Your search keyword '"Pierluigi Strippoli"' showing total 99 results

1. Commentary to the article: an estimation of the number of cells in the human body

Author

Pierluigi Strippoli, Raffaella Casadei, Flavia Frabetti, Lorenza Vitale, and Silvia Canaider

Subjects

Biology (General), QH301-705.5, Human anatomy, QM1-695, Physiology, QP1-981

Published

2024

2. Corrigendum: One-carbon pathway metabolites are altered in the plasma of subjects with Down syndrome: relation to chromosomal dosage

Author

Beatrice Vione, Giuseppe Ramacieri, Giacomo Zavaroni, Angela Piano, Giorgia La Rocca, Maria Caracausi, Lorenza Vitale, Allison Piovesan, Caterina Gori, Gian Luca Pirazzoli, Pierluigi Strippoli, Guido Cocchi, Luigi Corvaglia, Chiara Locatelli, Maria Chiara Pelleri, and Francesca Antonaros

Subjects

trisomy 21, Down syndrome, one-carbon pathway, folates, chromosomal dosage, Medicine (General), R5-920

Published

2024

3. Zinc metabolism and its role in immunity status in subjects with trisomy 21: chromosomal dosage effect

Author

Giuseppe Ramacieri, Chiara Locatelli, Michela Semprini, Maria Chiara Pelleri, Maria Caracausi, Allison Piovesan, Michela Cicilloni, Marco Vigna, Lorenza Vitale, Giacomo Sperti, Luigi Tommaso Corvaglia, Gian Luca Pirazzoli, Pierluigi Strippoli, Francesca Catapano, Beatrice Vione, and Francesca Antonaros

Subjects

down syndrome, zinc, immunity disorder, transcriptome, integration, Immunologic diseases. Allergy, RC581-607

Abstract

IntroductionTrisomy 21 (T21), which causes Down syndrome (DS), is the most common chromosomal aneuploidy in humankind and includes different clinical comorbidities, among which the alteration of the immune system has a heavy impact on patient’s lives. A molecule with an important role in immune response is zinc and it is known that its concentration is significantly lower in children with T21. Different hypotheses were made about this metabolic alteration and one of the reasons might be the overexpression of superoxide dismutase 1 (SOD1) gene, as zinc is part of the SOD1 active enzymatic center.MethodsThe aim of our work is to explore if there is a linear correlation between zinc level and immune cell levels measured in a total of 217 blood samples from subjects with T21. Furthermore, transcriptome map analyses were performed using Transcriptome Mapper (TRAM) software to investigate whether a difference in gene expression is detectable between subjects with T21 and euploid control group in tissues and cells involved in the immune response such as lymphoblastoid cells, thymus and white blood cells.ResultsOur results have confirmed the literature data stating that the blood zinc level in subjects with T21 is lower compared to the general population; in addition, we report that the T21/control zinc concentration ratio is 2:3, consistent with a chromosomal dosage effect due to the presence of three copies of chromosome 21. The transcriptome map analyses showed an alteration of some gene’s expression which might explain low levels of zinc in the blood.DiscussionOur data suggest that zinc level is not associated with the levels of immunity cells or proteins analyzed themselves and rather the main role of this ion might be played in altering immune cell function.

Published

2024

4. Down Syndrome: how to communicate the diagnosis

Author

Caterina Gori, Guido Cocchi, Luigi Tommaso Corvaglia, Giuseppe Ramacieri, Francesca Pulina, Giacomo Sperti, Valeria Cagnazzo, Francesca Catapano, Pierluigi Strippoli, Duccio Maria Cordelli, and Chiara Locatelli

Subjects

Down Syndrome, Communication, Prenatal diagnosis, Postnatal diagnosis, Decision-making process, Pediatrics, RJ1-570

Abstract

Abstract Communicating the diagnosis of Down Syndrome to a couple of parents is never easy, whether before or after birth. As doctors, we must certainly rely on our own relational skills, but it is also necessary to be confident in some general indications, which are often overlooked in the strict hospital routine. This article is intended as a summary of the main articles published on this subject in the international literature, collecting and summarising the most important indications that have emerged in years of medical practice all over the world as well as in our personal experience. The diffusion of these guidelines is essential to help the doctor in this difficult task, on which there is often little training, and above all to guarantee to the parents the least traumatic communication possible.

Published

2023

5. Partial trisomy 21 with or without highly restricted Down syndrome critical region (HR-DSCR): report of two new cases and reanalysis of the genotype–phenotype association

Author

Maria Chiara Pelleri, Chiara Locatelli, Teresa Mattina, Maria Clara Bonaglia, Francesca Piazza, Pamela Magini, Francesca Antonaros, Giuseppe Ramacieri, Beatrice Vione, Lorenza Vitale, Marco Seri, Pierluigi Strippoli, Guido Cocchi, Allison Piovesan, and Maria Caracausi

Subjects

Down syndrome, Partial trisomy 21, Highly restricted Down syndrome critical region, Internal medicine, RC31-1245, Genetics, QH426-470

Abstract

Abstract Background Down syndrome (DS) is caused by the presence of an extra copy of full or partial human chromosome 21 (Hsa21). Partial (segmental) trisomy 21 (PT21) is the duplication of only a delimited region of Hsa21 and can be associated or not to DS: the study of PT21 cases is an invaluable model for addressing genotype–phenotype correlation in DS. Previous works reported systematic reanalyses of 132 subjects with PT21 and allowed the identification of a 34-kb highly restricted DS critical region (HR-DSCR) as the minimal region whose duplication is shared by all PT21 subjects diagnosed with DS. Methods We report clinical data and cytogenetic analysis of two children with PT21, one with DS and the other without DS. Moreover, we performed a systematic bibliographic search for any new PT21 report. Results Clinical and cytogenetic analyses of the two PT21 children have been reported: in Case 1 the duplication involves the whole long arm of Hsa21, except for the last 2.7 Mb, which are deleted as a consequence of an isodicentric 21: the HR-DSCR is within the duplicated regions and the child is diagnosed with DS. In Case 2 the duplication involves 7.1 Mb of distal 21q22, with a deletion of 2.1 Mb of proximal 20p, as a consequence of an unbalanced translocation: the HR-DSCR is not duplicated and the child presents with psychomotor development delay but no clinical signs of DS. Furthermore, two PT21 reports recently published (named Case 3 and 4) have been discussed: Case 3 has DS diagnosis, nearly full trisomy for Hsa21 and a monosomy for the 21q22.3 region. Case 4 is a baby without DS and a 0.56-Mb duplication of 21q22.3. Genotype–phenotype correlation confirmed the presence of three copies of the HR-DSCR in all DS subjects and two copies in all non-DS individuals. Conclusions The results presented here are fully consistent with the hypothesis that the HR-DSCR is critically associated with DS diagnosis. No exception to this pathogenetic model was found. Further studies are needed to detect genetic determinants likely located in the HR-DSCR and possibly responsible for core DS features, in particular intellectual disability.

Published

2022

6. A reassessment of Jackson’s checklist and identification of two Down syndrome sub-phenotypes

Author

Chiara Locatelli, Sara Onnivello, Caterina Gori, Giuseppe Ramacieri, Francesca Pulina, Chiara Marcolin, Renzo Vianello, Beatrice Vione, Maria Caracausi, Maria Chiara Pelleri, Lorenza Vitale, Gian Luca Pirazzoli, Guido Cocchi, Luigi Corvaglia, Pierluigi Strippoli, Francesca Antonaros, Allison Piovesan, and Silvia Lanfranchi

Subjects

Medicine, Science

Abstract

Abstract Down syndrome (DS) is characterised by several clinical features including intellectual disability (ID) and craniofacial dysmorphisms. In 1976, Jackson and coll. identified a checklist of signs for clinical diagnosis of DS; the utility of these checklists in improving the accuracy of clinical diagnosis has been recently reaffirmed, but they have rarely been revised. The purpose of this work is to reassess the characteristic phenotypic signs and their frequencies in 233 DS subjects, following Jackson's checklist. 63.77% of the subjects showed more than 12 signs while none showed less than 5, confirming the effectiveness of Jackson's checklist for the clinical diagnosis of DS. An association between three phenotypic signs emerged, allowing us to distinguish two sub-phenotypes: Brachycephaly, short and broad Hands, short Neck (BHN), which is more frequent, and "non-BHN". The strong association of these signs might be interpreted in the context of the growth defects observed in DS children suggesting decreased cell proliferation. Lastly, cognitive assessments were investigated for 114 subjects. The lack of association between the presence of a physical sign or the number of signs present in a subject and cognitive skills disproves the stereotype that physical characteristics are predictive of degree of ID.

