Brazil Univ Fed São Paulo, Lab Mol Gynecol, Dept Gynecol, BR-04039001 São Paulo, Brazil São Paulo State Univ, Sch Pharmacol, Dept Biol Sci, BR-14801902 Araraquara, SP, Brazil Univ São Paulo, Discipl Genet, Fac Odontol, BR-14040900 Ribeirao Preto, SP, Brazil Univ Fed São Paulo, Dept Biofisica, BR-04023062 São Paulo, Brazil Univ Estadual Paulista, Dept Biol, Inst Biociencias Letras Ciências Exatas, BR-15054000 Sao Jose do Rio Preto, SP, Brazil Univ Estadual Paulista, Dept Genet, Inst Biociencias, BR-18618000 Botucatu, SP, Brazil Univ São Paulo, Dept Bioquim Imunol, Fac Med Ribeirao Preto, BR-14049900 Ribeirao Preto, SP, Brazil Univ Estadual Campinas, Lab Genet Mol Cancer, Dept Clin Med, Fac Ciências Med, BR-13083970 Campinas, SP, Brazil Univ Estadual Campinas, Dept Patol Clin, Fac Ciências Med, BR-13083970 Campinas, SP, Brazil Univ São Paulo, Setor Vetores Virals, Lab Cardiol Mol, Inst Coracao, BR-15403000 São Paulo, Brazil Univ Estadual Paulista, Lab Biol Mol, Hemocentro, Fac Med, BR-18618970 Botucatu, SP, Brazil São Paulo State Univ, Sch Pharmacol, Dept Biol Sci, BR-14801902 Araraquara, SP, Brazil Univ Estadual Paulista, Dept Biol, Inst Biociencias Letras Ciências Exatas, BR-15054000 Sao Jose do Rio Preto, SP, Brazil Univ Estadual Paulista, Dept Genet, Inst Biociencias, BR-18618000 Botucatu, SP, Brazil

Published
2004

13. Identification of human chromosome 22 transcribed sequences with ORF expressed sequence tags

Author

de Souza, S. J., primary, Camargo, A. A., additional, Briones, M. R. S., additional, Costa, F. F., additional, Nagai, M. A., additional, Verjovski-Almeida, S., additional, Zago, M. A., additional, Andrade, L. E. C., additional, Carrer, H., additional, El-Dorry, H. F. A., additional, Espreafico, E. M., additional, Habr-Gama, A., additional, Giannella-Neto, D., additional, Goldman, G. H., additional, Gruber, A., additional, Hackel, C., additional, Kimura, E. T., additional, Maciel, R. M. B., additional, Marie, S. K. N., additional, Martins, E. A. L., additional, Nobrega, M. P., additional, Paco-Larson, M. L., additional, Pardini, M. I. M. C., additional, Pereira, G. G., additional, Pesquero, J. B., additional, Rodrigues, V., additional, Rogatto, S. R., additional, da Silva, I. D. C. G., additional, Sogayar, M. C., additional, de Fatima Sonati, M., additional, Tajara, E. H., additional, Valentini, S. R., additional, Acencio, M., additional, Alberto, F. L., additional, Amaral, M. E. J., additional, Aneas, I., additional, Bengtson, M. H., additional, Carraro, D. M., additional, Carvalho, A. F., additional, Carvalho, L. H., additional, Cerutti, J. M., additional, Correa, M. L. C., additional, Costa, M. C. R., additional, Curcio, C., additional, Gushiken, T., additional, Ho, P. L., additional, Kimura, E., additional, Leite, L. C. C., additional, Maia, G., additional, Majumder, P., additional, Marins, M., additional, Matsukuma, A., additional, Melo, A. S. A., additional, Mestriner, C. A., additional, Miracca, E. C., additional, Miranda, D. C., additional, Nascimento, A. L. T. O., additional, Nobrega, F. G., additional, Ojopi, E. P. B., additional, Pandolfi, J. R. C., additional, Pessoa, L. G., additional, Rahal, P., additional, Rainho, C. A., additional, da Ro's, N., additional, de Sa, R. G., additional, Sales, M. M., additional, da Silva, N. P., additional, Silva, T. C., additional, da Silva, W., additional, Simao, D. F., additional, Sousa, J. F., additional, Stecconi, D., additional, Tsukumo, F., additional, Valente, V., additional, Zalcberg, H., additional, Brentani, R. R., additional, Reis, L. F. L., additional, Dias-Neto, E., additional, and Simpson, A. J. G., additional

Published
2000
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16. Detection of Borrelia-burgdorferi in Biological Samples Using the Polymerase Chain-reaction Assay

Author

UCL - MD/MIGE - Département de microbiologie, d'immunologie et de génétique, Debue, M., Gautier, Ph. E., Hackel, C., Vanelsen, A., Herzog, A., Bigaignon, Geoffroy, Bollen, A., UCL - MD/MIGE - Département de microbiologie, d'immunologie et de génétique, Debue, M., Gautier, Ph. E., Hackel, C., Vanelsen, A., Herzog, A., Bigaignon, Geoffroy, and Bollen, A.

Abstract

Oligonucleotide primers were used in the polymerase chain reaction assay to amplify specific DNA regions of the Borrelia burgdorferi 49-kb linear plasmid. One set of primers identifies a 442-bp DNA fragment in the OspA gene and a second pair of amplimers, a 176-bp DNA piece located in the OspB gene. The last set of primers, OspBpc3/pc4, outperformed the other pair in discriminating pathogenic North American or European isolates from related bacterial species, detected down to 4 spirochaetes, and was suitable for the identification of B. burgdorferi in biological samples, such as synovial and cerebrospinal fluids.

Published
1991

22. Identification and complete sequencing of novel human transcripts through the use of mouse orthologs and testis cDNA sequences

Author

Ferreira, E. N., Pires, L. C., Parmigiani, R. B., Bettoni, F., Puga, R. D., Pinheiro, D. G., Andrade, L. E. C., Cruz, L. O., Degaki, T. L., Faria Jr, M., Festa, F., Giannella-Neto, D., Giorgi, R. R., Goldman, G. H., Granja, F., Gruber, A., Hackel, C., Henrique-Silva, F., Malnic, B., Manzini, C. V. B., Marie, S. K. N., Martinez-Rossi, N. M., Oba-Shinjo, S. M., Pardini, M. I. M. C., Rahal, P., Rainho, C. A., Rogatto, S. R., Romano, C. M., Rodrigues, V., Sales, M. M., Savoldi, M., Da Silva, I. D. C. G., Da Silva, N. P., Souza, S. J., Tajara, E. H., Wilson Araujo Silva Jr, Simpson, A. J. G., Sogayar, M. C., Camargo, A. A., and Carraro, D. M.

