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3. GDNA qPCR is statistically more reliable than mRNA analysis in detecting leukemic cells to monitor CML

Author

Rainero, A, Angaroni, F, Conti, A, Pirrone, C, Micheloni, G, Tarara, L, Millefanti, G, Maserati, E, Valli, R, Spinelli, O, Buklijas, K, Michelato, A, Casalone, R, Barlassina, C, Barcella, M, Sirchia, S, Piscitelli, E, Caccia, M, Porta, G, Rainero A., Angaroni F., Conti A., Pirrone C., Micheloni G., Tarara L., Millefanti G., Maserati E., Valli R., Spinelli O., Buklijas K., Michelato A., Casalone R., Barlassina C., Barcella M., Sirchia S., Piscitelli E., Caccia M., Porta G., Rainero, A, Angaroni, F, Conti, A, Pirrone, C, Micheloni, G, Tarara, L, Millefanti, G, Maserati, E, Valli, R, Spinelli, O, Buklijas, K, Michelato, A, Casalone, R, Barlassina, C, Barcella, M, Sirchia, S, Piscitelli, E, Caccia, M, Porta, G, Rainero A., Angaroni F., Conti A., Pirrone C., Micheloni G., Tarara L., Millefanti G., Maserati E., Valli R., Spinelli O., Buklijas K., Michelato A., Casalone R., Barlassina C., Barcella M., Sirchia S., Piscitelli E., Caccia M., and Porta G.

Abstract

Chronic Myeloid Leukemia (CML) is a stem cell cancer that arises when t(9;22) translocation occurs in a hematopoietic stem cells. This event results in the expression of the BCR-ABL1 fusion gene, which codes for a constitutively active tyrosine kinase that is responsible for the transformation of a HSC into a CML stem cell, which then gives rise to a clonal myeloproliferative disease. The introduction of Tyrosine Kinase Inhibitors (TKIs) has revolutionized the management of the disease. However, these drugs do not seem to be able to eradicate the malignancy. Indeed, discontinuation trials (STIM; TWISER; DADI) for those patients who achieved a profound molecular response showed 50% relapsing within 12 months. We performed a comparative analysis on 15 CML patients and one B-ALL patient, between the standard quantitative reverse-transcriptase PCR (qRT-PCR) and our genomic DNA patient-specific quantitative PCR assay (gDNA qPCR). Here we demonstrate that gDNA qPCR is better than standard qRT-PCR in disease monitoring after an average follow-up period of 200 days. Specifically, we statistically demonstrated that DNA negativity is more reliable than RNA negativity in indicating when TKIs therapy can be safely stopped.

Published
2018

7. Characterization of multi-locus imprinting disturbances and underlying genetic defects in patients with chromosome 11p15.5 related imprinting disorders

Author

Fontana, L., primary, Bedeschi, M. F., additional, Maitz, S., additional, Cereda, A., additional, Faré, C., additional, Motta, S., additional, Seresini, A., additional, D’Ursi, P., additional, Orro, A., additional, Pecile, V., additional, Calvello, M., additional, Selicorni, A., additional, Lalatta, F., additional, Milani, D., additional, Sirchia, S. M., additional, Miozzo, M., additional, and Tabano, S., additional

Published
2018
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11. OTX1 expression in breast cancer is regulated by p53. Oncogene

Author

Terrinoni, A., Pagani, I. S., Zucchi, I., Chiaravalli, A. M., Serra, V., Rovera, F., Sirchia, S., Dionigi, Gianlorenzo, Miozzo, M., Frattini, A., Ferrari, A., Capella, C., Pasquali, F., Curto, F., Albertini, A., Melino, G., and Porta, G.

Published
2011

13. ESX1 mRNA expression in seminal fluid is an indicator of residual spermatogenesis in non-obstructive azoospermic men

Author

Pansa, A., primary, Sirchia, S. M., additional, Melis, S., additional, Giacchetta, D., additional, Castiglioni, M., additional, Colapietro, P., additional, Fiori, S., additional, Falcone, R., additional, Paganini, L., additional, Bonaparte, E., additional, Colpi, G., additional, Miozzo, M., additional, and Tabano, S., additional

Published
2014
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14. X chromosome inactivation pattern in BRCA gene mutation carriers

Author

Manoukian, S, Verderio, P, Tabano, S, Colapietro, P, Pizzamiglio, S, Grati, F, Calvello, M, Peissel, B, Burn, J, Pensotti, V, Allemani, C, Sirchia, S, Radice, P, Miozzo, M, Miozzo, M., VERDERIO, PAOLO, Manoukian, S, Verderio, P, Tabano, S, Colapietro, P, Pizzamiglio, S, Grati, F, Calvello, M, Peissel, B, Burn, J, Pensotti, V, Allemani, C, Sirchia, S, Radice, P, Miozzo, M, Miozzo, M., and VERDERIO, PAOLO

Abstract

An association of preferential X chromosome inactivation (XCI) with BRCA gene status and breast/ovarian cancer risk has been reported. We evaluated XCI in a large group of BRCA mutation carriers compared to non-carriers and investigated associations between preferential XCI (≥90:10) and age, mutated gene, cancer development and chemotherapy. XCI was analysed by human androgen receptor (HUMARA) assay and pyrosequencing in 437 BRCA1 or BRCA2 mutation carriers and 445 age-matched controls. The distribution of XCI patterns in the two groups was compared by logistic regression analysis. The association between preferential XCI and selected variables was investigated in both univariate and multivariate fashion. In univariate analyses preferential XCI was not significantly associated with the probability of being a BRCA mutation carrier, nor with cancer status, whereas chemotherapeutic regime and age both showed a significant association. In multivariate analysis only age maintained significance (odds ratio, 1.056; 95% confidence interval, 1.016-1.096). Our findings do not support the usefulness of XCI analysis for the identification of BRCA mutation carriers and cancer risk assessment. The increasing preferential XCI frequency with ageing and the association with chemotherapy justify extending the investigation to other categories of female cancer patients to identify possible X-linked loci implicated in cell survival. © 2012 Elsevier Ltd. All rights reserved.