Published

2022

7. One-carbon pathway metabolites are altered in the plasma of subjects with Down syndrome: Relation to chromosomal dosage

Author

Beatrice Vione, Giuseppe Ramacieri, Giacomo Zavaroni, Angela Piano, Giorgia La Rocca, Maria Caracausi, Lorenza Vitale, Allison Piovesan, Caterina Gori, Gian Luca Pirazzoli, Pierluigi Strippoli, Guido Cocchi, Luigi Corvaglia, Chiara Locatelli, Maria Chiara Pelleri, and Francesca Antonaros

Subjects

trisomy 21, Down syndrome, one-carbon pathway, folates, chromosomal dosage, Medicine (General), R5-920

Abstract

IntroductionDown syndrome (DS) is the most common chromosomal disorder and it is caused by trisomy of chromosome 21 (Hsa21). Subjects with DS show a large heterogeneity of phenotypes and the most constant clinical features present are typical facies and intellectual disability (ID). Several studies demonstrated that trisomy 21 causes an alteration in the metabolic profile, involving among all the one-carbon cycle.MethodsWe performed enzyme-linked immunosorbent assays (ELISAs) to identify the concentration of 5 different intermediates of the one-carbon cycle in plasma samples obtained from a total of 164 subjects with DS compared to 54 euploid subjects. We investigated: tetrahydrofolate (THF; DS n = 108, control n = 41), 5-methyltetrahydrofolate (5-methyl-THF; DS n = 140, control n = 34), 5-formyltetrahydrofolate (5-formyl-THF; DS n = 80, control n = 21), S-adenosyl-homocysteine (SAH; DS n = 94, control n = 20) and S-adenosyl-methionine (SAM; DS n = 24, control n = 15).ResultsResults highlight specific alterations of THF with a median concentration ratio DS/control of 2:3, a decrease of a necessary molecule perfectly consistent with a chromosomal dosage effect. Moreover, SAM and SAH show a ratio DS/control of 1.82:1 and 3.6:1, respectively.DiscussionThe relevance of these results for the biology of intelligence and its impairment in trisomy 21 is discussed, leading to the final proposal of 5-methyl-THF as the best candidate for a clinical trial aimed at restoring the dysregulation of one-carbon cycle in trisomy 21, possibly improving cognitive skills of subjects with DS.

Published

2022

8. The transcriptome profile of human trisomy 21 blood cells

Author

Francesca Antonaros, Rossella Zenatelli, Giulia Guerri, Matteo Bertelli, Chiara Locatelli, Beatrice Vione, Francesca Catapano, Alice Gori, Lorenza Vitale, Maria Chiara Pelleri, Giuseppe Ramacieri, Guido Cocchi, Pierluigi Strippoli, Maria Caracausi, and Allison Piovesan

Subjects

Transcriptome, RNA sequencing, Blood cells, Human chromosome 21, Trisomy 21, Down syndrome, Medicine, Genetics, QH426-470

Abstract

Abstract Background Trisomy 21 (T21) is a genetic alteration characterised by the presence of an extra full or partial human chromosome 21 (Hsa21) leading to Down syndrome (DS), the most common form of intellectual disability (ID). It is broadly agreed that the presence of extra genetic material in T21 gives origin to an altered expression of genes located on Hsa21 leading to DS phenotype. The aim of this study was to analyse T21 and normal control blood cell gene expression profiles obtained by total RNA sequencing (RNA-Seq). Results The results were elaborated by the TRAM (Transcriptome Mapper) software which generated a differential transcriptome map between human T21 and normal control blood cells providing the gene expression ratios for 17,867 loci. The obtained gene expression profiles were validated through real-time reverse transcription polymerase chain reaction (RT-PCR) assay and compared with previously published data. A post-analysis through transcriptome mapping allowed the identification of the segmental (regional) variation of the expression level across the whole genome (segment-based analysis of expression). Interestingly, the most over-expressed genes encode for interferon-induced proteins, two of them (MX1 and MX2 genes) mapping on Hsa21 (21q22.3). The altered expression of genes involved in mitochondrial translation and energy production also emerged, followed by the altered expression of genes encoding for the folate cycle enzyme, GART, and the folate transporter, SLC19A1. Conclusions The alteration of these pathways might be linked and involved in the manifestation of ID in DS.

Published

2021

9. One-carbon pathway and cognitive skills in children with Down syndrome

Author

Francesca Antonaros, Silvia Lanfranchi, Chiara Locatelli, Anna Martelli, Giulia Olivucci, Elena Cicchini, Ludovica Carosi Diatricch, Elisa Mannini, Beatrice Vione, Agnese Feliciello, Giuseppe Ramacieri, Sara Onnivello, Renzo Vianello, Lorenza Vitale, Maria Chiara Pelleri, Pierluigi Strippoli, Guido Cocchi, Francesca Pulina, Allison Piovesan, and Maria Caracausi

Subjects

Medicine, Science

Abstract

Abstract This work investigates the role of metabolite levels in the intellectual impairment of subjects with Down syndrome (DS). Homocysteine, folate, vitamin B12, uric acid (UA), creatinine levels and MTHFR C677T genotype were analyzed in 147 subjects with DS. For 77 subjects, metabolite levels were correlated with cognitive tests. Griffiths-III test was administered to 28 subjects (3.08–6.16 years) and WPPSI-III test was administered to 49 subjects (7.08–16.08 years). Significant correlations were found among some metabolite levels and between homocysteine levels and MTHFR C677T genotype. Moreover, homocysteine, UA and creatinine levels resulted increased with age. We did not find any correlation between metabolites and cognitive test score in the younger group. Homocysteine showed statistically significant correlation with WPPSI-III subtest scores when its level is ≥ 7.35 µmol/L, remaining correlated in higher thresholds only for non-verbal area scores. Vitamin B12 showed correlations with all WPPSI-III subtest scores when its level is

Published

2021

10. Structural Characterization of the Highly Restricted Down Syndrome Critical Region on 21q22.13: New KCNJ6 and DSCR4 Transcript Isoforms

Author

Francesca Antonaros, Margherita Pitocco, Domenico Abete, Beatrice Vione, Allison Piovesan, Lorenza Vitale, Pierluigi Strippoli, Maria Caracausi, and Maria Chiara Pelleri

Subjects

Down syndrome, trisomy 21 (Down syndrome), HR-DSCR, KCNJ6, DSCR4, RNA isoforms, Genetics, QH426-470

Abstract

Down syndrome (DS) is caused by trisomy of chromosome 21 and it is the most common genetic cause of intellectual disability (ID) in humans. Subjects with DS show a typical phenotype marked by facial dysmorphisms and ID. Partial trisomy 21 (PT21) is a rare genotype characterized by the duplication of a delimited chromosome 21 (Hsa21) portion and it may or may not be associated with DS diagnosis. The highly restricted Down syndrome critical region (HR-DSCR) is a region of Hsa21 present in three copies in all individuals with PT21 and a diagnosis of DS. This region, located on distal 21q22.13, is 34 kbp long and does not include characterized genes. The HR-DSCR is annotated as an intergenic region between KCNJ6-201 transcript encoding for potassium inwardly rectifying channel subfamily J member 6 and DSCR4-201 transcript encoding Down syndrome critical region 4. Two transcripts recently identified by massive RNA-sequencing (RNA-Seq) and automatically annotated on Ensembl database reveal that the HR-DSCR seems to be partially crossed by KCNJ6-202 and DSCR4-202 isoforms. KCNJ6-202 shares the coding sequence with KCNJ6-201 which is involved in many physiological processes, including heart rate in cardiac cells and circuit activity in neuronal cells. DSCR4-202 transcript has the first two exons in common with DSCR4-201, the only experimentally verified gene uniquely present in Hominidae. In this study, we performed in silico and in vitro analyses of the HR-DSCR. Bioinformatic data, obtained using Sequence Read Archive (SRA) and SRA-BLAST software, were confirmed by Reverse Transcription-Polymerase Chain Reaction (RT-PCR) and Sanger sequencing on a panel of human tissues. Our data demonstrate that the HR-DSCR cannot be defined as an intergenic region. Further studies are needed to investigate the functional role of the new transcripts, likely involved in DS phenotypes.

Published

2021

11. Human protein-coding genes and gene feature statistics in 2019

Author

Allison Piovesan, Francesca Antonaros, Lorenza Vitale, Pierluigi Strippoli, Maria Chiara Pelleri, and Maria Caracausi

Subjects

Human genes, Protein-coding genes, Gene statistics, Medicine, Biology (General), QH301-705.5, Science (General), Q1-390

Abstract

Abstract Objective A well-known limit of genome browsers is that the large amount of genome and gene data is not organized in the form of a searchable database, hampering full management of numerical data and free calculations. Due to the continuous increase of data deposited in genomic repositories, their content revision and analysis is recommended. Using GeneBase, a software with a graphical interface able to import and elaborate National Center for Biotechnology Information (NCBI) Gene database entries, we provide tabulated spreadsheets updated to 2019 about human nuclear protein-coding gene data set ready to be used for any type of analysis about genes, transcripts and gene organization. Results Comparison with previous reports reveals substantial change in the number of known nuclear protein-coding genes (now 19,116), the protein-coding non-redundant transcriptome space [now 59,281,518 base pair (bp), 10.1% increase], the number of exons (now 562,164, 36.2% increase) due to a relevant increase of the RNA isoforms recorded. Other parameters such as gene, exon or intron mean and extreme length appear to have reached a stability that is unlikely to be substantially modified by human genome data updates, at least regarding protein-coding genes. Finally, we confirm that there are no human introns shorter than 30 bp.

Published

2019

12. On the length, weight and GC content of the human genome

Author

Allison Piovesan, Maria Chiara Pelleri, Francesca Antonaros, Pierluigi Strippoli, Maria Caracausi, and Lorenza Vitale

Subjects

Human genome, Genome length, Genome weight, GC content, Mitochondrial DNA, Medicine, Biology (General), QH301-705.5, Science (General), Q1-390

Abstract

Abstract Objective Basic parameters commonly used to describe genomes including length, weight and relative guanine-cytosine (GC) content are widely cited in absence of a primary source. By using updated data and original software we determined these values to the best of our knowledge as standard reference for the whole human nuclear genome, for each chromosome and for mitochondrial DNA. We also devised a method to calculate the relative GC content in the whole messenger RNA sequence set and in transcriptomes by multiplying the GC content of each gene by its mean expression level. Results The male nuclear diploid genome extends for 6.27 Gigabase pairs (Gbp), is 205.00 cm (cm) long and weighs 6.41 picograms (pg). Female values are 6.37 Gbp, 208.23 cm, 6.51 pg. The individual variability and the implication for the DNA informational density in terms of bits/volume were discussed. The genomic GC content is 40.9%. Following analysis in different transcriptomes and species, we showed that the greatest deviation was observed in the pathological condition analysed (trisomy 21 leukaemic cells) and in Caenorhabditis elegans. Our results may represent a solid basis for further investigation on human structural and functional genomics while also providing a framework for other genome comparative analysis.