Subjects
Male, Mice, DNA, Complementary, Transcription, Genetic, Genome, Human, Molecular Sequence Data, Testis, Animals, Chromosome Mapping, Humans, Amino Acid Sequence, Sequence Analysis, DNA, Gene Library
Abstract

The correct identification of all human genes, and their derived transcripts, has not yet been achieved, and it remains one of the major aims of the worldwide genomics community. Computational programs suggest the existence of 30,000 to 40,000 human genes. However, definitive gene identification can only be achieved by experimental approaches. We used two distinct methodologies, one based on the alignment of mouse orthologous sequences to the human genome, and another based on the construction of a high-quality human testis cDNA library, in an attempt to identify new human transcripts within the human genome sequence. We generated 47 complete human transcript sequences, comprising 27 unannotated and 20 annotated sequences. Eight of these transcripts are variants of previously known genes. These transcripts were characterized according to size, number of exons, and chromosomal localization, and a search for protein domains was undertaken based on their putative open reading frames. In silico expression analysis suggests that some of these transcripts are expressed at low levels and in a restricted set of tissues.

24. Diagnosis of 5 alpha-reductase type 2 deficiency: Contribution of anti-Mullerian hormone evaluation

Author

Stuchi-Perez, Eg, Hackel, C., Oliveira, Lec, Ferraz, Lfc, Oliveira, Lc, Nunes-Silva, D., Toralles, Mb, Steinmetz, L., Damiani, D., Maciel-Guerra, At, Gil Guerra-Junior, Universidade Estadual de Campinas (UNICAMP), Universidade Federal da Bahia (UFBA), and Universidade Estadual Paulista (Unesp)

Subjects
endocrine system, 5 alpha-reductase, parasitic diseases, testosterone, androgen insensitivity syndrome, Mullerian inhibiting hormone, dihydrotestosterone, pseudohermaphroditism, hormones, hormone substitutes, and hormone antagonists
Abstract

Made available in DSpace on 2020-12-10T16:33:09Z (GMT). No. of bitstreams: 0 Previous issue date: 2005-01-01 Aim: To evaluate anti-Mullerian hormone (AMH) levels in patients with clinical and molecular diagnosis of 5 alpha-reductase 2 deficiency. Patients and Methods: Data from 14 patients whose age ranged from 21 days to 29 years were analyzed according to age and pubertal stage. Sexual ambiguity was rated as Prader III in 11 patients. LH, FSH, testosterone (T), dihydrotestosterone (DHT) and AMH serum levels were measured in all but two patients, who had been previously submitted to gonadectomy; T and DHT were also measured in 20 age-matched controls. Results: Gonadotropin levels were normal in all but one patient who retained gonads (six of whom had reached puberty) and T/DHT ratio was elevated in all patients when compared to controls. All prepubertal patients had AMH levels < -1 SD for age, while most pubertal patients had AMH levels compatible with pubertal stage. Conclusions: Prepubertal patients with 5 alpha-reductase 2 deficiency have AMH values in the lower part of the normal range. These data indicate that T does not need to be converted to DHT to inhibit AMH secretion by Sertoli cells. Univ Estadual Campinas, Sch Med, GIEDDS, Campinas, SP, Brazil Univ Estadual Campinas, Sch Med, CBMEG, Campinas, SP, Brazil Univ Estadual Campinas, Sch Med, Dept Clin Pathol, Physiol Lab, Campinas, SP, Brazil Univ Fed Bahia, Sch Med, Dept Pediat, Salvador, BA, Brazil State Univ Sao Paulo, Sch Med, Unit Pediat Endocrinol, Sao Paulo, Brazil State Univ Sao Paulo, Sch Med, Unit Pediat Endocrinol, Sao Paulo, Brazil

25. The trehalose coating effect on the internal protein dynamics

Author

Hackel C., Zinkevich T., Belton P., Achilles A., Reichert D., Krushelnitsky A., Hackel C., Zinkevich T., Belton P., Achilles A., Reichert D., and Krushelnitsky A.

Abstract

15N and 13C NMR experiments were applied to conduct a comparative study of a cold shock protein (Csp) in two states - lyophilized powder and a protein embedded in a glassy trehalose matrix. Both samples were studied at various levels of rehydration. The experiments used (measuring relaxation rates R 1 and R 1ρ, motionally averaged dipolar couplings and solid state exchange method detecting reorientation of the chemical shift anisotropy tensor) allow obtaining abundant information on the protein structural features and internal motions in a range of correlation times from nanoseconds to seconds. The main results are: (a) the trehalose coating makes the protein structure more native in comparison with the dehydrated lyophilized powder, however, trehalose still cannot remove all non-native hydrogen bonds which are present in a dehydrated protein; (b) trehalose has an appreciable effect on the internal dynamics: the motion of the backbone N-H groups in the nanosecond and microsecond time scales becomes slower while the motional amplitude remains constant; (c) upon adding water to the Csp-trehalose mixture, water molecules accumulate around proteins forming a layer between the protein surface and the trehalose matrix. The protein dynamics become faster, however, not as fast as in the fully hydrated state; (d) the hydration response of dynamics of the NH and CH(CH 2) groups in a protein is qualitatively different: upon increasing protein hydration, the correlation times of the N-H motions become shorter and the amplitude remains stable, and for CH(CH 2) groups the motional amplitude increases and the correlation times do not change. This can be explained by a different ability of the NH and CH(CH 2) groups to form hydrogen bonds. © the Owner Societies 2012.

26. The trehalose coating effect on the internal protein dynamics

Author

Hackel C., Zinkevich T., Belton P., Achilles A., Reichert D., Krushelnitsky A., Hackel C., Zinkevich T., Belton P., Achilles A., Reichert D., and Krushelnitsky A.

Abstract

15N and 13C NMR experiments were applied to conduct a comparative study of a cold shock protein (Csp) in two states - lyophilized powder and a protein embedded in a glassy trehalose matrix. Both samples were studied at various levels of rehydration. The experiments used (measuring relaxation rates R 1 and R 1ρ, motionally averaged dipolar couplings and solid state exchange method detecting reorientation of the chemical shift anisotropy tensor) allow obtaining abundant information on the protein structural features and internal motions in a range of correlation times from nanoseconds to seconds. The main results are: (a) the trehalose coating makes the protein structure more native in comparison with the dehydrated lyophilized powder, however, trehalose still cannot remove all non-native hydrogen bonds which are present in a dehydrated protein; (b) trehalose has an appreciable effect on the internal dynamics: the motion of the backbone N-H groups in the nanosecond and microsecond time scales becomes slower while the motional amplitude remains constant; (c) upon adding water to the Csp-trehalose mixture, water molecules accumulate around proteins forming a layer between the protein surface and the trehalose matrix. The protein dynamics become faster, however, not as fast as in the fully hydrated state; (d) the hydration response of dynamics of the NH and CH(CH 2) groups in a protein is qualitatively different: upon increasing protein hydration, the correlation times of the N-H motions become shorter and the amplitude remains stable, and for CH(CH 2) groups the motional amplitude increases and the correlation times do not change. This can be explained by a different ability of the NH and CH(CH 2) groups to form hydrogen bonds. © the Owner Societies 2012.