Published
2013

17. Posters * Reproductive Genetics (PGD/PGS)

Author

Crippa, A., primary, Magli, M. C., additional, Robles, F., additional, Capoti, A., additional, Ferraretti, A. P., additional, Gianaroli, L., additional, Gallina, A., additional, Bonaparte, E., additional, Moretti, M., additional, Colpi, G. M., additional, Nerva, F., additional, Contalbi, G., additional, Vacalluzzo, L., additional, Tabano, S., additional, Grati, F. R., additional, Gazzano, G., additional, Sirchia, S. M., additional, Simoni, G., additional, Miozzo, M., additional, Handyside, A., additional, Gabriel, A., additional, Thornhill, A. R., additional, Clemente, E., additional, Reitter, C., additional, Affara, N., additional, Griffin, D. K., additional, Macek, M., additional, Feldmar, P., additional, Kluckova, H., additional, Hrehorcak, M., additional, Diblik, J., additional, Paulasova, P., additional, Turnovec, M., additional, Vilimova, S., additional, Fontes, L., additional, Haddad, L., additional, Borges, E., additional, Iaconelli, A., additional, Braga, D. P. A. F., additional, Vianna-Morgante, A. M., additional, Komsky, A., additional, Kasterstein, E., additional, Komarovsky, D., additional, Bern, O., additional, Maslansky, B., additional, Kaplan, T., additional, Raziel, A., additional, Friedler, S., additional, Gidoni, Y., additional, Ben-Ami, I., additional, Ron-El, R., additional, Strassburger, D., additional, Maggiulli, R., additional, Monahan, D., additional, Neri, Q. V., additional, Hu, J. C. Y., additional, Rosenwaks, Z., additional, Palermo, G. D., additional, Beyazyurek, C., additional, Ekmekci, G. C., additional, Tac, H. A., additional, Ajredin, N., additional, Verlinsky, O., additional, Fiorentino, F., additional, Kahraman, S., additional, Camp, M., additional, Hesters, L., additional, Le Lorc'h, M., additional, Frydman, R., additional, Romana, S., additional, Frydman, N., additional, Perez Sanz, J., additional, Matorras, R., additional, Arluzea, J., additional, Romin, Y., additional, Bilbao, J., additional, Gonzalez-Santiago, N., additional, Manova-Todorova, K., additional, Koff, A., additional, Rivera-Pomar, J. M., additional, de la Hoz-Torres, C., additional, Xanthopoulou, L., additional, Ghevaria, H., additional, Mantzouratou, A., additional, Serhal, P., additional, Doshi, A., additional, Delhanty, J. D., additional, Ye, Y., additional, Qian, Y., additional, Jin, F., additional, Munne, S., additional, Gutierrez, C., additional, Wagner, C., additional, Hill, D., additional, Wiemer, K., additional, Fischer, J., additional, Kaplan, B., additional, Danzer, H., additional, Surrey, M., additional, Opsahl, M., additional, Hladikova, B., additional, Sobek, A., additional, Tkadlec, E., additional, Kyselova, K., additional, Nichi, M., additional, Figueira, R. C. S., additional, Setti, A. S., additional, Colturato, S. S., additional, Rubio, C., additional, Domingo, J., additional, Rodrigo, L., additional, Mercader, A., additional, De los Santos, M. J., additional, Pehlivan, T., additional, Bosch, E., additional, Fernandez, M., additional, Simon, C., additional, Remohi, J., additional, Pellicer, A., additional, Perez-Nevot, B., additional, Lendinez, A. M., additional, Palomares, A. R., additional, Polo, M., additional, Rodriguez, A., additional, Reche, A., additional, Ruiz-Galdon, M., additional, Reyes-Engel, A., additional, Knauff, E. A. H., additional, Blauw, H. M., additional, Kok, K., additional, Wijmenga, C., additional, Fauser, B. C. J. M., additional, Franke, L., additional, Paffoni, A., additional, Paracchini, V., additional, Ferrari, S., additional, Restelli, L., additional, Coviello, D. A., additional, Scarduelli, C., additional, Seia, M., additional, Ragni, G., additional, Aoyama, N., additional, Takehara, Y., additional, Kawachiya, S., additional, Kuroda, T., additional, Kawasaki, N., additional, Yamadera, R., additional, Suzuki, T., additional, Kato, K., additional, Kato, O., additional, Xu, Q. H., additional, Zhang, Z. G., additional, Zhou, P., additional, Wei, Z. L., additional, Huang, D. K., additional, Xing, Q., additional, Cao, Y. X., additional, Fauque, P., additional, Ripoche, M. A., additional, Tost, J., additional, Journot, L., additional, Jouannet, P., additional, Vaiman, D., additional, Dandolo, L., additional, Jammes, H., additional, Hellani, A., additional, Elsheikh, A., additional, Abuamero, K. K., additional, Elakoum, S., additional, Martinez, F., additional, Perez de la Blanca, E., additional, Koutna, O., additional, Cepelak, T., additional, and Sobek, A. J. R., additional

Published
2010
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19. Losses of heterozygosity in oral and oropharyngeal epithelial carcinomas

Author

Grati, F, Sirchia, S, Garagiola, I, Sironi, E, Galioto, S, Rossella, F, Serafini, P, Dulcetti, F, Bozzetti, A, Brusati, R, Simoni, G, Grati, FR, Sirchia, SM, Grati, F, Sirchia, S, Garagiola, I, Sironi, E, Galioto, S, Rossella, F, Serafini, P, Dulcetti, F, Bozzetti, A, Brusati, R, Simoni, G, Grati, FR, and Sirchia, SM

Abstract

We analyzed 25 oral and oropharyngeal epithelial carcinomas for loss of heterozygosity (LOH) and microsatellite instability by using 55 oligonucleotide repeat markers located in 45 chromosomal regions. The aim was to identify which chromosomal regions and tumor-suppressor genes (TSGs) are preferentially lost in these tumors and to relate LOH at specific loci to clinicopathologic data. The analysis was performed on tumor tissue and on a corresponding normal tissue (blood lymphocytes) with the use of the polymerase chain reaction technique followed by microsatellite allele separation with denaturing gel electrophoresis. Thirty-two of 45 chromosomal regions demonstrated a significant (>/=20%) incidence of LOH. An allelic loss of >/=50% was found in 9p21 (77.8%), 8p22-23 (70%), 3p12 (61.5%), 1p36.1 and 12q22 (60%), 3q28 (57.1%), 5q23.3 (54.5%), 3p25-26, 3p24, and 7q35 (50%). We did not find any microsatellite instability. Our results suggest that in addition to a group of TSGs, pleiotropic for several tumor types, other suppressor genes are specifically involved in oral and oropharyngeal carcinogenesis

Published
2000

32. Highly sensitive chemiluminescent method for the detection of cell contamination<FN ID="fn1">This paper has not been peer reviewed.</FN>

Author

Sirchia, S. M., Garagiola, I., Andreis, C. De, Pedranzini, L., Poli, F., Grati, F. R., Diomelli, B., and Simoni, G.