Published

2019

13. A molecular view of the normal human thyroid structure and function reconstructed from its reference transcriptome map

Author

Lorenza Vitale, Allison Piovesan, Francesca Antonaros, Pierluigi Strippoli, Maria Chiara Pelleri, and Maria Caracausi

Subjects

Human thyroid, Gene expression, Integrated transcriptome map, Meta-analysis, Human chromosome 21, Biotechnology, TP248.13-248.65, Genetics, QH426-470

Abstract

Abstract Background The thyroid is the earliest endocrine structure to appear during human development, and thyroid hormones are necessary for proper organism development, in particular for the nervous system and heart, normal growth and skeletal maturation. To date a quantitative, validated transcriptional atlas of the whole normal human thyroid does not exist and the availability of a detailed expression map might be an excellent occasion to investigate the many features of the thyroid transcriptome. Results We present a view at the molecular level of the normal human thyroid histology and physiology obtained by a systematic meta-analysis of all the available gene expression profiles for the whole organ. A quantitative transcriptome reference map was generated by using the TRAM (Transcriptome Mapper) software able to combine, normalize and integrate a total of 35 suitable datasets from different sources thus providing a typical reference expression value for each of the 27,275 known, mapped transcripts obtained. The experimental in vitro validation of data was performed by “Real-Time” reverse transcription polymerase chain reaction showing an excellent correlation coefficient (r = 0.93) with data obtained in silico. Conclusions Our study provides a quantitative global reference portrait of gene expression in the normal human thyroid and highlights differential expression between normal human thyroid and a pool of non-thyroid tissues useful for modeling correlations between thyroidal gene expression and specific thyroid functions and diseases. The experimental in vitro validation supports the possible usefulness of the human thyroid transcriptome map as a reference for molecular studies of the physiology and pathology of this organ.

Published

2017

14. Reference quantitative transcriptome dataset for adult Caenorhabditis elegans

Author

Allison Piovesan, Francesca Antonaros, Pierluigi Strippoli, Lorenza Vitale, Maria Chiara Pelleri, and Maria Caracausi

Subjects

Computer applications to medicine. Medical informatics, R858-859.7, Science (General), Q1-390

Abstract

Caenorhabditis elegans is a nematode widely used in biology and genomics as a model organism. We provide an integrated, quantitative reference map for the transcriptome of whole, wild type Bristol N2 strain C. elegans worms. The map has been obtained by meta-analysis of 110 gene expression profiles available in Gene Expression Omnibus (GEO) repository and integrated using the computational biology tool Transcriptome Mapper (TRAM). Following probe assignment to the relative locus and intra- and inter-sample normalization (in particular using the scaled quantile method), a mean, consensus reference value is provided for 45,932 transcripts, along with standard deviation. Expression values are all mapped in the context of genomic coordinates. The map provides easy access to relationships among expression values of different genes in this standard condition, highlights genomic segments with relatively high over-/under-expression and may serve as a reference to test for gene expression variation for both individual genes and the whole transcriptome in specific biological conditions (e.g. mutated strains or differently grown worms). Keywords: C. elegans, Transcriptome map, Gene expression, Adult worms, Meta-analysis

Published

2019

15. Partial trisomy 21 map: Ten cases further supporting the highly restricted Down syndrome critical region (HR‐DSCR) on human chromosome 21

Author

Maria Chiara Pelleri, Elena Cicchini, Michael B. Petersen, Lisbeth Tranebjærg, Teresa Mattina, Pamela Magini, Francesca Antonaros, Maria Caracausi, Lorenza Vitale, Chiara Locatelli, Marco Seri, Pierluigi Strippoli, Allison Piovesan, and Guido Cocchi

Subjects

computational biology, Down syndrome, highly restricted Down syndrome critical region, human chromosome 21, intellectual disability, partial trisomy 21, Genetics, QH426-470

Abstract

Abstract Background Down syndrome (DS) is characterized by the presence of an extra full or partial human chromosome 21 (Hsa21). An invaluable model to define genotype‐phenotype correlations in DS is the study of the extremely rare cases of partial (segmental) trisomy 21 (PT21), the duplication of only a delimited region of Hsa21 associated or not to DS. A systematic retrospective reanalysis of 125 PT21 cases described up to 2015 allowed the creation of the most comprehensive PT21 map and the identification of a 34‐kb highly restricted DS critical region (HR‐DSCR) as the minimal region whose duplication is shared by all PT21 subjects diagnosed with DS. We reanalyzed at higher resolution three cases previously published and we accurately searched for any new PT21 reports in order to verify whether HR‐DSCR limits could prospectively be confirmed and possibly refined. Methods Hsa21 partial duplications of three PT21 subjects were refined by adding array‐based comparative genomic hybridization data. Seven newly described PT21 cases fulfilling stringent cytogenetic and clinical criteria have been incorporated into the PT21 integrated map. Results The PT21 map now integrates fine structure of Hsa21 sequence intervals of 132 subjects onto a common framework fully consistent with the presence of a duplicated HR‐DSCR, on distal 21q22.13 sub‐band, only in DS subjects and not in non‐DS individuals. No documented exception to the HR‐DSCR model was found. Conclusions The findings presented here further support the association of the HR‐DSCR with the diagnosis of DS, representing an unbiased validation of the original model. Further studies are needed to identify and characterize genetic determinants presumably located in the HR‐DSCR and functionally associated to the critical manifestations of DS.

Published

2019

16. Dataset of differential gene expression between total normal human thyroid and histologically normal thyroid adjacent to papillary thyroid carcinoma

Author

Lorenza Vitale, Allison Piovesan, Francesca Antonaros, Pierluigi Strippoli, Maria Chiara Pelleri, and Maria Caracausi

Subjects

Computer applications to medicine. Medical informatics, R858-859.7, Science (General), Q1-390

Abstract

This article contains further data and information from our published manuscript [1]. We aim to identify significant transcriptome alterations of total normal human thyroid vs. histologically normal thyroid adjacent to papillary thyroid carcinoma. We performed a systematic meta-analysis of all the available gene expression profiles for the whole organ also collecting gene expression data for the normal thyroid adjacent to papillary thyroid carcinoma. A differential quantitative transcriptome reference map was generated by using TRAM (Transcriptome Mapper) software able to combine, normalize and integrate a total of 35 datasets from total normal thyroid and 40 datasets from histologically normal thyroid adjacent to papillary thyroid carcinoma from different sources. This analysis identified genes and genome segments that significantly discriminated the two groups of samples. Differentially expressed genes were grouped and enrichment function analyses were performed identifying the main features of the differentially expressed genes between total normal thyroid and histologically normal thyroid adjacent to papillary thyroid carcinoma. The search for housekeeping genes retrieved 414 loci.

Published

2019

17. Is the Age of Developmental Milestones a Predictor for Future Development in Down Syndrome?

Author

Chiara Locatelli, Sara Onnivello, Francesca Antonaros, Agnese Feliciello, Sonia Filoni, Sara Rossi, Francesca Pulina, Chiara Marcolin, Renzo Vianello, Enrico Toffalini, Giuseppe Ramacieri, Anna Martelli, Giulia Procaccini, Giacomo Sperti, Maria Caracausi, Maria Chiara Pelleri, Lorenza Vitale, Gian Luca Pirazzoli, Pierluigi Strippoli, Guido Cocchi, Allison Piovesan, and Silvia Lanfranchi

Subjects

Down Syndrome, developmental milestones, development, Neurosciences. Biological psychiatry. Neuropsychiatry, RC321-571

Abstract

Down Syndrome (DS) is the most common genetic alteration responsible for intellectual disability, which refers to deficits in both intellectual and adaptive functioning. According to this, individuals with Down Syndrome (DS) reach developmental milestones (e.g., sitting, walking, and babbling) in the same order as their typically developing peers, but later in life. Since developmental milestones are the first blocks on which development builds, the aims of the current study are to: (i) expand the knowledge of developmental milestone acquisition; and (ii) explore the relationship between developmental milestone acquisition and later development. For this purpose 105 children/adolescents with DS were involved in this study, divided in two groups, Preschoolers (n = 39) and School-age participants (n = 66). Information on the age of acquisition of Sitting, Walking, Babbling, and Sphincter Control was collected, together with cognitive, motor, and adaptive functioning. Sitting predicted later motor development, but, with age, it became less important in predicting motor development in everyday life. Babbling predicted later language development in older children. Finally, Sphincter Control emerged as the strongest predictor of motor, cognitive, language, and adaptive skills, with its role being more evident with increasing age. Our data suggest that the age of reaching the milestones considered in the study has an influence on successive development, a role that can be due to common neural substrates, the environment, and the developmental cascade effect.