28. Instabilidade cromossômica induzida por agroquímicos em trabalhadores rurais na região de Passo Fundo, Rio Grande do Sul, Brasil

Author

Pacheco Adil de Oliveira and Hackel Christine

Subjects
Saúde Ocupacional, Envenenamento, Exposição a Praguicidas, Aberrações Cromossômicas, Medicine, Public aspects of medicine, RA1-1270
Abstract

A região de Passo Fundo no Planalto Médio do Rio Grande do Sul, caracteriza-se pela produção de grãos (trigo, soja), nas quais grandes quantidades de agroquímicos (fungicidas, inseticidas e herbicidas) são utilizadas. Para avaliar a atividade genotóxica desses produtos em seres humanos, utilizou-se a técnica de micronúcleos, através de amostras de sangue periférico de trinta trabalhadores expostos e de trinta indivíduos controles não expostos. A freqüência de micronúcleos foi avaliada em 1.000 células binucleadas por indivíduo em ambos os grupos. Fatores como tabagismo, idade e tempo de exposição não exerceram qualquer efeito sobre a freqüência de micronúcleos em ambos os grupos. No entanto, a análise estatística revelou números significativamente mais elevados de micronúcleos em expostos (14,3/1.000 células) do que em não expostos (7,1/1.000 células), indicando que o teste do micronúcleo é um ensaio biológico eficiente para monitorar populações expostas a misturas de agroquímicos.

Published
2002

29. New insights into the interaction of proteins and disaccharides-The effect of pH and concentration.

Author

Reichert D, Gröger S, and Hackel C

Subjects
Diffusion, Hydrogen-Ion Concentration, Magnetic Resonance Spectroscopy, Muramidase chemistry, Protein Binding, Sucrose chemistry, Trehalose chemistry, Viscosity, Muramidase metabolism, Sucrose metabolism, Trehalose metabolism
Abstract

To gain new insights into the interaction of proteins and disaccharides, we investigated the hydrodynamic radii, RhProt, of lysozyme molecules in solution and in a ternary protein-sugar-water system by PFG-NMR. Our approach is based on the assumption that the anhydrobiotic properties of disaccharides like trehalose are based on aggregation of sugar molecules to the proteins, i.e., accumulation of sugar molecules close to the protein, and that this process can be investigated by the experimentally detectable RhProt value of the protein. The R h values are calculated from the experimentally determined diffusion coefficients and the application of a viscosity correction using the inert molecule dioxane as an internal viscosity reference. The experiments were performed as a function of sugar concentration, the overall particle concentration and the pH value. We investigated the disaccharides trehalose and sucrose, mainly for the reason that trehalose has well know cryptobiotic properties while sucrose, which is similar in size and structure, lacks these properties. The results show the formation of a protective sugar shell around the proteins over a wider range of concentrations and pH values in the case of trehalose., (© 2016 Wiley Periodicals, Inc.)

Published
2017
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30. The trehalose coating effect on the internal protein dynamics.

Author

Hackel C, Zinkevich T, Belton P, Achilles A, Reichert D, and Krushelnitsky A

Subjects
Hydrogen Bonding, Nuclear Magnetic Resonance, Biomolecular, Proteins chemistry, Trehalose chemistry
Abstract

(15)N and (13)C NMR experiments were applied to conduct a comparative study of a cold shock protein (Csp) in two states-lyophilized powder and a protein embedded in a glassy trehalose matrix. Both samples were studied at various levels of rehydration. The experiments used (measuring relaxation rates R(1) and R(1ρ), motionally averaged dipolar couplings and solid state exchange method detecting reorientation of the chemical shift anisotropy tensor) allow obtaining abundant information on the protein structural features and internal motions in a range of correlation times from nanoseconds to seconds. The main results are: (a) the trehalose coating makes the protein structure more native in comparison with the dehydrated lyophilized powder, however, trehalose still cannot remove all non-native hydrogen bonds which are present in a dehydrated protein; (b) trehalose has an appreciable effect on the internal dynamics: the motion of the backbone N-H groups in the nanosecond and microsecond time scales becomes slower while the motional amplitude remains constant; (c) upon adding water to the Csp-trehalose mixture, water molecules accumulate around proteins forming a layer between the protein surface and the trehalose matrix. The protein dynamics become faster, however, not as fast as in the fully hydrated state; (d) the hydration response of dynamics of the NH and CH(CH(2)) groups in a protein is qualitatively different: upon increasing protein hydration, the correlation times of the N-H motions become shorter and the amplitude remains stable, and for CH(CH(2)) groups the motional amplitude increases and the correlation times do not change. This can be explained by a different ability of the NH and CH(CH(2)) groups to form hydrogen bonds.

Published
2012
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31. Signal loss in 1D magic-angle spinning exchange NMR (CODEX): radio-frequency limitations and intermediate motions.

Author

Hackel C, Franz C, Achilles A, Saalwächter K, and Reichert D

Abstract

The popular 1D MAS exchange experiment CODEX suffers limitations due to signal loss during the finite recoupling periods, during which the magnetization evolves in the transverse plane. Here, we address the origins and possible improvements of this problem, aimed at (i) an optimization of the signal-to-noise ratio in the experiments, as well as harnessing intermediate-motion induced signal loss for obtaining approximate information on (ii) correlation times and (iii) potential distributions, where the latter are often found in polymeric systems. First, we show that the intensity of the signal is sensitive to the radiofrequency (rf) parameters of the carbon recoupling and proton decoupling, and care must be taken to gain optimal signal intensity. Optimum conditions are found for recoupling pulses being as short as possible for large chemical shift anisotropy (CSA) values, and approaching a ratio of 3 between the nutation frequencies for protonated carbons, calling for an individual adjustment in each case. Second, we demonstrate that the effect of intermediate motions can be studied semi-quantitatively by combining CODEX data with its constant-time modification CONTRA, which allows for a tuning of the signal loss due to intermediate motions. Third, for the case of samples featuring a distribution of correlation times, we propose a procedure to obtain an estimate of the proportion of molecular segments in the sample for which the CODEX data are representative, i.e., which share of segments moves truly in the slow-motion regime. The procedure involves the combination of CODEX data with a cross-polarisation (CP) reference experiment for an estimate of the full sample magnetization; it is demonstrated on the example of semi-crystalline poly(ethylene oxide).

Published
2009
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32. Molecular analysis of KAL-1, GnRH-R, NELF and EBF2 genes in a series of Kallmann syndrome and normosmic hypogonadotropic hypogonadism patients.