Abstract

Minisatellite analysis is commonly used in forensic disputes but can also be applied to the investigation of cell contamination. Such a problem arises, for example, when transplantation is performed. The presence of contamination has been investigated by other authors using radioactive methods. In the present study we describe a method that allows the detection of contamination with high sensitivity without using radioactive substances. Our technique is based on the use of polymerase chain reaction (PCR) amplification of minisatellite sequences (VNTR), followed by chemiluminescent detection. In particular, biotin-labelled dCTP is included in the PCR mixture and detection of PCR products is obtained following the CSPD chemiluminescent protocol (Southern-Light Nucleic Acid Detection Systems). We applied this method to artificial mixes of DNA of two individuals with alleles of different sizes. We performed progressive dilutions of an individual DNA into the other’s DNA and revealed a contamination of 1 in 2500 cells. We also tested our technique searching for maternal contamination in cord blood samples in 60 cases and revealed a 18.3% contamination. The technique that we set up proves to be a very sensitive one which could be applied not only to the detection of maternal cells in cord blood but also in studying any other kind of contamination. © 1998 John Wiley & Sons, Ltd.

Published
1998
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34. OTX1 expression in breast cancer is regulated by p53.

Author

Terrinoni, A, Pagani, I S, Zucchi, I, Chiaravalli, A M, Serra, V, Rovera, F, Sirchia, S, Dionigi, G, Miozzo, M, Frattini, A, Ferrari, A, Capella, C, Pasquali, F, Lo Curto, F, Albertini, A, Melino, G, and Porta, G

Subjects
GENE expression, P53 antioncogene, HOMEOBOX proteins, BREAST cancer patients, BREAST cancer treatment
Published
2014
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35. Assessment of pregnancy dietary intake and association with maternal and neonatal outcomes

Author

Enrico Ferrazzi, Paola Roggero, Valentina De Cosmi, Tamara Stampalija, Tatjana Radaelli, Daniela Alberico, Fabio Parazzini, Silvia Motta, Jole Costanza, Chiara Tabasso, Giulia Privitera, Patrizia Colapietro, Fabio Mosca, Laura Fontana, Margherita Camanni, Silvano Bosari, Maria Maddalena Ferrari, Monica Miozzo, Silvia Tabano, Carlo Agostoni, Silvia M. Sirchia, Costanza, J., Camanni, M., Ferrari, M. M., De Cosmi, V., Tabano, S., Fontana, L., Radaelli, T., Privitera, G., Alberico, D., Colapietro, P., Motta, S., Sirchia, S., Stampalija, T., Tabasso, C., Roggero, P., Parazzini, F., Mosca, F., Ferrazzi, E., Bosari, S., Miozzo, M., and Agostoni, C.

Subjects
medicine.medical_specialty, Birth weight, Placenta, Population, Weight Gain, Body Mass Index, Eating, Pregnancy, medicine, Birth Weight, Humans, Prospective Studies, education, education.field_of_study, Obstetrics, business.industry, Infant, Newborn, Pregnancy Outcome, Gestational age, medicine.disease, Gestational Weight Gain, European Prospective Investigation into Cancer and Nutrition, n/a, Pediatrics, Perinatology and Child Health, Gestation, Female, medicine.symptom, business, Body mass index, Weight gain
Abstract

Background Maternal dietary habits are contributors of maternal and fetal health; however, available data are heterogeneous and not conclusive. Methods Nutrient intake during pregnancy was assessed in 503 women with uncomplicated pregnancies, using the validated Food Frequency Questionnaire developed by the European Prospective Investigation into Cancer and Nutrition (EPIC-FFQ). Results In all, 68% of women had a normal body mass index at the beginning of pregnancy, and 83% of newborns had an appropriate weight for gestational age. Maternal pre-pregnancy body mass index (BMI), gestational weight gain (GWG), and placental weight were independently correlated with birth weight. GWG was not related to the pre-pregnancy BMI. EPIC-FFQ evaluation showed that 30% of women adhered to the European Food Safety Authority (EFSA) ranges for macronutrient intake. In most pregnant women (98.1%), consumption of water was below recommendations. Comparing women with intakes within EFSA ranges for macronutrients with those who did not, no differences were found in BMI, GWG, and neonatal or placental weight. Neither maternal nor neonatal parameters were associated with the maternal dietary profiles. Conclusions In our population, maternal pre-pregnancy BMI, GWG, and placental weight are determinants of birth weight percentile, while no association was found with maternal nutrition. Future studies should explore associations through all infancy. Impact Maternal anthropometrics and nutrition status may affect offspring birth weight. In 503 healthy women, maternal pre-pregnancy body mass index (BMI), gestational weight gain (GWG), and placental weight were independently correlated to neonatal birth weight. GWG was not related to the pre-pregnancy BMI. In all, 30% of women respected the EFSA ranges for macronutrients. Neither maternal nor neonatal parameters were associated with maternal dietary profiles considered in this study. Maternal pre-pregnancy BMI, GWG, and placental weight are determinants of neonatal birth weight percentile, while a connection with maternal nutrition profiles was not found.