Published

2021

18. Integrated Quantitative Transcriptome Maps of Human Trisomy 21 Tissues and Cells

Author

Maria Chiara Pelleri, Chiara Cattani, Lorenza Vitale, Francesca Antonaros, Pierluigi Strippoli, Chiara Locatelli, Guido Cocchi, Allison Piovesan, and Maria Caracausi

Subjects

integrated transcriptome map, meta-analysis, human chromosome 21, trisomy 21, Down syndrome, Genetics, QH426-470

Abstract

Down syndrome (DS) is due to the presence of an extra full or partial chromosome 21 (Hsa21). The identification of genes contributing to DS pathogenesis could be the key to any rational therapy of the associated intellectual disability. We aim at generating quantitative transcriptome maps in DS integrating all gene expression profile datasets available for any cell type or tissue, to obtain a complete model of the transcriptome in terms of both expression values for each gene and segmental trend of gene expression along each chromosome. We used the TRAM (Transcriptome Mapper) software for this meta-analysis, comparing transcript expression levels and profiles between DS and normal brain, lymphoblastoid cell lines, blood cells, fibroblasts, thymus and induced pluripotent stem cells, respectively. TRAM combined, normalized, and integrated datasets from different sources and across diverse experimental platforms. The main output was a linear expression value that may be used as a reference for each of up to 37,181 mapped transcripts analyzed, related to both known genes and expression sequence tag (EST) clusters. An independent example in vitro validation of fibroblast transcriptome map data was performed through “Real-Time” reverse transcription polymerase chain reaction showing an excellent correlation coefficient (r = 0.93, p < 0.0001) with data obtained in silico. The availability of linear expression values for each gene allowed the testing of the gene dosage hypothesis of the expected 3:2 DS/normal ratio for Hsa21 as well as other human genes in DS, in addition to listing genes differentially expressed with statistical significance. Although a fraction of Hsa21 genes escapes dosage effects, Hsa21 genes are selectively over-expressed in DS samples compared to genes from other chromosomes, reflecting a decisive role in the pathogenesis of the syndrome. Finally, the analysis of chromosomal segments reveals a high prevalence of Hsa21 over-expressed segments over the other genomic regions, suggesting, in particular, a specific region on Hsa21 that appears to be frequently over-expressed (21q22). Our complete datasets are released as a new framework to investigate transcription in DS for individual genes as well as chromosomal segments in different cell types and tissues.

Published

2018

19. Complexity of bidirectional transcription and alternative splicing at human RCAN3 locus.

Author

Federica Facchin, Lorenza Vitale, Eva Bianconi, Francesco Piva, Flavia Frabetti, Pierluigi Strippoli, Raffaella Casadei, Maria Chiara Pelleri, Allison Piovesan, and Silvia Canaider

Subjects

Medicine, Science

Abstract

Human RCAN3 (regulator of calcineurin 3) belongs to the human RCAN gene family.In this study we provide, with in silico and in vitro analyses, the first detailed description of the human multi-transcript RCAN3 locus. Its analysis revealed that it is composed of a multigene system that includes at least 21 RCAN3 alternative spliced isoforms (16 of them identified here for the first time) and a new RCAN3 antisense gene (RCAN3AS). In particular, we cloned RCAN3-1,3,4,5 (lacking exon 2), RCAN3-1a,2,3,4,5, RCAN3-1a,3,4,5, RCAN3-1b,2,3,4,5, RCAN3-1c,2,3,4,5, RCAN3-1c,2,4,5 and RCAN3-1c,3,4,5, isoforms that present a different 5' untranslated region when compared to RCAN3. Moreover, in order to verify the possible 5' incompleteness of previously identified cDNA isoforms with the reference exon 1, ten more alternative isoforms were retrieved. Bioinformatic searches allowed us to identify RCAN3AS, which overlaps in part with exon 1a, on the opposite strand, for which four different RCAN3AS isoforms were cloned.In order to analyze the different expression patterns of RCAN3 alternative first exons and of RCAN3AS mRNA isoforms, RT-PCR was performed in 17 human tissues. Finally, analyses of RCAN3 and RCAN3AS genomic sequences were performed to identify possible promoter regions, to examine donor and acceptor splice sequences and to compare evolutionary conservation, in particular of alternative exon 1 or 1c--exon 2 junctions in different species.The description of its number of transcripts, of their expression patterns and of their regulatory regions can be important to clarify the functions of RCAN3 gene in different pathways and cellular processes.

Published

2011

20. A reassessment of Jackson's checklist and identification of two Down syndrome sub-phenotypes

Author

Chiara Locatelli, Sara Onnivello, Caterina Gori, Giuseppe Ramacieri, Francesca Pulina, Chiara Marcolin, Renzo Vianello, Beatrice Vione, Maria Caracausi, Maria Chiara Pelleri, Lorenza Vitale, Gian Luca Pirazzoli, Guido Cocchi, Luigi Corvaglia, Pierluigi Strippoli, Francesca Antonaros, Allison Piovesan, Silvia Lanfranchi, Locatelli, Chiara, Onnivello, Sara, Gori, Caterina, Ramacieri, Giuseppe, Pulina, Francesca, Marcolin, Chiara, Vianello, Renzo, Vione, Beatrice, Caracausi, Maria, Pelleri, Maria Chiara, Vitale, Lorenza, Pirazzoli, Gian Luca, Cocchi, Guido, Corvaglia, Luigi, Strippoli, Pierluigi, Antonaros, Francesca, Piovesan, Allison, and Lanfranchi, Silvia

Subjects

Down syndrome phenotype, Multidisciplinary, Jackson's checklist, Phenotype, Neurology, Intellectual Disability, Genetics, Humans, Genetics, Behavioral, Down Syndrome, Checklist, Behavioral

Abstract

Down syndrome (DS) is characterised by several clinical features including intellectual disability (ID) and craniofacial dysmorphisms. In 1976, Jackson and coll. identified a checklist of signs for clinical diagnosis of DS; the utility of these checklists in improving the accuracy of clinical diagnosis has been recently reaffirmed, but they have rarely been revised. The purpose of this work is to reassess the characteristic phenotypic signs and their frequencies in 233 DS subjects, following Jackson's checklist. 63.77% of the subjects showed more than 12 signs while none showed less than 5, confirming the effectiveness of Jackson's checklist for the clinical diagnosis of DS. An association between three phenotypic signs emerged, allowing us to distinguish two sub-phenotypes: Brachycephaly, short and broad Hands, short Neck (BHN), which is more frequent, and "non-BHN". The strong association of these signs might be interpreted in the context of the growth defects observed in DS children suggesting decreased cell proliferation. Lastly, cognitive assessments were investigated for 114 subjects. The lack of association between the presence of a physical sign or the number of signs present in a subject and cognitive skills disproves the stereotype that physical characteristics are predictive of degree of ID.

Published

2021

21. The transcriptome profile of human trisomy 21 blood cells

Author

Allison Piovesan, Chiara Locatelli, Francesca Catapano, Pierluigi Strippoli, Rossella Zenatelli, Giulia Guerri, Lorenza Vitale, Maria Chiara Pelleri, Guido Cocchi, Beatrice Vione, Alice Gori, Giuseppe Ramacieri, Maria Caracausi, Francesca Antonaros, Matteo Bertelli, Antonaros F., Zenatelli R., Guerri G., Bertelli M., Locatelli C., Vione B., Catapano F., Gori A., Vitale L., Pelleri M.C., Ramacieri G., Cocchi G., Strippoli P., Caracausi M., and Piovesan A.

Subjects

Myxovirus Resistance Proteins, 0301 basic medicine, Blood cells, Trisomy 21, Chromosomes, Human, Pair 21, Mitochondrial translation, Down syndrome, Human chromosome 21, QH426-470, Biology, Genome, Transcriptome, Reduced Folate Carrier Protein, 03 medical and health sciences, 0302 clinical medicine, Intellectual Disability, Drug Discovery, Gene expression, Genetics, Humans, Carbon-Nitrogen Ligases, RNA-Seq, Molecular Biology, Gene, Phosphoribosylglycinamide Formyltransferase, Genome, Human, Blood cell, RNA sequencing, Phenotype, Mitochondria, Reverse transcription polymerase chain reaction, 030104 developmental biology, Gene Expression Regulation, Medicine, Molecular Medicine, Energy Metabolism, Primary Research, Chromosome 21, Software, 030217 neurology & neurosurgery

Abstract

Background Trisomy 21 (T21) is a genetic alteration characterised by the presence of an extra full or partial human chromosome 21 (Hsa21) leading to Down syndrome (DS), the most common form of intellectual disability (ID). It is broadly agreed that the presence of extra genetic material in T21 gives origin to an altered expression of genes located on Hsa21 leading to DS phenotype. The aim of this study was to analyse T21 and normal control blood cell gene expression profiles obtained by total RNA sequencing (RNA-Seq). Results The results were elaborated by the TRAM (Transcriptome Mapper) software which generated a differential transcriptome map between human T21 and normal control blood cells providing the gene expression ratios for 17,867 loci. The obtained gene expression profiles were validated through real-time reverse transcription polymerase chain reaction (RT-PCR) assay and compared with previously published data. A post-analysis through transcriptome mapping allowed the identification of the segmental (regional) variation of the expression level across the whole genome (segment-based analysis of expression). Interestingly, the most over-expressed genes encode for interferon-induced proteins, two of them (MX1 and MX2 genes) mapping on Hsa21 (21q22.3). The altered expression of genes involved in mitochondrial translation and energy production also emerged, followed by the altered expression of genes encoding for the folate cycle enzyme, GART, and the folate transporter, SLC19A1. Conclusions The alteration of these pathways might be linked and involved in the manifestation of ID in DS.