Author

Trarbach EB, Baptista MT, Garmes HM, and Hackel C

Subjects
Amino Acids genetics, Exons genetics, Gene Deletion, Humans, Male, Point Mutation genetics, Polymorphism, Genetic genetics, Sequence Analysis, DNA methods, Basic Helix-Loop-Helix Transcription Factors genetics, Extracellular Matrix Proteins genetics, Hypogonadism genetics, Kallmann Syndrome genetics, Nerve Tissue Proteins genetics, Receptors, LHRH genetics, Transcription Factors genetics
Abstract

We report the results of molecular analysis in a series of twelve Kallmann syndrome (KS) and five normosmic hypogonadotropic hypogonadism (nHH) Brazilian patients. Kallman syndrome 1 (KAL-1) gene analysis was performed in all patients and the gonadotrophin releasing hormone receptor (GnRH-R) gene was investigated in nHH patients using PCR analysis with exon-flanking primers followed by automated sequencing techniques. Two-point mutations at the KAL-1 locus were found in two KS patients. One case exhibited a novel C deletion (del1956C) in exon 12 leading to a premature stop codon at position 617. The second case, a C to T transition at exon 5, showed a stop codon at aminoacid 191 (Arg191X). Renal agenesis and bimanual synkinesis, which are frequently found in patients with the KAL-1 mutation, were observed in these cases. Among the KS patients, two previously reported cases had intragenic deletions of exons 5-10, while a third patient had a KAL-1 gene microdeletion detected by fluorescence in situ hybridization. For the nHH patients, no abnormalities were observed at the exonic and flanking sequences of the KAL-1 or GnRH-R genes. Nasal embryonic LHRH factor (NELF) and early B-cell factor 2 (EBF2) exons were evaluated in KAL-1/GnRH-R mutation-negative cases (seven KS and five nHH) by sequence analysis but no mutations were identified in the coding regions in these patients. In conclusion, this report includes the description of a novel point mutation of the KAL-1 gene and suggests that the KAL-1 mutations and deletions might be more prevalent in KS Brazilian patients than previously described in other series. NELF and EBF2 genes have been considered good candidates for HH and a large number of patients need to be studied to assess their contribution to reproductive function.

Published
2005
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33. Large-scale transcriptome analyses reveal new genetic marker candidates of head, neck, and thyroid cancer.

Author

Reis EM, Ojopi EP, Alberto FL, Rahal P, Tsukumo F, Mancini UM, Guimarães GS, Thompson GM, Camacho C, Miracca E, Carvalho AL, Machado AA, Paquola AC, Cerutti JM, da Silva AM, Pereira GG, Valentini SR, Nagai MA, Kowalski LP, Verjovski-Almeida S, Tajara EH, Dias-Neto E, Bengtson MH, Canevari RA, Carazzolle MF, Colin C, Costa FF, Costa MC, Estécio MR, Esteves LI, Federico MH, Guimarães PE, Hackel C, Kimura ET, Leoni SG, Maciel RM, Maistro S, Mangone FR, Massirer KB, Matsuo SE, Nobrega FG, Nóbrega MP, Nunes DN, Nunes F, Pandolfi JR, Pardini MI, Pasini FS, Peres T, Rainho CA, dos Reis PP, Rodrigus-Lisoni FC, Rogatto SR, dos Santos A, dos Santos PC, Sogayar MC, and Zanelli CF

Subjects
Alternative Splicing, Expressed Sequence Tags, Head and Neck Neoplasms metabolism, Humans, Larynx metabolism, Mouth metabolism, Pharynx metabolism, Polymerase Chain Reaction, Protein Isoforms, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, DNA, Thyroid Gland metabolism, Thyroid Neoplasms metabolism, Gene Expression Profiling, Genetic Markers, Head and Neck Neoplasms genetics, RNA, Messenger genetics, Thyroid Neoplasms genetics, Transcription, Genetic
Abstract

A detailed genome mapping analysis of 213,636 expressed sequence tags (EST) derived from nontumor and tumor tissues of the oral cavity, larynx, pharynx, and thyroid was done. Transcripts matching known human genes were identified; potential new splice variants were flagged and subjected to manual curation, pointing to 788 putatively new alternative splicing isoforms, the majority (75%) being insertion events. A subset of 34 new splicing isoforms (5% of 788 events) was selected and 23 (68%) were confirmed by reverse transcription-PCR and DNA sequencing. Putative new genes were revealed, including six transcripts mapped to well-studied chromosomes such as 22, as well as transcripts that mapped to 253 intergenic regions. In addition, 2,251 noncoding intronic RNAs, eventually involved in transcriptional regulation, were found. A set of 250 candidate markers for loss of heterozygosis or gene amplification was selected by identifying transcripts that mapped to genomic regions previously known to be frequently amplified or deleted in head, neck, and thyroid tumors. Three of these markers were evaluated by quantitative reverse transcription-PCR in an independent set of individual samples. Along with detailed clinical data about tumor origin, the information reported here is now publicly available on a dedicated Web site as a resource for further biological investigation. This first in silico reconstruction of the head, neck, and thyroid transcriptomes points to a wealth of new candidate markers that can be used for future studies on the molecular basis of these tumors. Similar analysis is warranted for a number of other tumors for which large EST data sets are available.

Published
2005
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34. [5alpha-reductase type 2 deficiency: experiences from Campinas (SP) and Salvador (BA)].

Author

Hackel C, Oliveira LE, Toralles MB, Nunes-Silva D, Tonini MM, Ferraz LF, Steinmetz L, Damiani D, Oliveira LC, Maciel-Guerra AT, Stuchi-Perez EG, and Guerra-Júnior G

Subjects
3-Oxo-5-alpha-Steroid 4-Dehydrogenase genetics, Adolescent, Adult, Brazil, Child, Child, Preschool, Disorders of Sex Development genetics, Humans, Infant, Infant, Newborn, Male, Mutation, 3-Oxo-5-alpha-Steroid 4-Dehydrogenase deficiency, Disorders of Sex Development enzymology
Abstract

Objective: To report the experience regarding patients with steroid 5alpha-reductase type 2 deficiency from three different clinical services in Brazil., Casuistic and Methods: Twenty five patients with clinical and hormonal features of 5alpha-reductase deficiency from 23 families (15 from Bahia, 7 from São Paulo and 1 from Minas Gerais) were included in this study. Clinical, hormonal and molecular data were evaluated. The molecular analysis of the five exons of the SRD5A2 gene was done by automatic or manual sequencing of PCR products., Results: In ten families, SRD5A2 mutations were found in homozygosis (5 with G183S, 2 with R246W, 1 with G196S, 1 with del642T, 1 with 217&#95;218insC), in three in compound heterozygosis (1 with Q126R/IVS3+1G>A, 1 with Q126R/del418T, 1 with Q126R/G158R) while other three were heterozygous, with only one deleterious mutation (1 with G196S, 1 with A207D, and 1 with R246W). In seven cases, no sequencing abnormalities were detected. The G183S substitution was the most frequently found among miscegenated patients (Afro-Euro-Brazilians) from Bahia. Hormonal and clinical findings did not differ between patients with or without mutations, exception made to a higher frequency of consanguinity and greater severity of genital ambiguity in the first group., Conclusion: Our results reinforce the importance of molecular investigation for the diagnosis of this disease and point out to the finding of a very frequent mutation (G183S) in our series, especially in patients with mixed ethnic background from Bahia, and the description of mutations that have only been reported in Brazilian patients so far.

Published
2005
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35. [Genes involved in sex determination and differentiation].

Author

Mello MP, Assumpção Jde G, and Hackel C

Subjects
Animals, Female, Humans, Male, Molecular Biology, Sex Determination Processes, Sex Differentiation genetics
Abstract

Chromosomal sex is established at fertilization by the presence of an X or Y chromosome. The first step of male and female development is gonadal specialization in testes or ovaries; all other processes that follow result from secondary effects produced by testis and ovary hormones. Gonadal determination and differentiation and the development of external genitalia involve time- and tissue-specific expression of genes forming a gene cascade. Those genes, their expression profile and their role in the pathological manifestations related to gonadal and external genitalia development will be discussed in this review.