Published
2020

36. gDNA qPCR is statistically more reliable than mRNA analysis in detecting leukemic cells to monitor CML

Author

Andrea Conti, Anna Michelato, Cristina Barlassina, Giovanni Micheloni, Alessia Rainero, Giorgia Millefanti, Matteo Barcella, Francesca D'Avila, Eleonora Piscitelli, Ksenija Buklijas, Silvia M. Sirchia, Cristina Pirrone, Orietta Spinelli, Emanuela Maserati, Fabrizio Angaroni, R. Casalone, Giovanni Porta, Lucia Tararà, Massimo Caccia, Roberto Valli, Rainero, A, Angaroni, F, Conti, A, Pirrone, C, Micheloni, G, Tarara, L, Millefanti, G, Maserati, E, Valli, R, Spinelli, O, Buklijas, K, Michelato, A, Casalone, R, Barlassina, C, Barcella, M, Sirchia, S, Piscitelli, E, Caccia, M, and Porta, G

Subjects
Male, 0301 basic medicine, Cancer Research, Immunology, Fusion Proteins, bcr-abl, Leukemia, Myelogenous, Chronic,Treatment Outcome, Real-Time Polymerase Chain Reaction, Article, Follow-Up Studie, Fusion gene, Young Adult, 03 medical and health sciences, Cellular and Molecular Neuroscience, 0302 clinical medicine, Cancer stem cell, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, Precursor B-Cell Lymphoblastic Leukemia-Lymphoma, hemic and lymphatic diseases, Humans, Medicine, RNA, Messenger, lcsh:QH573-671, Protein Kinase Inhibitors, Aged, Cell Biology, Reverse Transcriptase Polymerase Chain Reaction, business.industry, lcsh:Cytology, Reproducibility of Results, Myeloid leukemia, DNA, Middle Aged, Protein-Tyrosine Kinases, medicine.disease, genomic DNA, Leukemia, Haematopoiesis, Treatment Outcome, 030104 developmental biology, Real-time polymerase chain reaction, 030220 oncology & carcinogenesis, Imatinib Mesylate, Neoplastic Stem Cells, Cancer research, Female, Stem cell, business, Follow-Up Studies
Abstract

Chronic Myeloid Leukemia (CML) is a stem cell cancer that arises when t(9;22) translocation occurs in a hematopoietic stem cells. This event results in the expression of the BCR-ABL1 fusion gene, which codes for a constitutively active tyrosine kinase that is responsible for the transformation of a HSC into a CML stem cell, which then gives rise to a clonal myeloproliferative disease. The introduction of Tyrosine Kinase Inhibitors (TKIs) has revolutionized the management of the disease. However, these drugs do not seem to be able to eradicate the malignancy. Indeed, discontinuation trials (STIM; TWISER; DADI) for those patients who achieved a profound molecular response showed 50% relapsing within 12 months. We performed a comparative analysis on 15 CML patients and one B-ALL patient, between the standard quantitative reverse-transcriptase PCR (qRT–PCR) and our genomic DNA patient-specific quantitative PCR assay (gDNA qPCR). Here we demonstrate that gDNA qPCR is better than standard qRT–PCR in disease monitoring after an average follow-up period of 200 days. Specifically, we statistically demonstrated that DNA negativity is more reliable than RNA negativity in indicating when TKIs therapy can be safely stopped.

Published
2018
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37. DNA methylation in the diagnosis of monogenic diseases

Author

Maurizio Genuardi, Cristiana Lo Lo Nigro, Andrea Riccio, Flavia Cerrato, Eugenio Sangiorgi, Elisabetta Tabolacci, Francesca Ariani, Giovanni Neri, Fabio Coppedè, Luciano Calzari, Fiorella Gurrieri, Alessandro De Luca, Gabriella Maria Squeo, Angela Sparago, Giuseppe Merla, Fulvia Brugnoletti, Isabella Torrente, Monica Miozzo, Silvia Russo, Silvia Tabano, Silvia M. Sirchia, Cristina Gervasini, Emiliano Giardina, Cerrato, F., Sparago, A., Ariani, F., Brugnoletti, F., Calzari, L., Coppede, F., De Luca, A., Gervasini, C., Giardina, E., Gurrieri, F., Nigro, C. L., Merla, G., Miozzo, M., Russo, S., Sangiorgi, E., Sirchia, S. M., Squeo, G. M., Tabano, S., Tabolacci, E., Torrente, I., Genuardi, M., Neri, G., Riccio, A., and Lo Nigro, C.

Subjects
0301 basic medicine, Epigenomics, Methyltransferase, Genetic testing, lcsh:QH426-470, Prenatal diagnosis, neuromuscular diseases, Review, 030105 genetics & heredity, Settore MED/03 - GENETICA MEDICA, Genome, Imprinting disorder, 03 medical and health sciences, chemistry.chemical_compound, Developmental delay/intellectual disability disorder, Genetics, medicine, imprinting disorders, Humans, Genetics (clinical), DNA methylation, developmental delay/intellectual disability disorders, epi-signatures, genetic testing, hereditary tumors, high-throughput analysis, prenatal diagnosis, biology, medicine.diagnostic_test, Genome, Human, High-throughput analysi, Genetic Diseases, Inborn, Methylation, Developmental delay/intellectual disability disorders, Epi-signatures, Hereditary tumors, High-throughput analysis, Imprinting disorders, Neuromuscular diseases, Neuromuscular disease, lcsh:Genetics, 030104 developmental biology, Histone, Phenotype, chemistry, Settore MED/03, biology.protein, Hereditary tumor, Human genome, Epi-signature, DNA
Abstract

DNA methylation in the human genome is largely programmed and shaped by transcription factor binding and interaction between DNA methyltransferases and histone marks during gamete and embryo development. Normal methylation profiles can be modified at single or multiple loci, more frequently as consequences of genetic variants acting in cis or in trans, or in some cases stochastically or through interaction with environmental factors. For many developmental disorders, specific methylation patterns or signatures can be detected in blood DNA. The recent use of high-throughput assays investigating the whole genome has largely increased the number of diseases for which DNA methylation analysis provides information for their diagnosis. Here, we review the methylation abnormalities that have been associated with mono/oligogenic diseases, their relationship with genotype and phenotype and relevance for diagnosis, as well as the limitations in their use and interpretation of results.