Published

2021

22. GeneRecords: a relational database for GenBank flat file parsing and data manipulation in personal computers.

Author

Pietro D'Addabbo, Luca Lenzi, Federica Facchin, Raffaella Casadei, Silvia Canaider, Lorenza Vitale, Flavia Frabetti, Paolo Carinci, Maria Zannotti, and Pierluigi Strippoli

Published

2004

23. Is the Age of Developmental Milestones a Predictor for Future Development in Down Syndrome?

Author

Allison Piovesan, Silvia Lanfranchi, Chiara Marcolin, Gian Luca Pirazzoli, Francesca Pulina, Maria Chiara Pelleri, Chiara Locatelli, Giacomo Sperti, Sara Rossi, Giuseppe Ramacieri, Agnese Feliciello, Giulia Procaccini, Anna Martelli, Maria Caracausi, Renzo Vianello, Sonia Filoni, Lorenza Vitale, Guido Cocchi, Enrico Toffalini, Francesca Antonaros, Sara Onnivello, Pierluigi Strippoli, Locatelli C., Onnivello S., Antonaros F., Feliciello A., Filoni S., Rossi S., Pulina F., Marcolin C., Vianello R., Toffalini E., Ramacieri G., Martelli A., Procaccini G., Sperti G., Caracausi M., Pelleri M.C., Vitale L., Pirazzoli G.L., Strippoli P., Cocchi G., Piovesan A., and Lanfranchi S.

Subjects

Down syndrome, Neurosciences. Biological psychiatry. Neuropsychiatry, Babbling, Article, Developmental psychology, 03 medical and health sciences, 0302 clinical medicine, Developmental milestone, Intellectual disability, medicine, 0501 psychology and cognitive sciences, development, Motor skill, General Neuroscience, 05 social sciences, Down syndrome, milestones, development, Cognition, medicine.disease, Down Syndrome, developmental milestones, Language development, Age of Acquisition, Developmental Milestone, milestones, Psychology, 030217 neurology & neurosurgery, RC321-571, 050104 developmental & child psychology

Abstract

Down Syndrome (DS) is the most common genetic alteration responsible for intellectual disability, which refers to deficits in both intellectual and adaptive functioning. According to this, individuals with Down Syndrome (DS) reach developmental milestones (e.g., sitting, walking, and babbling) in the same order as their typically developing peers, but later in life. Since developmental milestones are the first blocks on which development builds, the aims of the current study are to: (i) expand the knowledge of developmental milestone acquisition; and (ii) explore the relationship between developmental milestone acquisition and later development. For this purpose 105 children/adolescents with DS were involved in this study, divided in two groups, Preschoolers (n = 39) and School-age participants (n = 66). Information on the age of acquisition of Sitting, Walking, Babbling, and Sphincter Control was collected, together with cognitive, motor, and adaptive functioning. Sitting predicted later motor development, but, with age, it became less important in predicting motor development in everyday life. Babbling predicted later language development in older children. Finally, Sphincter Control emerged as the strongest predictor of motor, cognitive, language, and adaptive skills, with its role being more evident with increasing age. Our data suggest that the age of reaching the milestones considered in the study has an influence on successive development, a role that can be due to common neural substrates, the environment, and the developmental cascade effect.

Published

2021

24. One-carbon pathway and cognitive skills in children with Down syndrome

Author

Renzo Vianello, Francesca Pulina, Silvia Lanfranchi, Ludovica Carosi Diatricch, Elena Cicchini, Elisa Mannini, Giuseppe Ramacieri, Maria Caracausi, Chiara Locatelli, Lorenza Vitale, Guido Cocchi, Pierluigi Strippoli, Sara Onnivello, Allison Piovesan, Anna Martelli, Giulia Olivucci, Maria Chiara Pelleri, Agnese Feliciello, Beatrice Vione, Francesca Antonaros, Antonaros, Francesca, Lanfranchi, Silvia, Locatelli, Chiara, Martelli, Anna, Olivucci, Giulia, Cicchini, Elena, Carosi Diatricch, Ludovica, Mannini, Elisa, Vione, Beatrice, Feliciello, Agnese, Ramacieri, Giuseppe, Onnivello, Sara, Vianello, Renzo, Vitale, Lorenza, Pelleri, Maria Chiara, Strippoli, Pierluigi, Cocchi, Guido, Pulina, Francesca, Piovesan, Allison, and Caracausi, Maria

Subjects

Male, Down syndrome, medicine.medical_specialty, Homocysteine, Science, Metabolite, Article, Correlation, chemistry.chemical_compound, Medical research, Cognition, MTHFR C677T genotype, folate cycle, Homocysteine plasma level, WPPSI-III test, Griffiths-III test, Down syndrome, Internal medicine, medicine, Genetics, Humans, Vitamin B12, Child, Methylenetetrahydrofolate Reductase (NADPH2), Creatinine, Multidisciplinary, business.industry, Fasting, medicine.disease, Carbon, Cognitive test, Endocrinology, chemistry, Medicine, Uric acid, Female, Down Syndrome, business, Energy Metabolism, metabolism, Biomarkers, Metabolic Networks and Pathways, Down syndrome, metabolism, cognitive development, cognitive development, Neuroscience

Abstract

This work investigates the role of metabolite levels in the intellectual impairment of subjects with Down syndrome (DS). Homocysteine, folate, vitamin B12, uric acid (UA), creatinine levels and MTHFR C677T genotype were analyzed in 147 subjects with DS. For 77 subjects, metabolite levels were correlated with cognitive tests. Griffiths-III test was administered to 28 subjects (3.08–6.16 years) and WPPSI-III test was administered to 49 subjects (7.08–16.08 years). Significant correlations were found among some metabolite levels and between homocysteine levels and MTHFR C677T genotype. Moreover, homocysteine, UA and creatinine levels resulted increased with age. We did not find any correlation between metabolites and cognitive test score in the younger group. Homocysteine showed statistically significant correlation with WPPSI-III subtest scores when its level is ≥ 7.35 µmol/L, remaining correlated in higher thresholds only for non-verbal area scores. Vitamin B12 showed correlations with all WPPSI-III subtest scores when its level is

Published

2021

25. Plasma metabolome and cognitive skills in Down syndrome

Author

Pierluigi Strippoli, Elisa Mannini, Francesca Pulina, Maria Chiara Pelleri, Allison Piovesan, Renzo Vianello, Chiara Locatelli, Silvia Lanfranchi, Francesca Antonaros, Paola Turano, Anna Martelli, Sara Onnivello, Claudio Luchinat, Lorenza Vitale, Guido Cocchi, Agnese Feliciello, Veronica Ghini, Giuseppe Ramacieri, Elena Cicchini, Maria Caracausi, and Antonaros F, Ghini V, Pulina F, Ramacieri G, Cicchini E, Mannini E, Martelli A, Feliciello A, Lanfranchi S, Onnivello S, Vianello R, Locatelli C, Cocchi G, Pelleri MC, Vitale L, Strippoli P, Luchinat C, Turano P, Piovesan A, Caracausi M

Subjects

Adult, Male, Metabolism, cognitive skills, Down syndrome, Down syndrome, medicine.medical_specialty, Magnetic Resonance Spectroscopy, Adolescent, Metabolite, lcsh:Medicine, Trisomy, Biochemistry, Article, chemistry.chemical_compound, Plasma, Young Adult, cognitive skills, Metabolomics, Cognition, Internal medicine, Intellectual Disability, medicine, Metabolome, Humans, Child, lcsh:Science, Univariate analysis, Multidisciplinary, Intelligence quotient, Medical genetics, Neurodevelopmental disorders, lcsh:R, Case-control study, Genomics, medicine.disease, Mitochondria, Chemistry, Metabolism, Endocrinology, chemistry, Case-Control Studies, Child, Preschool, Multivariate Analysis, Female, lcsh:Q, Down Syndrome, Metabolomics, Genomics, Medical genetics, Neurodevelopmental disorders, Biochemistry, Chemistry

Abstract

Trisomy 21 (Down syndrome, DS) is the main human genetic cause of intellectual disability (ID). Lejeune hypothesized that DS could be considered a metabolic disease, and we found that subjects with DS have a specific plasma and urinary metabolomic profile. In this work we confirmed the alteration of mitochondrial metabolism in DS and also investigated if metabolite levels are related to cognitive aspects of DS. We analyzed the metabolomic profiles of plasma samples from 129 subjects with DS and 46 healthy control (CTRL) subjects by 1H Nuclear Magnetic Resonance (NMR). Multivariate analysis of the NMR metabolomic profiles showed a clear discrimination (up to 94% accuracy) between the two groups. The univariate analysis revealed a significant alteration in 7 metabolites out of 28 assigned unambiguously. Correlations among the metabolite levels in DS and CTRL groups were separately investigated and statistically significant relationships appeared. On the contrary, statistically significant correlations among the NMR-detectable part of DS plasma metabolome and the different intelligence quotient ranges obtained by Griffiths-III or WPPSI-III tests were not found. Even if metabolic imbalance provides a clear discrimination between DS and CTRL groups, it appears that the investigated metabolomic profiles cannot be associated with the degree of ID.