Published
2005
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36. Identification and complete sequencing of novel human transcripts through the use of mouse orthologs and testis cDNA sequences.

Author

Ferreira EN, Pires LC, Parmigiani RB, Bettoni F, Puga RD, Pinheiro DG, Andrade LE, Cruz LO, Degaki TL, Faria M Jr, Festa F, Giannella-Neto D, Giorgi RR, Goldman GH, Granja F, Gruber A, Hackel C, Henrique-Silva F, Malnic B, Manzini CV, Marie SK, Martinez-Rossi NM, Oba-Shinjo SM, Pardini MI, Rahal P, Rainho CA, Rogatto SR, Romano CM, Rodrigues V, Sales MM, Savoldi M, da Silva ID, da Silva NP, de Souza SJ, Tajara EH, Silva WA Jr, Simpson AJ, Sogayar MC, Camargo AA, and Carraro DM

Subjects
Amino Acid Sequence, Animals, Chromosome Mapping, Gene Library, Humans, Male, Mice, Molecular Sequence Data, DNA, Complementary genetics, Genome, Human, Sequence Analysis, DNA methods, Testis chemistry, Transcription, Genetic genetics
Abstract

The correct identification of all human genes, and their derived transcripts, has not yet been achieved, and it remains one of the major aims of the worldwide genomics community. Computational programs suggest the existence of 30,000 to 40,000 human genes. However, definitive gene identification can only be achieved by experimental approaches. We used two distinct methodologies, one based on the alignment of mouse orthologous sequences to the human genome, and another based on the construction of a high-quality human testis cDNA library, in an attempt to identify new human transcripts within the human genome sequence. We generated 47 complete human transcript sequences, comprising 27 unannotated and 20 annotated sequences. Eight of these transcripts are variants of previously known genes. These transcripts were characterized according to size, number of exons, and chromosomal localization, and a search for protein domains was undertaken based on their putative open reading frames. In silico expression analysis suggests that some of these transcripts are expressed at low levels and in a restricted set of tissues.

Published
2004

37. A transcript finishing initiative for closing gaps in the human transcriptome.

Author

Sogayar MC, Camargo AA, Bettoni F, Carraro DM, Pires LC, Parmigiani RB, Ferreira EN, de Sá Moreira E, do Rosário D de O Latorre M, Simpson AJ, Cruz LO, Degaki TL, Festa F, Massirer KB, Sogayar MC, Filho FC, Camargo LP, Cunha MA, De Souza SJ, Faria M Jr, Giuliatti S, Kopp L, de Oliveira PS, Paiva PB, Pereira AA, Pinheiro DG, Puga RD, S de Souza JE, Albuquerque DM, Andrade LE, Baia GS, Briones MR, Cavaleiro-Luna AM, Cerutti JM, Costa FF, Costanzi-Strauss E, Espreafico EM, Ferrasi AC, Ferro ES, Fortes MA, Furchi JR, Giannella-Neto D, Goldman GH, Goldman MH, Gruber A, Guimarães GS, Hackel C, Henrique-Silva F, Kimura ET, Leoni SG, Macedo C, Malnic B, Manzini B CV, Marie SK, Martinez-Rossi NM, Menossi M, Miracca EC, Nagai MA, Nobrega FG, Nobrega MP, Oba-Shinjo SM, Oliveira MK, Orabona GM, Otsuka AY, Paço-Larson ML, Paixão BM, Pandolfi JR, Pardini MI, Passos Bueno MR, Passos GA, Pesquero JB, Pessoa JG, Rahal P, Rainho CA, Reis CP, Ricca TI, Rodrigues V, Rogatto SR, Romano CM, Romeiro JG, Rossi A, Sá RG, Sales MM, Sant'Anna SC, Santarosa PL, Segato F, Silva WA Jr, Silva ID, Silva NP, Soares-Costa A, Sonati MF, Strauss BE, Tajara EH, Valentini SR, Villanova FE, Ward LS, and Zanette DL

Subjects
Alternative Splicing genetics, Cell Line, Cell Line, Tumor, Computational Biology methods, Computational Biology statistics & numerical data, Consensus Sequence genetics, DNA, Neoplasm, Databases, Genetic classification, Expressed Sequence Tags, Genes genetics, Genome, Human, HeLa Cells pathology, Humans, Molecular Sequence Data, Open Reading Frames genetics, Software Design, Software Validation, U937 Cells pathology, Software, Transcription, Genetic genetics
Abstract

We report the results of a transcript finishing initiative, undertaken for the purpose of identifying and characterizing novel human transcripts, in which RT-PCR was used to bridge gaps between paired EST clusters, mapped against the genomic sequence. Each pair of EST clusters selected for experimental validation was designated a transcript finishing unit (TFU). A total of 489 TFUs were selected for validation, and an overall efficiency of 43.1% was achieved. We generated a total of 59,975 bp of transcribed sequences organized into 432 exons, contributing to the definition of the structure of 211 human transcripts. The structure of several transcripts reported here was confirmed during the course of this project, through the generation of their corresponding full-length cDNA sequences. Nevertheless, for 21% of the validated TFUs, a full-length cDNA sequence is not yet available in public databases, and the structure of 69.2% of these TFUs was not correctly predicted by computer programs. The TF strategy provides a significant contribution to the definition of the complete catalog of human genes and transcripts, because it appears to be particularly useful for identification of low abundance transcripts expressed in a restricted set of tissues as well as for the delineation of gene boundaries and alternatively spliced isoforms., (Copyright 2004 Cold Spring Harbor Laboratory Press ISSN)

Published
2004
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38. The generation and utilization of a cancer-oriented representation of the human transcriptome by using expressed sequence tags.