Published
2020
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38. Losses of Heterozygosity in Oral and Oropharyngeal Epithelial Carcinomas

Author

Isabella Garagiola, Giuseppe Simoni, Silvestre Galioto, Francesca Romana Grati, Francesca Dulcetti, F. Rossella, P. Serafini, Roberto Brusati, Elena Sironi, A. Bozzetti, Silvia M. Sirchia, Grati, F, Sirchia, S, Garagiola, I, Sironi, E, Galioto, S, Rossella, F, Serafini, P, Dulcetti, F, Bozzetti, A, Brusati, R, and Simoni, G

Subjects
Oropharyngeal Neoplasm, Adult, Male, Cancer Research, Loss of Heterozygosity, Biology, medicine.disease_cause, Loss of heterozygosity, Gene Frequency, Genetics, medicine, Humans, Genes, Tumor Suppressor, Lymphocytes, Molecular Biology, Allele frequency, Alleles, Aged, Neoplasm Staging, Allele, Aged, 80 and over, Mouth neoplasm, Chi-Square Distribution, Microsatellite instability, Lymphatic Metastasi, Middle Aged, medicine.disease, Mouth Neoplasm, Molecular biology, Oropharyngeal Neoplasms, Epidermoid carcinoma, Lymphatic Metastasis, Carcinoma, Squamous Cell, Microsatellite Repeat, Microsatellite, Female, Mouth Neoplasms, Carcinogenesis, Human, Microsatellite Repeats
Abstract

We analyzed 25 oral and oropharyngeal epithelial carcinomas for loss of heterozygosity (LOH) and microsatellite instability by using 55 oligonucleotide repeat markers located in 45 chromosomal regions. The aim was to identify which chromosomal regions and tumor-suppressor genes (TSGs) are preferentially lost in these tumors and to relate LOH at specific loci to clinicopathologic data. The analysis was performed on tumor tissue and on a corresponding normal tissue (blood lymphocytes) with the use of the polymerase chain reaction technique followed by microsatellite allele separation with denaturing gel electrophoresis. Thirty-two of 45 chromosomal regions demonstrated a significant (>/=20%) incidence of LOH. An allelic loss of >/=50% was found in 9p21 (77.8%), 8p22-23 (70%), 3p12 (61.5%), 1p36.1 and 12q22 (60%), 3q28 (57.1%), 5q23.3 (54.5%), 3p25-26, 3p24, and 7q35 (50%). We did not find any microsatellite instability. Our results suggest that in addition to a group of TSGs, pleiotropic for several tumor types, other suppressor genes are specifically involved in oral and oropharyngeal carcinogenesis

Published
2000
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39. X chromosome inactivation pattern in BRCA gene mutation carriers

Author

Monica Miozzo, Silvia Tabano, Siranoush Manoukian, Mariarosaria Calvello, Bernard Peissel, F.R. Grati, Valeria Pensotti, Claudia Allemani, Silva M. Sirchia, John Burn, Patrizia Colapietro, Paolo Radice, Sara Pizzamiglio, Paolo Verderio, Manoukian, S, Verderio, P, Tabano, S, Colapietro, P, Pizzamiglio, S, Grati, F, Calvello, M, Peissel, B, Burn, J, Pensotti, V, Allemani, C, Sirchia, S, Radice, P, and Miozzo, M

Subjects
Oncology, Adult, medicine.medical_specialty, Heterozygote, Cancer Research, DNA Mutational Analysis, BRCA gene, Genes, BRCA2, Genes, BRCA1, Breast Neoplasms, Predictive Value of Test, Gene mutation, Biology, X-inactivation, DNA Mutational Analysi, Young Adult, Predictive Value of Tests, X Chromosome Inactivation, Internal medicine, medicine, Humans, Chemotherapy, Aged, Genetics, Ovarian Neoplasms, Aged, 80 and over, Ovarian Neoplasm, BRCA mutation, Carcinoma, Case-control study, Cancer, HUMARA test, Odds ratio, Middle Aged, medicine.disease, Ageing, Receptors, Androgen, Case-Control Studies, Mutation (genetic algorithm), Mutation, Female, Ovarian cancer, Case-Control Studie, Breast Neoplasm, Human
Abstract

An association of preferential X chromosome inactivation (XCI) with BRCA gene status and breast/ovarian cancer risk has been reported. We evaluated XCI in a large group of BRCA mutation carriers compared to non-carriers and investigated associations between preferential XCI (≥90:10) and age, mutated gene, cancer development and chemotherapy. XCI was analysed by human androgen receptor (HUMARA) assay and pyrosequencing in 437 BRCA1 or BRCA2 mutation carriers and 445 age-matched controls. The distribution of XCI patterns in the two groups was compared by logistic regression analysis. The association between preferential XCI and selected variables was investigated in both univariate and multivariate fashion. In univariate analyses preferential XCI was not significantly associated with the probability of being a BRCA mutation carrier, nor with cancer status, whereas chemotherapeutic regime and age both showed a significant association. In multivariate analysis only age maintained significance (odds ratio, 1.056; 95% confidence interval, 1.016-1.096). Our findings do not support the usefulness of XCI analysis for the identification of BRCA mutation carriers and cancer risk assessment. The increasing preferential XCI frequency with ageing and the association with chemotherapy justify extending the investigation to other categories of female cancer patients to identify possible X-linked loci implicated in cell survival. © 2012 Elsevier Ltd. All rights reserved.

Published
2013

40. Radiomic Gradient in Peritumoural Tissue of Liver Metastases: A Biomarker for Clinical Practice? Analysing Density, Entropy, and Uniformity Variations with Distance from the Tumour.

Author

Fiz F, Ragaini EM, Sirchia S, Masala C, Viganò S, Francone M, Cavinato L, Lanzarone E, Ammirabile A, and Viganò L

Abstract

The radiomic analysis of the tissue surrounding colorectal liver metastases (CRLM) enhances the prediction accuracy of pathology data and survival. We explored the variation of the textural features in the peritumoural tissue as the distance from CRLM increases. We considered patients with hypodense CRLMs >10 mm and high-quality computed tomography (CT). In the portal phase, we segmented (1) the tumour, (2) a series of concentric rims at a progressively increasing distance from CRLM (from one to ten millimetres), and (3) a cylinder of normal parenchyma (Liver-VOI). Sixty-three CRLMs in 51 patients were analysed. Median peritumoural HU values were similar to Liver-VOI, except for the first millimetre around the CRLM. Entropy progressively decreased (from 3.11 of CRLM to 2.54 of Liver-VOI), while uniformity increased (from 0.135 to 0.199, p < 0.001). At 10 mm from CRLM, entropy was similar to the Liver-VOI in 62% of cases and uniformity in 46%. In small CRLMs (≤30 mm) and responders to chemotherapy, normalisation of entropy and uniformity values occurred in a higher proportion of cases and at a shorter distance. The radiomic analysis of the parenchyma surrounding CRLMs unveiled a wide halo of progressively decreasing entropy and increasing uniformity despite a normal radiological aspect. Underlying pathology data should be investigated.

Published
2024
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41. Assessment of pregnancy dietary intake and association with maternal and neonatal outcomes.