Published

2020

26. Genotype-phenotype correlation for congenital heart disease in Down syndrome through analysis of partial trisomy 21 cases

Author

Chiara Locatelli, Elena Gennari, Allison Piovesan, Maria Chiara Pelleri, Marco Seri, Costanza Maria Donati, Alessandro Rocca, Pierluigi Strippoli, Francesca Antonaros, Lorenza Vitale, Guido Cocchi, Letizia Conti, Maria Caracausi, Pelleri, Maria Chiara, Gennari, Elena, Locatelli, Chiara, Piovesan, Allison, Caracausi, Maria, Antonaros, Francesca, Rocca, Alessandro, Donati, Costanza Maria, Conti, Letizia, Strippoli, Pierluigi, Seri, Marco, Vitale, Lorenza, and Cocchi, Guido

Subjects

Heart Defects, Congenital, 0301 basic medicine, Down syndrome, Heart disease, Chromosomes, Human, Pair 21, Human chromosome 21, Pregnancy Proteins, Biology, Bioinformatics, Pathogenesis, Correlation, 03 medical and health sciences, DSCAM, Genetics, medicine, Aspartic Acid Endopeptidases, Humans, Genetic Predisposition to Disease, cardiovascular diseases, Genetic Association Studies, Congenital heart disease, Partial Trisomy, Chromosome Mapping, Partial trisomy 21, medicine.disease, 030104 developmental biology, RNA, Long Noncoding, Amyloid Precursor Protein Secretases, Trisomy, Chromosome 21, Cell Adhesion Molecules

Abstract

Among Down syndrome (DS) children, 40-50% have congenital heart disease (CHD). Although trisomy 21 is not sufficient to cause CHD, three copies of at least part of chromosome 21 (Hsa21) increases the risk for CHD. In order to establish a genotype-phenotype correlation for CHD in DS, we built an integrated Hsa21 map of all described partial trisomy 21 (PT21) cases with sufficient indications regarding presence or absence of CHD (n=107), focusing on DS PT21 cases. We suggest a DS CHD candidate region on 21q22.2 (0.96Mb), being shared by most PT21 cases with CHD and containing three known protein-coding genes (DSCAM, BACE2, PLAC4) and four known non-coding RNAs (DSCAM-AS1, DSCAM-IT1, LINC00323, MIR3197). The characterization of a DS CHD candidate region provides a useful approach to identify specific genes contributing to the pathology and to orient further investigations and possibly more effective therapy in relation to the multifactorial pathogenesis of CHD.

Published

2017

27. Dataset of differential gene expression between total normal human thyroid and histologically normal thyroid adjacent to papillary thyroid carcinoma

Author

Allison Piovesan, Maria Caracausi, Francesca Antonaros, Maria Chiara Pelleri, Lorenza Vitale, Pierluigi Strippoli, Vitale L., Piovesan A., Antonaros F., Strippoli P., Pelleri M.C., and Caracausi M.

Subjects

Pathology, medicine.medical_specialty, endocrine system, endocrine system diseases, Biology, lcsh:Computer applications to medicine. Medical informatics, Genome, Thyroid carcinoma, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, Human thyroid, Gene expression, medicine, Meta-analysi, lcsh:Science (General), Gene, 030304 developmental biology, 0303 health sciences, Genetics, Genomics and Molecular Biology, Multidisciplinary, Integrated transcriptome map, Normal thyroid, Housekeeping gene, lcsh:R858-859.7, Histologically normal thyroid adjacent to papillary thyroid carcinoma, 030217 neurology & neurosurgery, lcsh:Q1-390

Abstract

This article contains further data and information from our published manuscript [1]. We aim to identify significant transcriptome alterations of total normal human thyroid vs. histologically normal thyroid adjacent to papillary thyroid carcinoma. We performed a systematic meta-analysis of all the available gene expression profiles for the whole organ also collecting gene expression data for the normal thyroid adjacent to papillary thyroid carcinoma. A differential quantitative transcriptome reference map was generated by using TRAM (Transcriptome Mapper) software able to combine, normalize and integrate a total of 35 datasets from total normal thyroid and 40 datasets from histologically normal thyroid adjacent to papillary thyroid carcinoma from different sources. This analysis identified genes and genome segments that significantly discriminated the two groups of samples. Differentially expressed genes were grouped and enrichment function analyses were performed identifying the main features of the differentially expressed genes between total normal thyroid and histologically normal thyroid adjacent to papillary thyroid carcinoma. The search for housekeeping genes retrieved 414 loci.

Published

2019

28. Human protein-coding genes and gene feature statistics in 2019

Author

Francesca Antonaros, Maria Chiara Pelleri, Lorenza Vitale, Maria Caracausi, Pierluigi Strippoli, Allison Piovesan, Piovesan A., Antonaros F., Vitale L., Strippoli P., Pelleri M.C., and Caracausi M.

Subjects

0301 basic medicine, Base pair, lcsh:Medicine, Computational biology, Biology, Genome, General Biochemistry, Genetics and Molecular Biology, Transcriptome, 03 medical and health sciences, Exon, Open Reading Frames, 0302 clinical medicine, RNA Isoforms, Databases, Genetic, Gene statistic, Humans, 030212 general & internal medicine, lcsh:Science (General), Gene, lcsh:QH301-705.5, Genome, Human, Protein-coding genes, Gene statistics, lcsh:R, Intron, Computational Biology, Nuclear Proteins, General Medicine, Exons, Introns, Human genes, Research Note, 030104 developmental biology, lcsh:Biology (General), Gene Expression Regulation, Human genome, Human gene, Software, lcsh:Q1-390

Abstract

Objective A well-known limit of genome browsers is that the large amount of genome and gene data is not organized in the form of a searchable database, hampering full management of numerical data and free calculations. Due to the continuous increase of data deposited in genomic repositories, their content revision and analysis is recommended. Using GeneBase, a software with a graphical interface able to import and elaborate National Center for Biotechnology Information (NCBI) Gene database entries, we provide tabulated spreadsheets updated to 2019 about human nuclear protein-coding gene data set ready to be used for any type of analysis about genes, transcripts and gene organization. Results Comparison with previous reports reveals substantial change in the number of known nuclear protein-coding genes (now 19,116), the protein-coding non-redundant transcriptome space [now 59,281,518 base pair (bp), 10.1% increase], the number of exons (now 562,164, 36.2% increase) due to a relevant increase of the RNA isoforms recorded. Other parameters such as gene, exon or intron mean and extreme length appear to have reached a stability that is unlikely to be substantially modified by human genome data updates, at least regarding protein-coding genes. Finally, we confirm that there are no human introns shorter than 30 bp.

Published

2019

29. On the length, weight and GC content of the human genome

Author

Maria Chiara Pelleri, Maria Caracausi, Francesca Antonaros, Allison Piovesan, Lorenza Vitale, Pierluigi Strippoli, Piovesan A., Pelleri M.C., Antonaros F., Strippoli P., Caracausi M., and Vitale L.

Subjects

0301 basic medicine, Male, Mitochondrial DNA, Nuclear gene, lcsh:Medicine, Genomics, Computational biology, Biology, Genome, DNA, Mitochondrial, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, 0302 clinical medicine, Humans, 030212 general & internal medicine, lcsh:Science (General), lcsh:QH301-705.5, Gene, GC content, Base Composition, Genome weight, Human genome, Genome, Human, lcsh:R, Chromosome, General Medicine, Research Note, 030104 developmental biology, lcsh:Biology (General), Female, GC-content, Genome length, lcsh:Q1-390, Human

Abstract

Objective Basic parameters commonly used to describe genomes including length, weight and relative guanine-cytosine (GC) content are widely cited in absence of a primary source. By using updated data and original software we determined these values to the best of our knowledge as standard reference for the whole human nuclear genome, for each chromosome and for mitochondrial DNA. We also devised a method to calculate the relative GC content in the whole messenger RNA sequence set and in transcriptomes by multiplying the GC content of each gene by its mean expression level. Results The male nuclear diploid genome extends for 6.27 Gigabase pairs (Gbp), is 205.00 cm (cm) long and weighs 6.41 picograms (pg). Female values are 6.37 Gbp, 208.23 cm, 6.51 pg. The individual variability and the implication for the DNA informational density in terms of bits/volume were discussed. The genomic GC content is 40.9%. Following analysis in different transcriptomes and species, we showed that the greatest deviation was observed in the pathological condition analysed (trisomy 21 leukaemic cells) and in Caenorhabditis elegans. Our results may represent a solid basis for further investigation on human structural and functional genomics while also providing a framework for other genome comparative analysis. Electronic supplementary material The online version of this article (10.1186/s13104-019-4137-z) contains supplementary material, which is available to authorized users.

Published

2019

30. MTHFR C677T polymorphism analysis: A simple, effective restriction enzyme-based method improving previous protocols

Author

Maria Chiara Pelleri, Elena Cicchini, Allison Piovesan, Lorenza Vitale, Guido Cocchi, Giulia Olivucci, Francesca Antonaros, Chiara Locatelli, Giuseppe Ramacieri, Maria Caracausi, Pierluigi Strippoli, Antonaros F., Olivucci G., Cicchini E., Ramacieri G., Pelleri M.C., Vitale L., Strippoli P., Locatelli C., Cocchi G., Piovesan A., and Caracausi M.

Subjects

0301 basic medicine, new primer pair, Computer science, Base pair, PCR‐RFLP, Single-nucleotide polymorphism, Computational biology, 030105 genetics & heredity, MTHFR C677T, Polymorphism, Single Nucleotide, 03 medical and health sciences, PCR-RFLP, Biological specificity, Polymorphism (computer science), single nucleotide polymorphism, Genetics, Humans, Amplified Fragment Length Polymorphism Analysis, Molecular Biology, Genotyping, Genetics (clinical), Methylenetetrahydrofolate Reductase (NADPH2), Restriction Fragment Length Polymorphism Analysi, biology, Original Articles, Restriction enzyme, 030104 developmental biology, risk factor, Methylenetetrahydrofolate reductase, biology.protein, Methylenetetrahydrofolate Reductase (MTHFR), Original Article, Primer (molecular biology), Genome-Wide Association Study, Human

Abstract

Background: 5,10-Methylentetrahydrofolate reductase (MTHFR) C677T polymorphism is one of the most studied genetic variations in the human genome. Polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) is one of the most used techniques to characterize the point mutations in genomic sequences because of its suitability and low cost. The most widely used method for the MTHFR C677T polymorphism characterization was developed by Frosst et al. (1995) but appears to have some technical limitations. The aim of this study was to propose a novel PCR-RFLP method for the detection of this polymorphism. Methods: In order to retrieve all published articles possibly describing any PCR-RFLP methods useful to analyze MTHFR C677T polymorphism, we performed systematic queries on PubMed, using a combination of Boolean operators (AND/OR) and MeSH terms. Amplify software was used in order to design a new primer pair following the optimal standard criteria. Primer-BLAST software was used to check primer pair's biological specificity. Results: The analysis of previous literature showed that PCR-RFLP method remains the most used technique. None of the 108 primer pairs described was ideal with regard to main accepted primer pair biochemical technical parameters. The new primer pair amplifies a DNA-fragment of 513 base pair (bp) that, in the presence of the polymorphism, is cut by HinfI enzyme in two pieces of 146bp and 367bp and clearly visible on 2% agarose gel. The level of expertise and the materials required are minimal and the protocol takes one day to carry out. Conclusion: Our original PCR-RFLP strategy, specifically designed to make the analysis optimal with respect to PCR primers and gel analysis, fits the ideal criteria compared to the widely used strategy by Frosst et al (1995) as well as any other PCR-RFLP strategies proposed for MTHFR C677T polymorphism genotyping to date.