Author

Brentani H, Caballero OL, Camargo AA, da Silva AM, da Silva WA Jr, Dias Neto E, Grivet M, Gruber A, Guimaraes PE, Hide W, Iseli C, Jongeneel CV, Kelso J, Nagai MA, Ojopi EP, Osorio EC, Reis EM, Riggins GJ, Simpson AJ, de Souza S, Stevenson BJ, Strausberg RL, Tajara EH, Verjovski-Almeida S, Acencio ML, Bengtson MH, Bettoni F, Bodmer WF, Briones MR, Camargo LP, Cavenee W, Cerutti JM, Coelho Andrade LE, Costa dos Santos PC, Ramos Costa MC, da Silva IT, Estécio MR, Sa Ferreira K, Furnari FB, Faria M Jr, Galante PA, Guimaraes GS, Holanda AJ, Kimura ET, Leerkes MR, Lu X, Maciel RM, Martins EA, Massirer KB, Melo AS, Mestriner CA, Miracca EC, Miranda LL, Nobrega FG, Oliveira PS, Paquola AC, Pandolfi JR, Campos Pardini MI, Passetti F, Quackenbush J, Schnabel B, Sogayar MC, Souza JE, Valentini SR, Zaiats AC, Amaral EJ, Arnaldi LA, de Araújo AG, de Bessa SA, Bicknell DC, Ribeiro de Camaro ME, Carraro DM, Carrer H, Carvalho AF, Colin C, Costa F, Curcio C, Guerreiro da Silva ID, Pereira da Silva N, Dellamano M, El-Dorry H, Espreafico EM, Scattone Ferreira AJ, Ayres Ferreira C, Fortes MA, Gama AH, Giannella-Neto D, Giannella ML, Giorgi RR, Goldman GH, Goldman MH, Hackel C, Ho PL, Kimura EM, Kowalski LP, Krieger JE, Leite LC, Lopes A, Luna AM, Mackay A, Mari SK, Marques AA, Martins WK, Montagnini A, Mourão Neto M, Nascimento AL, Neville AM, Nobrega MP, O'Hare MJ, Otsuka AY, Ruas de Melo AI, Paco-Larson ML, Guimarães Pereira G, Pereira da Silva N, Pesquero JB, Pessoa JG, Rahal P, Rainho CA, Rodrigues V, Rogatto SR, Romano CM, Romeiro JG, Rossi BM, Rusticci M, Guerra de Sá R, Sant' Anna SC, Sarmazo ML, Silva TC, Soares FA, Sonati Mde F, de Freitas Sousa J, Queiroz D, Valente V, Vettore AL, Villanova FE, Zago MA, and Zalcberg H

Subjects
Chromosome Mapping, Databases, Genetic, Genetic Variation, Humans, Neoplasms metabolism, Polymorphism, Single Nucleotide, Tissue Distribution, Expressed Sequence Tags, Gene Expression Regulation, Neoplastic, Neoplasms genetics, Proteome, RNA, Messenger metabolism
Abstract

Whereas genome sequencing defines the genetic potential of an organism, transcript sequencing defines the utilization of this potential and links the genome with most areas of biology. To exploit the information within the human genome in the fight against cancer, we have deposited some two million expressed sequence tags (ESTs) from human tumors and their corresponding normal tissues in the public databases. The data currently define approximately 23,500 genes, of which only approximately 1,250 are still represented only by ESTs. Examination of the EST coverage of known cancer-related (CR) genes reveals that <1% do not have corresponding ESTs, indicating that the representation of genes associated with commonly studied tumors is high. The careful recording of the origin of all ESTs we have produced has enabled detailed definition of where the genes they represent are expressed in the human body. More than 100,000 ESTs are available for seven tissues, indicating a surprising variability of gene usage that has led to the discovery of a significant number of genes with restricted expression, and that may thus be therapeutically useful. The ESTs also reveal novel nonsynonymous germline variants (although the one-pass nature of the data necessitates careful validation) and many alternatively spliced transcripts. Although widely exploited by the scientific community, vindicating our totally open source policy, the EST data generated still provide extensive information that remains to be systematically explored, and that may further facilitate progress toward both the understanding and treatment of human cancers.

Published
2003
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39. [Chromosome instability induced by agrochemicals among farm workers in Passo Fundo, Rio Grande do Sul, Brazil].

Author

Pacheco Ade O and Hackel C

Subjects
Adult, Aged, Alcoholic Beverages adverse effects, Brazil, Case-Control Studies, Female, Humans, Lymphocytes drug effects, Male, Micronucleus Tests, Middle Aged, Sex Distribution, Smoking adverse effects, Time Factors, Agriculture, Chromosome Aberrations chemically induced, Occupational Exposure adverse effects, Pesticides adverse effects
Abstract

A major share of the grain farming (wheat and soybeans) in the State of Rio Grande do Sul is in the Passo Fundo area. For crop pest control, large amounts of agrochemicals (fungicides, insecticides, and herbicides) are used. To evaluate the genotoxicity of these products, the micronucleus test was performed in farm workers directly exposed to these chemicals. Heparinized blood samples were drawn by venipuncture from 30 exposed workers and 30 non-exposed controls. Micronuclei frequency was evaluated by counting 1,000 binucleated cells per individual in both groups. Smoking habits, age, and duration of exposure showed no effect on the frequency of micronuclei in both groups. However, statistical analysis showed significantly higher mean numbers of binucleated cells with micronuclei in exposed individuals (14.3/1,000 cells) as compared to controls (7.1/1,000 cells), allowing the authors to conclude that the micronucleus test is an efficient biological assay for monitoring population exposure to mixtures of agrochemicals.

Published
2002
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40. Polymorphisms in the DNA repair gene XRCC1 and susceptibility to alcoholic liver cirrhosis in older Southeastern Brazilians.

Author

Rossit AR, Cabral IR, Hackel C, da Silva R, Froes ND, and Abdel-Rahman SZ

Subjects
Adult, Age Factors, Alleles, Brazil, Cytochrome P-450 CYP1A1 genetics, Genotype, Humans, Male, Middle Aged, X-ray Repair Cross Complementing Protein 1, DNA Repair genetics, DNA-Binding Proteins genetics, Genetic Predisposition to Disease, Liver Cirrhosis, Alcoholic genetics, Polymorphism, Genetic
Abstract

The population of Southeastern Brazil has a very high mortality rate from liver cirrhosis, a disease that is considered an irreversible pre-malignant condition. This is largely due to the high prevalence of alcohol abuse in the region. Chronic alcohol consumption is associated with the production of free radical intermediates that can cause several DNA lesions. Reduced repair of these DNA lesions would, therefore, constitute a significant risk factor for liver cirrhosis and subsequent cancer. Recently, a number of polymorphisms in several DNA repair genes have been discovered, and it is possible that these polymorphisms may affect DNA repair capacity and thus modulate susceptibility to the disease. In this study, we tested the hypothesis that polymorphisms in the DNA repair gene XRCC1 are associated with increased risk of liver cirrhosis in Southeastern Brazilians. We conducted a pilot case-control study of 97 liver cirrhosis cases and 96 controls (matched for age, sex, and ethnicity) to investigate the role of two allelic variants coding for amino acid changes in the XRCC1 gene (the Arg194Trp and the Arg399Gln polymorphisms). Overall, we observed a 1.8-fold increase in the relative risk of liver cirrhosis associated with the 399Gln allele (either the heterozygous Arg/Gln or the homozygous Gln/Gln genotypes). The adjusted odds ratio (OR) was 1.82 (95% confidence limit (CL) 1.10-3.30). The relative risk appears to be highest among the Mestiso ethnic group (OR 2.60, 95% CL 0.92-7.34). There was a significant association between the 399Gln polymorphism and the risk of liver cirrhosis in older individuals over the age of 45 years (OR 2.70 (95% CL 1.14-6.48) compared to an OR of 1.24 (95% CL 0.55-2.78) for those under 45 years of age. No association was observed between the XRCC1 194Trp polymorphism and risk of liver cirrhosis. These preliminary results suggest that the XRCC1 399Gln polymorphism may be a significant risk modifier for alcoholic liver cirrhosis and justifies additional studies in that direction.

Published
2002
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41. The contribution of 700,000 ORF sequence tags to the definition of the human transcriptome.