Author

Costanza J, Camanni M, Ferrari MM, De Cosmi V, Tabano S, Fontana L, Radaelli T, Privitera G, Alberico D, Colapietro P, Motta S, Sirchia S, Stampalija T, Tabasso C, Roggero P, Parazzini F, Mosca F, Ferrazzi E, Bosari S, Miozzo M, and Agostoni C

Subjects
Birth Weight, Body Mass Index, Eating, Female, Humans, Infant, Newborn, Placenta, Pregnancy, Pregnancy Outcome, Prospective Studies, Gestational Weight Gain, Weight Gain
Abstract

Background: Maternal dietary habits are contributors of maternal and fetal health; however, available data are heterogeneous and not conclusive., Methods: Nutrient intake during pregnancy was assessed in 503 women with uncomplicated pregnancies, using the validated Food Frequency Questionnaire developed by the European Prospective Investigation into Cancer and Nutrition (EPIC-FFQ)., Results: In all, 68% of women had a normal body mass index at the beginning of pregnancy, and 83% of newborns had an appropriate weight for gestational age. Maternal pre-pregnancy body mass index (BMI), gestational weight gain (GWG), and placental weight were independently correlated with birth weight. GWG was not related to the pre-pregnancy BMI. EPIC-FFQ evaluation showed that 30% of women adhered to the European Food Safety Authority (EFSA) ranges for macronutrient intake. In most pregnant women (98.1%), consumption of water was below recommendations. Comparing women with intakes within EFSA ranges for macronutrients with those who did not, no differences were found in BMI, GWG, and neonatal or placental weight. Neither maternal nor neonatal parameters were associated with the maternal dietary profiles., Conclusions: In our population, maternal pre-pregnancy BMI, GWG, and placental weight are determinants of birth weight percentile, while no association was found with maternal nutrition. Future studies should explore associations through all infancy., Impact: Maternal anthropometrics and nutrition status may affect offspring birth weight. In 503 healthy women, maternal pre-pregnancy body mass index (BMI), gestational weight gain (GWG), and placental weight were independently correlated to neonatal birth weight. GWG was not related to the pre-pregnancy BMI. In all, 30% of women respected the EFSA ranges for macronutrients. Neither maternal nor neonatal parameters were associated with maternal dietary profiles considered in this study. Maternal pre-pregnancy BMI, GWG, and placental weight are determinants of neonatal birth weight percentile, while a connection with maternal nutrition profiles was not found., (© 2021. The Author(s).)

Published
2022
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43. A multi-method approach to the molecular diagnosis of overt and borderline 11p15.5 defects underlying Silver-Russell and Beckwith-Wiedemann syndromes.

Author

Russo S, Calzari L, Mussa A, Mainini E, Cassina M, Di Candia S, Clementi M, Guzzetti S, Tabano S, Miozzo M, Sirchia S, Finelli P, Prontera P, Maitz S, Sorge G, Calcagno A, Maghnie M, Divizia MT, Melis D, Manfredini E, Ferrero GB, Pecile V, and Larizza L

Subjects
Beckwith-Wiedemann Syndrome genetics, Blotting, Southern methods, Child, Child, Preschool, CpG Islands genetics, DNA Methylation genetics, Epigenesis, Genetic genetics, Female, Humans, Infant, Male, Mosaicism, Multiplex Polymerase Chain Reaction methods, Oligonucleotide Array Sequence Analysis, Silver-Russell Syndrome genetics, Beckwith-Wiedemann Syndrome diagnosis, Chromosomes, Human, Pair 11 genetics, Silver-Russell Syndrome diagnosis
Abstract

Background: Multiple (epi)genetic defects affecting the expression of the imprinted genes within the 11p15.5 chromosomal region underlie Silver-Russell (SRS) and Beckwith-Wiedemann (BWS) syndromes. The molecular diagnosis of these opposite growth disorders requires a multi-approach flowchart to disclose known primary and secondary (epi)genetic alterations; however, up to 20 and 30 % of clinically diagnosed BWS and SRS cases remain without molecular diagnosis. The complex structure of the 11p15 region with variable CpG methylation and low-rate mosaicism may account for missed diagnoses. Here, we demonstrate the relevance of complementary techniques for the assessment of different CpGs and the importance of testing multiple tissues to increase the SRS and BWS detection rate., Results: Molecular testing of 147 and 450 clinically diagnosed SRS and BWS cases provided diagnosis in 34 SRS and 185 BWS patients, with 9 SRS and 21 BWS cases remaining undiagnosed and herein referred to as "borderline." A flowchart including complementary techniques and, when applicable, the analysis of buccal swabs, allowed confirmation of the molecular diagnosis in all borderline cases. Comparison of methylation levels by methylation-specific multiplex ligation-dependent probe amplification (MS-MLPA) in borderline and control cases defined an interval of H19/IGF2:IG-DMR loss of methylation that was distinct between "easy to diagnose" and "borderline" cases, which were characterized by values ≤mean -3 standard deviations (SDs) compared to controls. Values ≥mean +1 SD at H19/IGF2: IG-DMR were assigned to borderline hypermethylated BWS cases and those ≤mean -2 SD at KCNQ1OT1: TSS-DMR to hypomethylated BWS cases; these were supported by quantitative pyrosequencing or Southern blot analysis. Six BWS cases suspected to carry mosaic paternal uniparental disomy of chromosome 11 were confirmed by SNP array, which detected mosaicism till 10 %. Regarding the clinical presentation, borderline SRS were representative of the syndromic phenotype, with exception of one patient, whereas BWS cases showed low frequency of the most common features except hemihyperplasia., Conclusions: A conclusive molecular diagnosis was reached in borderline methylation cases, increasing the detection rate by 6 % for SRS and 5 % for BWS cases. The introduction of complementary techniques and additional tissue analyses into routine diagnostic work-up should facilitate the identification of cases undiagnosed because of mosaicism, a distinctive feature of epigenetic disorders.

Published
2016
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44. Beckwith-Wiedemann syndrome prenatal diagnosis by methylation analysis in chorionic villi.