Published

2019

31. Genetics and genomics of Down syndrome

Author

Maria Chiara Pelleri, Maria Caracausi, Pierluigi Strippoli, Francesca Antonaros, Allison Piovesan, and Lorenza Vitale

Subjects

Genetics, Down syndrome, Intellectual disability, medicine, Genomics, Biology, medicine.disease, Chromosome 21, Trisomy, Gene, Phenotype, Human genetics

Abstract

Down Syndrome (DS) is the most frequent form of intellectual disability (ID) of genetic origin, whose main features include craniofacial dysmorphisms and cardiovascular defects. In 1959, Lejeune and coll. described an extra copy of chromosome 21 (Hsa21) in children with DS (trisomy 21, or T21). We first review how different biological mechanisms may lead to the gain of genetic material of Hsa21 in the cells, originating from different combinations of genetic conditions, including a free or translocated extra copy of Hsa21, distributed in all cells or only in a part of them (mosaicism), with a complete or partial representation of the Hsa21 long arm (21q). Although it is broadly agreed that the DS phenotype originates from the altered expression of the genes located on Hsa21, its molecular pathogenesis is still unknown. We therefore illustrate how recent genomic science may be useful in the elucidation of the genotype-phenotype relationship in DS.

Published

2019

32. UniGene Tabulator: a full parser for the UniGene format.

Author

Luca Lenzi, Flavia Frabetti, Federica Facchin, Raffaella Casadei, Lorenza Vitale, Silvia Canaider, Paolo Carinci, Maria Zannotti, and Pierluigi Strippoli

Published

2006

33. Characterization of human gene locus CYYR1: a complex multi-transcript system

Author

Silvia Canaider, Francesco Piva, Allison Piovesan, Federica Facchin, Elisa Mariani, Flavia Frabetti, Matteo Vian, Raffaella Casadei, Eva Bianconi, Maria Chiara Pelleri, Pierluigi Strippoli, Lorenza Vitale, Raffaella Casadei, Maria Chiara Pelleri, Lorenza Vitale, Federica Facchin, Silvia Canaider, Pierluigi Strippoli, Matteo Vian, Allison Piovesan, Eva Bianconi, Elisa Mariani, Francesco Piva, and Flavia Frabetti

Subjects

Gene isoform, cyyr1, Molecular Sequence Data, Gene Expression, Human chromosome 21, Locus (genetics), Biology, Splicing, Trisomy 21 (Down syndrome), Exon, Gene expression, Genetics, Humans, Protein Isoforms, Coding region, Computer Simulation, Amino Acid Sequence, Molecular Biology, Gene, Tumour cell lines, Alternative splicing, Membrane Proteins, Exons, General Medicine, Multi-transcript locu, Molecular biology, Antisense RNA, Alternative Splicing, Genes, Genetic Loci, Organ Specificity

Abstract

Cysteine/tyrosine-rich 1 (CYYR1) is a gene we previously identified on human chromosome 21 starting from an in-depth bioinformatics analysis of chromosome 21 segment 40/105 (21q21.3), where no coding region had previously been predicted. CYYR1 was initially characterized as a four-exon gene, whose brain-derived cDNA sequencing predicts a 154-amino acid product. In this study we provide, with in silico and in vitro analyses, the first detailed description of the human CYYR1 locus. The analysis of this locus revealed that it is composed of a multi-transcript system, which includes at least seven CYYR1 alternative spliced isoforms and a new CYYR1 antisense gene (named CYYR1-AS1). In particular, we cloned, for the first time, the following isoforms: CYYR1-1,2,3,4b and CYYR1-1,2,3b, which present a different 3' transcribed region, with a consequent different carboxy-terminus of the predicted proteins; CYYR1-1,2,4 lacks exon 3; CYYR1-1,2,2bis,3,4 presents an additional exon between exon 2 and exon 3; CYYR1-1b,2,3,4 presents a different 5' untranslated region when compared to CYYR1. The complexity of the locus is enriched by the presence of an antisense transcript. We have cloned a long transcript overlapping with CYYR1 as an antisense RNA, probably a non-coding RNA. Expression analysis performed in different normal tissues, tumour cell lines as well as in trisomy 21 and euploid fibroblasts has confirmed a quantitative and qualitative variability in the expression pattern of the multi-transcript locus, suggesting a possible role in complex diseases that should be further investigated.

Published

2014

34. Improving mRNA 5′ coding sequence determination in the mouse genome

Author

Allison Piovesan, Lorenza Vitale, Raffaella Casadei, Maria Chiara Pelleri, Pierluigi Strippoli, Annalisa Gurioli, Chiara Bassani, Maria Caracausi, Giulia Soldà, Silvia Martini, Allison Piovesan, Maria Caracausi, Maria Chiara Pelleri, Lorenza Vitale, Silvia Martini, Chiara Bassani, Annalisa Gurioli, Raffaella Casadei, Giulia Soldà, and Pierluigi Strippoli

Subjects

5' Flanking Region, Sequence analysis, Molecular Sequence Data, expressed sequence tag, mouse genome, Biology, Genome, Mice, Open Reading Frames, Start codon, Databases, Genetic, Genetics, 5' coding sequence, Animals, Coding region, RNA, Messenger, Cloning, Molecular, Gene, Sequence (medicine), Expressed sequence tag, Base Sequence, messenger RNA, Computational Biology, Sequence Analysis, DNA, Stop codon, start codon

Abstract

The incomplete determination of the mRNA 5' end sequence may lead to the incorrect assignment of the first AUG codon and to errors in the prediction of the encoded protein product. Due to the significance of the mouse as a model organism in biomedical research, we performed a systematic identification of coding regions at the 5' end of all known mouse mRNAs, using an automated expressed sequence tag (EST)-based approach which we have previously described. By parsing almost 4 million BLAT alignments we found 351 mouse loci, out of 20,221 analyzed, in which an extension of the mRNA 5' coding region was identified. Proof-of-concept confirmation was obtained by in vitro cloning and sequencing for Apc2 and Mknk2 cDNAs. We also generated a list of 16,330 mouse mRNAs where the presence of an in-frame stop codon upstream of the known start codon indicates completeness of the coding sequence at 5' end in the current form. Systematic searches in the main mouse genome databases and genome browsers showed that 82 % of our results are original and have not been identified by their annotation pipelines. Moreover, the same information is not easily derivable from RNA-Seq data, due to short sequence length and laboriousness in building full-length transcript structures. In conclusion, our results improve the determination of full-length 5' coding sequences and might be useful in order to reduce errors when studying mouse gene structure and function in biomedical research.

Published

2014

35. Human trisomy 21 fibroblasts rescue methotrexate toxic effect after treatment with 5-methyl-tetrahydrofolate and 5-formyl-tetrahydrofolate

Author

Valentina Serpieri, Lorenza Vitale, Guido Cocchi, Allison Piovesan, Francesca Antonaros, Mattia Lauriola, Chiara Locatelli, Pierluigi Strippoli, Elena Cicchini, Maria Caracausi, Vitale, Lorenza, Serpieri, Valentina, Lauriola, Mattia, Piovesan, Allison, Antonaros, Francesca, Cicchini, Elena, Locatelli, Chiara, Cocchi, Guido, Strippoli, Pierluigi, and Caracausi, Maria

Subjects

0301 basic medicine, Down syndrome, Physiology, Clinical Biochemistry, Pharmacology, folate, fibroblast, methotrexate, 03 medical and health sciences, 0302 clinical medicine, Dihydrofolate reductase, Medicine, Fibroblast, chemistry.chemical_classification, biology, business.industry, Cell Biology, medicine.disease, one-carbon metabolism, trisomy 21, 030104 developmental biology, Enzyme, medicine.anatomical_structure, chemistry, Cell culture, 030220 oncology & carcinogenesis, Toxicity, biology.protein, Methotrexate, business, Trisomy, medicine.drug

Abstract

Trisomy 21 causes Down syndrome (DS), the most common human genetic disorder and the leading genetic cause of intellectual disability. The alteration of one-carbon metabolism was described as the possible metabolic cause of the intellectual disability development in subjects with DS. One of the biochemical pathways involved in the one-carbon group transfer is the folate cycle. The cytotoxic drug methotrexate (MTX) is a folic acid (FA) analogue which inhibits the activity of dihydrofolate reductase enzyme involved in the one-carbon metabolic cycle. Trisomy 21 cells are more sensitive to the MTX effect than euploid cells, and in 1986 Jerome Lejeune and Coll. demonstrated that MTX was twice as toxic in trisomy 21 lymphocytes than in control cells. In the present work, the rescue effect on MTX toxicity mediated by FA and some of its derivatives, tetrahydrofolate (THF), 5-formyl-THF, and 5-methyl-THF, in both normal and trisomy 21 skin fibroblast cells, was evaluated. A statistically significant rescue effect was obtained by 5-formyl-THF, 5-methyl-THF, and their combination, administered together with MTX. In conclusion, trisomy 21 fibroblast cell lines showed a good response to the rescue effects of 5-formyl-THF and 5-methyl-THF on the MTX toxicity almost as normal cell lines.