Author

Camargo AA, Samaia HP, Dias-Neto E, Simão DF, Migotto IA, Briones MR, Costa FF, Nagai MA, Verjovski-Almeida S, Zago MA, Andrade LE, Carrer H, El-Dorry HF, Espreafico EM, Habr-Gama A, Giannella-Neto D, Goldman GH, Gruber A, Hackel C, Kimura ET, Maciel RM, Marie SK, Martins EA, Nobrega MP, Paco-Larson ML, Pardini MI, Pereira GG, Pesquero JB, Rodrigues V, Rogatto SR, da Silva ID, Sogayar MC, Sonati MF, Tajara EH, Valentini SR, Alberto FL, Amaral ME, Aneas I, Arnaldi LA, de Assis AM, Bengtson MH, Bergamo NA, Bombonato V, de Camargo ME, Canevari RA, Carraro DM, Cerutti JM, Correa ML, Correa RF, Costa MC, Curcio C, Hokama PO, Ferreira AJ, Furuzawa GK, Gushiken T, Ho PL, Kimura E, Krieger JE, Leite LC, Majumder P, Marins M, Marques ER, Melo AS, Melo MB, Mestriner CA, Miracca EC, Miranda DC, Nascimento AL, Nobrega FG, Ojopi EP, Pandolfi JR, Pessoa LG, Prevedel AC, Rahal P, Rainho CA, Reis EM, Ribeiro ML, da Ros N, de Sa RG, Sales MM, Sant'anna SC, dos Santos ML, da Silva AM, da Silva NP, Silva WA Jr, da Silveira RA, Sousa JF, Stecconi D, Tsukumo F, Valente V, Soares F, Moreira ES, Nunes DN, Correa RG, Zalcberg H, Carvalho AF, Reis LF, Brentani RR, Simpson AJ, and de Souza SJ

Subjects
Humans, Expressed Sequence Tags, Genome, Human, Open Reading Frames, Transcription, Genetic
Abstract

Open reading frame expressed sequences tags (ORESTES) differ from conventional ESTs by providing sequence data from the central protein coding portion of transcripts. We generated a total of 696,745 ORESTES sequences from 24 human tissues and used a subset of the data that correspond to a set of 15,095 full-length mRNAs as a means of assessing the efficiency of the strategy and its potential contribution to the definition of the human transcriptome. We estimate that ORESTES sampled over 80% of all highly and moderately expressed, and between 40% and 50% of rarely expressed, human genes. In our most thoroughly sequenced tissue, the breast, the 130,000 ORESTES generated are derived from transcripts from an estimated 70% of all genes expressed in that tissue, with an equally efficient representation of both highly and poorly expressed genes. In this respect, we find that the capacity of the ORESTES strategy both for gene discovery and shotgun transcript sequence generation significantly exceeds that of conventional ESTs. The distribution of ORESTES is such that many human transcripts are now represented by a scaffold of partial sequences distributed along the length of each gene product. The experimental joining of the scaffold components, by reverse transcription-PCR, represents a direct route to transcript finishing that may represent a useful alternative to full-length cDNA cloning.

Published
2001
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42. Evaluation of the tubular and interstitial functions of the testis in 46,XY patients with ambiguous genitalia.

Author

Stuchi-Perez EG, Lukas-Croisier C, De Castro M, Baptista MT, Ribeiro Scolfaro M, Marques-De-Faria AP, Hackel C, Maciel-Guerra AT, and Guerra Júnior G

Subjects
3-Hydroxysteroid Dehydrogenases deficiency, 3-Oxo-5-alpha-Steroid 4-Dehydrogenase deficiency, Adolescent, Androgen-Insensitivity Syndrome physiopathology, Anti-Mullerian Hormone, Child, Child, Preschool, Chorionic Gonadotropin pharmacology, Follicle Stimulating Hormone blood, Gonadal Dysgenesis physiopathology, Growth Inhibitors blood, Humans, Infant, Karyotyping, Leydig Cells physiology, Luteinizing Hormone blood, Male, Sertoli Cells physiology, Testicular Hormones blood, Testosterone blood, Disorders of Sex Development physiopathology, Glycoproteins, Testis physiopathology
Abstract

Investigation of the origin of sexual ambiguity is complex. Although testicular function has traditionally been assessed only by examining the steroidogenic capacity of Leydig cells and spermatogenesis, it has recently been shown that the measurement of serum anti-Müllerian hormone (AMH) as a marker of Sertoli cell function may also help clinicians. The aim of this study was to evaluate both Leydig and Sertoli cell functions in 46,XY patients with intersex states in order to establish biochemical patterns that would help to reach an etiologic diagnosis. We measured serum androgens, AMH and gonadotropins in 24 patients with sexual ambiguity and XY karyotype: 8 with gonadal dysgenesis (GD), 3 with 3beta-hydroxysteroid dehydrogenase deficiency (3betaHSD), 5 with androgen insensitivity syndrome (AIS), 4 with 5alpha-reductase 2 (SRD5A2) deficiency, and 4 were of unknown origin or idiopathic. Our results showed that while testosterone was low and gonadotropins elevated in patients with either GD or 3betaHSD, AMH was low in the former and high in the latter. Serum AMH and gonadotropins were normal or high in patients with 3betaHSD or AIS, but these could be distinguished by testosterone levels. Serum testosterone and gonadotropins were normal or high in AIS and SRD5A2 deficiency patients; however, while AMH was elevated in AIS, it was not the case in SRD5A2 deficiency patients, indicating that testosterone is sufficient to inhibit AMH within the testis. In idiopathic cases gonadotropins and testosterone were normal, and AMH was normal or low. We conclude that the combined measurement of androgens, AMH and gonadotropins helps to establish the diagnosis in intersex patients.

Published
2000
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43. Molecular mapping of an idic(Yp) chromosome in an Ullrich-Turner patient.

Author

Godoy Assumpção J, Hackel C, Marques-De-Faria AP, and Palandi de Mello M

Subjects
Adult, Blotting, Southern, Chromosome Banding, Female, Genetic Markers, Humans, In Situ Hybridization, Fluorescence, Karyotyping, Male, Models, Genetic, Polymerase Chain Reaction, Sequence Tagged Sites, Isochromosomes, Turner Syndrome genetics, Y Chromosome
Abstract

We describe a woman with Ullrich-Turner manifestations and a 45,X/46, X,+mar karyotype. Fluorescence in situ hybridization (FISH) and DNA analysis were carried out in order to determine the origin and structure of the marker. FISH showed that the marker was a Y-derived dicentric chromosome. The breakpoint at Yq11 (interval 6) was mapped using Southern blotting and polymerase chain reaction (PCR). There were no nucleotide alterations in the SRY conserved domain. Histological analysis of the gonads showed an ovarian-like stroma with no signs of testicular tissue. These findings indicate that the patient was a mosaic 45,X/46,X,idic(Yp) whose phenotypic expression, including sex determination, appeared to have had more influence from the 45,X cell line., (Copyright 2000 Wiley-Liss, Inc.)

Published
2000
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44. New frameshift mutation in the 5alpha-reductase type 2 gene in a Brazilian patient with 5alpha-reductase deficiency.