Author

Paganini L, Carlessi N, Fontana L, Silipigni R, Motta S, Fiori S, Guerneri S, Lalatta F, Cereda A, Sirchia S, Miozzo M, and Tabano S

Subjects
Beckwith-Wiedemann Syndrome genetics, Cells, Cultured, Female, Genomic Imprinting, Humans, Pregnancy, Promoter Regions, Genetic, Beckwith-Wiedemann Syndrome diagnosis, Chorionic Villi metabolism, DNA Methylation, Prenatal Diagnosis
Abstract

Beckwith-Wiedemann syndrome (BWS) is an imprinting disorder that can be prenatally suspected or diagnosed based on established clinical guidelines. Molecular confirmation is commonly performed on amniocytes. The possibility to use fresh (CVF) and cultured (CVC) chorionic villi has never been investigated. To verify whether CVF and CVC are reliable sources of DNA to study fetal methylation, we used pyrosequencing to test the methylation level of a number of differentially methylated regions (DMRs) at several imprinted loci (ICR1, ICR2, H19, PWS/AS-ICR, GNASXL, GNAS1A, ZAC/PLAGL1, and MEST) and at non-imprinted MGMT and RASSF1A promoters. We analyzed these regions in 19 healthy pregnancies and highlighted stable methylation levels between CVF and CVC at ICR1, ICR2, GNASXL, PWS/AS-ICR, and MEST. Conversely, the methylation levels at H19 promoter, GNAS1A and ZAC/PLAGL1 were different in CVC compared to fresh CV. We also investigated ICR1 and ICR2 methylation level of CVF/CVC of 2 BWS-suspected fetuses (P1 and P2). P1 showed ICR2 hypomethylation, P2 showed normal methylation at both ICR1 and ICR2. Our findings, although limited to one case of BWS fetus with an imprinting defect, can suggest that ICR1 and ICR2, but not H19, could be reliable targets for prenatal BWS diagnosis by methylation test in CVF and CVC. In addition, PWS/AS-ICR, GNASXL, and MEST, but not GNAS1A and ZAC/PLAGL1, are steadily hemimethylated in CV from healthy pregnancies, independently from culture. Thus, prenatal investigation of genomic imprinting in CV needs to be validated in a locus-specific manner.

Published
2015
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45. Increased loss of the Y chromosome in peripheral blood cells in male patients with autoimmune thyroiditis.

Author

Persani L, Bonomi M, Lleo A, Pasini S, Civardi F, Bianchi I, Campi I, Finelli P, Miozzo M, Castronovo C, Sirchia S, Gershwin ME, and Invernizzi P

Subjects
Age Factors, Case-Control Studies, Female, Humans, Male, Sex Factors, Thyroiditis, Autoimmune immunology, Blood Cells metabolism, Chromosome Deletion, Chromosomes, Human, Y, Thyroiditis, Autoimmune genetics
Abstract

Multiple mechanisms have been proposed to explain the peculiar distribution of autoimmune thyroiditis (AIT) among women and men. Most attention has been focused on the detection of the role of estrogens and the X chromosome. Specifically, a potential role for X haploinsufficiency has been proposed in the female patient population and an association with the disease has been confirmed. Our knowledge of the etiopathogenesis of autoimmunity in male patients remains, however, limited. Next to the possible role of androgens and their imbalances, the Y chromosome appears as a potential candidate for influence of the immune function in men. Herein we analyzed a population of male patients with AIT (n=31) and healthy controls (n=88) to define a potential association of disease and the loss of the Y chromosome. Y chromosome loss increases in AIT compared to unaffected subjects; these phenomenon increases with aging as expected, however, the degree of loss is significantly increased in the patient population compared to the healthy controls. We were, thus, able to confirm the existence of an analogous mechanism in the male population to previously identified X haploinsufficiency in female patients with AIT. We propose that this commonality might represent a relevant feature in the etiopathogenesis of AIT that should be further investigated., (Copyright © 2011 Elsevier Ltd. All rights reserved.)

Published
2012
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46. The mammary gland and the homeobox gene Otx1.

Author

Pagani IS, Terrinoni A, Marenghi L, Zucchi I, Chiaravalli AM, Serra V, Rovera F, Sirchia S, Dionigi G, Miozzo M, Frattini A, Ferrari A, Capella C, Pasquali F, Lo Curto F, Albertini A, Melino G, and Porta G

Subjects
Animals, Epithelial Cells metabolism, Female, Humans, Mammary Glands, Animal embryology, Mammary Glands, Human embryology, Neoplastic Stem Cells, Breast Neoplasms metabolism, Breast Neoplasms pathology, Otx Transcription Factors metabolism
Abstract

The mammary gland, the unique organ that primarily form at puberty, is an ideal model to study the functions of homeobox (HB) genes in both development and tumorigenesis. HB genes comprise a large family of developmental regulators that have a critical role in cell growth and differentiation. In the normal mammary gland, homeobox genes are involved in ductal formation, epithelial branching, and lobulo-alveolar development by regulating epithelial proliferation and differentiation. The HB genes are controlled in a spatial and temporal manner in both stromal and epithelial cells. They are coordinately regulated by hormones and extracellular matrix, suggesting that many signaling pathways are involved in homeobox gene functions. When homeobox genes are misexpressed in animal models, different defects are displayed in mammary gland development. Aberrant expression of homeobox genes, overexpressed or downregulated, is found in primary carcinomas and in breast cancer. The Otx1 HB gene is a classic regulatory of nervous system development during embryogenesis. Postnatally Otx1 is transcribed in the anterior pituitary gland, where activates transcription of the pituitary hormones, and plays a role in hematopoiesis, enhancing pluripotent cells, and erythroid differentiation. Otx1 can still be detected in mature cells of the erythroid and megacaryocytic lineage. During cyclical development of mammary gland, the Otx1 gene is overexpressed in lactation, confirming a role of this transcription factor in cell differentiation. Recent studies report that Otx1 is overexpressed in breast cancer. Otx1 is expressed during embryogenesis, and it is expressed again during carcinogenesis, implying its possible function in differentiation of neoplastic cells., (© 2010 Wiley Periodicals, Inc.)

Published
2010
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47. Preferential X chromosome loss but random inactivation characterize primary biliary cirrhosis.

Author

Miozzo M, Selmi C, Gentilin B, Grati FR, Sirchia S, Oertelt S, Zuin M, Gershwin ME, Podda M, and Invernizzi P

Subjects
Adult, Aged, Aged, 80 and over, Female, Humans, Male, Microsatellite Repeats, Middle Aged, Chromosome Aberrations, Chromosomes, Human, X, Liver Cirrhosis, Biliary genetics
Abstract

Unlabelled: Recent work has demonstrated enhanced X monosomy in women with primary biliary cirrhosis (PBC) as well as two other female-predominant autoimmune diseases, systemic sclerosis and autoimmune thyroid disease. To further our understanding of these events, we have investigated the mechanisms of X chromosome loss and X chromosome inactivation (XCI) in 166 women with PBC and 226 rigorously age-matched healthy and liver disease controls. X chromosome analysis and determination of loss pattern was performed by quantitative fluorescent polymerase chain reaction (QF-PCR) with 4 X-linked short tandem repeats. Further definition of the XCI was based on analysis of methylation-sensitive restriction sites. Importantly, in PBC the X chromosome loss occurs not only more frequently but also in a preferential fashion. This observation supports our thesis that the enhanced X monosomy involves only one parentally derived chromosome and is not secondary to a constitutive non random pattern of XCI. In fact, in the presence of monosomy, the lost X chromosome is necessarily the inactive homologue., Conclusion: The finding that the X chromosome loss is preferential suggests the critical involvement of X chromosome gene products in the female predisposition to PBC and also emphasizes the need to determine the parental origin of the maintained chromosome to investigate the role of imprinting.

Published
2007
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48. Fetal and placental chromosomal mosaicism revealed by QF-PCR in severe IUGR pregnancies.

Author

Grati FR, Miozzo M, Cassani B, Rossella F, Antonazzo P, Gentilin B, Sirchia SM, Mori L, Rigano S, Bulfamante G, Cetin I, and Simoni G

Subjects
Adult, Cells, Cultured, Chromosome Banding, Female, Fetal Growth Retardation diagnostic imaging, Fetal Growth Retardation etiology, Fluorescence, Gestational Age, Humans, In Situ Hybridization, Fluorescence, Karyotyping, Leukocytes, Mononuclear, Male, Phenotype, Polymerase Chain Reaction methods, Pregnancy, Tandem Repeat Sequences genetics, Ultrasonography, Chromosomes, Human, Fetal Development genetics, Fetal Growth Retardation genetics, Genetic Predisposition to Disease, Mosaicism embryology, Placenta pathology
Abstract

A number of genetic and environmental factors are taken into account as responsible for intrauterine growth restriction (IUGR); nevertheless, the relevance of genetic alteration in IUGR aetiology remains to be determined. The aim of this study was to investigate using a combined cytogenetic-molecular approach, improved by a new application of QF-PCR method, the presence of mosaic chromosomal changes in fetal/placental samples from 12 pregnancies with unexplained severe IUGR. This multiple approach allowed us to reveal and quantify subtle chromosomal mosaicisms with less than 5% of trisomic cells even in cases in which cytogenetic and FISH analyses failed to reveal them. These are three pregnancies with a mosaic trisomy for chromosomes 7, 2 and 14; the former case presented matUPD7 and was previously described in this journal (Placenta 22 (2001) 813) in association with pre- and postnatal growth restriction. It is intriguing that chromosomes 7, 2 and 14 are known or suspected to harbour imprinted genes, so that an unbalanced gene dosage in a subset of cells during embryonic development could lead to an early impairment of placental function. Our findings indicate that extensive molecular and cytogenetic studies of IUGR fetal and placental tissues are necessary to reveal at least part of the heterogeneous genetic lesions implicated in IUGR phenotypes.

Published
2005
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49. Detection of maternal DNA in cord blood at birth after elective caesarean section or vaginal delivery.

Author

Semprini AE, De Andreis C, Fiore S, Garagiola I, Sirchia SM, Savasi V, Newell ML, and Simoni G

Subjects
Blood Cells virology, Cesarean Section, DNA genetics, Female, HIV Seronegativity, Humans, Infant, Newborn, Infectious Disease Transmission, Vertical, Maternal-Fetal Exchange, Pregnancy, Blood Cells chemistry, DNA analysis, Delivery, Obstetric, Fetal Blood virology, HIV-1
Published
2000
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50. Evidence of epigenetic changes affecting the chromatin state of the retinoic acid receptor beta2 promoter in breast cancer cells.

Author

Sirchia SM, Ferguson AT, Sironi E, Subramanyan S, Orlandi R, Sukumar S, and Sacchi N

Subjects
Antimetabolites, Antineoplastic, Azacitidine analogs & derivatives, Azacitidine pharmacology, Breast cytology, Breast Neoplasms drug therapy, Cell Line, CpG Islands, DNA Methylation, Decitabine, Enzyme Inhibitors pharmacology, Epithelial Cells cytology, Female, Gene Expression Regulation drug effects, Histone Deacetylase Inhibitors, Humans, Hydroxamic Acids pharmacology, Promoter Regions, Genetic, Receptors, Estrogen metabolism, Receptors, Retinoic Acid drug effects, Receptors, Retinoic Acid metabolism, Tretinoin pharmacology, Tumor Cells, Cultured, Breast Neoplasms genetics, Chromatin genetics, Receptors, Retinoic Acid genetics
Abstract

Retinoic acid (RA)-resistance in breast cancer cells has been associated with irreversible loss of retinoic acid receptor beta, RARbeta, gene expression. Search of the causes affecting RARbeta gene activity has been oriented at identifying possible differences either at the level of one of the RARbeta promoters, RARbeta2, or at regulatory factors. We hypothesized that loss of RARbeta2 activity occurs as a result of multiple factors, including epigenetic modifications, which can pattern RARbeta2 chromatin state. Using methylation-specific PCR, we found hypermethylation at RARbeta2 in a significant proportion of both breast cancer cell lines and primary breast tumors. Treatment of cells with a methylated RARbeta2 promoter, by means of the DNA methyltransferase inhibitor 5-Aza-2'-deoxycytidine (5-Aza-CdR), led to demethylation within RARbeta2 and expression of RARbeta indicating that DNA methylation is at least one factor, contributing to RARbeta inactivity. However, identically methylated promoters can differentially respond to RA, suggesting that RARbeta2 activity may be associated to different repressive chromatin states. This supposition is supported by the finding that the more stable repressive RARbeta2 state in the RA-resistant MDA-MB-231 cell line can be alleviated by the HDAC inhibitor, trichostatin A (TSA), with restoration of RA-induced RARbeta transcription. Thus, chromatin-remodeling drugs might provide a strategy to restore RARbeta activity, and help to overcome the hurdle of RA-resistance in breast cancer.

Published
2000
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