Author

Ferraz LF, Mathias Baptista MT, Maciel-Guerra AT, Júnior GG, and Hackel C

Subjects
3-Oxo-5-alpha-Steroid 4-Dehydrogenase deficiency, Amino Acid Sequence, Amino Acid Substitution, Base Sequence, Brazil, Codon genetics, Disorders of Sex Development diagnosis, Disorders of Sex Development enzymology, Disorders of Sex Development psychology, Exons genetics, Gender Identity, Genes, Recessive, Heterozygote, Humans, Hypospadias etiology, Hypospadias surgery, Infant, Newborn, Isoenzymes deficiency, Male, Molecular Sequence Data, Phenotype, Point Mutation, Puberty, Sequence Deletion, Sexual Behavior, Terminator Regions, Genetic, 3-Oxo-5-alpha-Steroid 4-Dehydrogenase genetics, Disorders of Sex Development genetics, Frameshift Mutation, Isoenzymes genetics
Abstract

Male pseudohermaphroditism caused by steroid 5alpha-reductase deficiency is an autosomal recessive disorder. The enzyme steroid 5alpha-reductase 2 (encoded by the SRD5A2 gene) catalyses the conversion of testosterone to dihydrotestosterone, which is required for normal differentiation of the external male genitalia. This report describes the molecular analysis of the 5alpha-reductase type 2 gene in a Brazilian patient who was raised as a female, underwent a reversal of gender role behavior, and is now a married man. This patient is a compound heterozygote bearing an A-->G mutation within exon 2, changing codon 126 from Glu to Arg on one allele and a novel single base deletion (418delT) causing a frameshift mutation at codon 140 in the same exon, on the other allele. This last mutation probably leads to the synthesis of a truncated protein, because a premature termination signal is created at codon 159., (Copyright 1999 Wiley-Liss, Inc.)

Published
1999
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45. Determination of the allele frequencies of three polymorphisms in the promoter region of the human protein C gene in three Brazilian ethnic groups.

Author

Mendes CP, Hackel C, Arruda VR, and Annichino-Bizzacchi JM

Subjects
Adolescent, Adult, Aged, Alleles, Brazil, Female, Gene Frequency, Haplotypes, Heterozygote, Humans, Male, Middle Aged, Promoter Regions, Genetic genetics, Black People genetics, Indians, South American genetics, Polymorphism, Genetic genetics, Protein C genetics, White People genetics
Abstract

The frequencies of three polymorphisms in the promoter region of the human protein C gene have been determined in three ethnic groups of the Brazilian population. The allele frequencies observed in south-eastern Brazilian Caucasians and Blacks were similar to the values obtained for the Dutch population and were different from those observed in Amazonian Indians living in the north of the country. The most frequent genotypic combination found in this latter group was the CC/GG/AA genotype, which is very rare among Caucasians. The complete heterozygous genotype CT/AG/AT was the most frequent both in Brazilian Caucasians and Blacks. Among 27 possible genotypic combinations, 21 were found in the Caucasian group and 15 in Blacks, revealing a high degree of genetic diversity in south-eastern Brazilian populations.

Published
1999
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46. Two cases of Y; autosome translocations: A 45,X male and a clinically trisomy 18 patient.

Author

Farah SB, Ramos CF, de Mello MP, Sartorato EL, Horelli-Kuitunen N, Lopes VL, Cavalcanti DP, and Hackel C

Subjects
Base Sequence, Cells, Cultured, Child, Chromosome Banding, DNA Primers, Humans, In Situ Hybridization, Infant, Infant, Newborn, Karyotyping, Male, Molecular Sequence Data, Chromosomes, Human, Pair 15, Chromosomes, Human, Pair 18, Translocation, Genetic, Trisomy, Y Chromosome
Abstract

We report on 2 cases of Y; autosome translocations. One is a male with normal external genitalia and 45,X karyotype without evidence of mosaicism or apparent translocation on cytogenetic analysis. In situ hybridization showed that the euchromatic portion of the Y-chromosome is translocated to the chromosome 15. The other case is a clinically trisomy 18 male patient, with modal number of 46, a small metacentric marker with appearance of an i(18p) and cytogenetic and molecular evidence of Y;18 translocation. The occurrence of Y;18 translocation associated with clinical signs of trisomy 18 is reported here for the first time.

Published
1994
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47. Chromosomal aberrations in cultures of skin fibroblasts of leprosy patients.

Author

Hackel C and Beiguelman B

Subjects
Adolescent, Adult, Aged, Aneuploidy, Biopsy, Chromatids ultrastructure, Dapsone therapeutic use, Diploidy, Female, Fibroblasts ultrastructure, Humans, Leprosy drug therapy, Leprosy pathology, Male, Metaphase, Middle Aged, Skin pathology, Chromosome Aberrations, Leprosy genetics, Skin ultrastructure
Abstract

A search for structural and numerical chromosomal aberrations was made on metaphases obtained by culturing in vitro skin fibroblasts of 16 leprosy patients (10 lepromatous, 2 borderline, and 4 tuberculoid cases) and 2 healthy individuals used as controls. The data were analyzed taking into account sex, age, race, form of leprosy, bacterial index, type of therapy, and age of the fibroblast cultures. Structural chromosomal aberrations are the only type of chromosomal abnormality that may be accepted as significantly increased in the skin fibroblasts of leprosy patients who are under treatment with dapsone alone or with combined therapy.

Published
1985

48. Duchenne muscular dystrophy in a girl with an (X;15) translocation.

Author

Ribeiro MC, Melaragno MI, Schmidt B, Brunoni D, Gabbai AA, and Hackel C

Subjects
Child, Chromosome Banding, Female, Humans, Chromosomes, Human, Pair 15, Muscular Dystrophies genetics, Translocation, Genetic, X Chromosome
Abstract

This is a report of a girl with Duchenne muscular dystrophy (DMD) associated with an 46,X,t (X;15) (p21; q 26) chromosome constitution. Although in the eight published cases of girls with DMD and a t(X;aut) different autosomes were involved in the translocation, the breakpoint was always at Xp21. The present case supports the hypothesis that the DMD gene must be located at Xp21. In this study, involvement of the father's chromosomes in the translocation was detected.

Published
1986
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49. A case of de novo i(12p) with 12q whole-arm translocation mosaicism.

Author

Marques-de-Faria AP and Hackel C

Subjects
Child, Preschool, Chromosome Banding, Chromosomes, Human, Pair 11, Chromosomes, Human, Pair 7, Electrophoresis, Polyacrylamide Gel, Female, Humans, Infant, Isoenzymes, Karyotyping, L-Lactate Dehydrogenase analysis, Chromosome Aberrations, Chromosomes, Human, Pair 12, Mosaicism, Translocation, Genetic
Abstract

We report a dup(12p) due to a de novo i(12p) in a girl with mosaicism for 12q whole-arm translocations onto 7p, 7q, and 11q terminal regions. The dup(12p) syndrome was confirmed by clinical, cytogenetic, and LDH-dosage studies.

Published
1989
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