Published

2018

36. LGALS4, CEACAM6, TSPAN8, and COL1A2: Blood Markers for Colorectal Cancer-Validation in a Cohort of Subjects With Positive Fecal Immunochemical Test Result

Author

Giampaolo Ugolini, Luigi Ricciardiello, Rossella Solmi, Rossella Miglio, Elena Nardi, Maria Teresa Rodia, Mattia Lauriola, Gabriella Mattei, Francesco Pasini, Pierluigi Strippoli, Rodia, Maria Teresa, Solmi, Rossella, Pasini, Francesco, Nardi, Elena, Mattei, Gabriella, Ugolini, Giampaolo, Ricciardiello, Luigi, Strippoli, Pierluigi, Miglio, Rossella, and Lauriola, Mattia

Subjects

0301 basic medicine, Male, Colorectal cancer, Tetraspanins, Galectin 4, Colonoscopy, Gastroenterology, Feces, Fecal occult blood test, 0302 clinical medicine, Mass Screening, Early Detection of Cancer, medicine.diagnostic_test, Middle Aged, Immunohistochemistry, 3. Good health, CRC, Reverse transcription polymerase chain reaction, Oncology, 030220 oncology & carcinogenesis, Area Under Curve, Cohort, Female, Colorectal Neoplasms, medicine.medical_specialty, GPI-Linked Proteins, Real-Time Polymerase Chain Reaction, Sensitivity and Specificity, Collagen Type I, 03 medical and health sciences, Antigens, CD, Internal medicine, medicine, Biomarkers, Tumor, Blood test, Humans, RNA, Messenger, Liquid biopsy, Aged, Receiver operating characteristic, business.industry, TSPAN8, medicine.disease, FIT, 030104 developmental biology, ROC Curve, business, Cell Adhesion Molecules

Abstract

Background A noninvasive blood test for the early detection of colorectal cancer (CRC) is highly required. We evaluated a panel of 4 mRNAs as putative markers of CRC. Materials and Methods We tested LGALS4, CEACAM6, TSPAN8, and COL1A2, referred to as the CELTiC panel, using quantitative reverse transcription polymerase chain reaction, on subjects with positive fecal immunochemical test (FIT) results and undergoing colonoscopy. Using a nonparametric test and multinomial logistic model, FIT-positive subjects were compared with CRC patients and healthy individuals. Results All the genes of the CELTiC panel displayed statistically significant differences between the healthy subjects (n = 67), both low-risk (n = 36) and high-risk/CRC (n = 92) subjects, and those in the negative-colonoscopy, FIT-positive group (n = 36). The multinomial logistic model revealed LGALS4 was the most powerful marker discriminating the 4 groups. When assessing the diagnostic values by analysis of the areas under the receiver operating characteristic curves (AUCs), the CELTiC panel reached an AUC of 0.91 (sensitivity, 79%; specificity, 94%) comparing normal subjects to low-risk subjects, and 0.88 (sensitivity, 75%; specificity, 87%) comparing normal and high-risk/CRC subjects. The comparison between the normal subjects and the negative-colonoscopy, FIT-positive group revealed an AUC of 0.93 (sensitivity, 82%; specificity, 97%). Conclusion The CELTiC panel could represent a useful tool for discriminating subjects with positive FIT findings and for the early detection of precancerous adenomatous lesions and CRC.

Published

2018

37. A quantitative transcriptome reference map of the normal human hippocampus

Author

Pierluigi Strippoli, Lorenza Vitale, Maria Chiara Pelleri, Maria Caracausi, Vania Rigon, and Allison Piovesan

Subjects

0301 basic medicine, Expressed sequence tag, Cognitive Neuroscience, In silico, Computational biology, Biology, Housekeeping gene, Transcriptome, 03 medical and health sciences, 030104 developmental biology, Gene expression, Microarray databases, Gene family, Gene, Neuroscience

Abstract

We performed an innovative systematic meta-analysis of 41 gene expression profiles of normal human hippocampus to provide a quantitative transcriptome reference map of it, i.e. a reference typical value of expression for each of the 30,739 known mapped and the 16,258 uncharacterized (unmapped) transcripts. For this aim, we used the software called TRAM (Transcriptome Mapper), which is able to generate transcriptome maps based on gene expression data from multiple sources. We also analyzed differential expression by comparing the hippocampus with the whole brain transcriptome map to identify a typical expression pattern of this subregion compared with the whole organ. Finally, due to the fact that the hippocampus is one of the main brain region to be severely affected in trisomy 21 (the best known genetic cause of intellectual disability), a particular attention was paid to the expression of chromosome 21 (chr21) genes. Data were downloaded from microarray databases, processed, and analyzed using TRAM software. Among the main findings, the most over-expressed loci in the hippocampus are the expressed sequence tag cluster Hs.732685 and the member of the calmodulin gene family CALM2. The tubulin folding cofactor B (TBCB) gene is the best gene at behaving like a housekeeping gene. The hippocampus vs. the whole brain differential transcriptome map shows the over-expression of LINC00114, a long non-coding RNA mapped on chr21. The hippocampus transcriptome map was validated in vitro by assaying gene expression through several magnitude orders by “Real-Time” reverse transcription polymerase chain reaction (RT-PCR). The highly significant agreement between in silico and experimental data suggested that our transcriptome map may be a useful quantitative reference benchmark for gene expression studies related to human hippocampus. Furthermore, our analysis yielded biological insights about those genes that have an intrinsic over-/under-expression in the hippocampus. © 2015 Wiley Periodicals, Inc.

Published

2015

38. A molecular view of the normal human thyroid structure and function reconstructed from its reference transcriptome map

Author

Maria Chiara Pelleri, Allison Piovesan, Francesca Antonaros, Lorenza Vitale, Maria Caracausi, Pierluigi Strippoli, Vitale, Lorenza, Piovesan, Allison, Antonaros, Francesca, Strippoli, Pierluigi, Pelleri, Maria Chiara, and Caracausi, Maria

Subjects

Male, 0301 basic medicine, endocrine system, lcsh:QH426-470, endocrine system diseases, lcsh:Biotechnology, In silico, Thyroid Gland, Human chromosome 21, Computational biology, Biology, Proteomics, Transcriptome, 03 medical and health sciences, Human thyroid, lcsh:TP248.13-248.65, Databases, Genetic, Gene expression, Genetics, medicine, Humans, Genes, Essential, Integrated transcriptome map, Gene Expression Profiling, Thyroid, Reference Standards, Reverse transcription polymerase chain reaction, lcsh:Genetics, Meta-analysis, Phenotype, 030104 developmental biology, medicine.anatomical_structure, Organ Specificity, Mutation, Female, DNA microarray, Research Article, Biotechnology

Abstract

Background The thyroid is the earliest endocrine structure to appear during human development, and thyroid hormones are necessary for proper organism development, in particular for the nervous system and heart, normal growth and skeletal maturation. To date a quantitative, validated transcriptional atlas of the whole normal human thyroid does not exist and the availability of a detailed expression map might be an excellent occasion to investigate the many features of the thyroid transcriptome. Results We present a view at the molecular level of the normal human thyroid histology and physiology obtained by a systematic meta-analysis of all the available gene expression profiles for the whole organ. A quantitative transcriptome reference map was generated by using the TRAM (Transcriptome Mapper) software able to combine, normalize and integrate a total of 35 suitable datasets from different sources thus providing a typical reference expression value for each of the 27,275 known, mapped transcripts obtained. The experimental in vitro validation of data was performed by “Real-Time” reverse transcription polymerase chain reaction showing an excellent correlation coefficient (r = 0.93) with data obtained in silico. Conclusions Our study provides a quantitative global reference portrait of gene expression in the normal human thyroid and highlights differential expression between normal human thyroid and a pool of non-thyroid tissues useful for modeling correlations between thyroidal gene expression and specific thyroid functions and diseases. The experimental in vitro validation supports the possible usefulness of the human thyroid transcriptome map as a reference for molecular studies of the physiology and pathology of this organ. Electronic supplementary material The online version of this article (doi:10.1186/s12864-017-4049-z) contains supplementary material, which is available to authorized users.

Published

2017

39. Integrated Quantitative Transcriptome Maps of Human Trisomy 21 Tissues and Cells

Author

Allison Piovesan, Chiara Locatelli, Chiara Cattani, Maria Chiara Pelleri, Lorenza Vitale, Pierluigi Strippoli, Guido Cocchi, Maria Caracausi, Francesca Antonaros, Pelleri, Maria Chiara, Cattani, Chiara, Vitale, Lorenza, Antonaros, Francesca, Strippoli, Pierluigi, Locatelli, Chiara, Cocchi, Guido, Piovesan, Allison, and Caracausi, Maria

Subjects

0301 basic medicine, lcsh:QH426-470, In silico, Down syndrome, Computational biology, Biology, Gene dosage, Transcriptome, 03 medical and health sciences, Genetic, Gene expression, Genetics, Meta-analysi, Gene, Genetics (clinical), Original Research, integrated transcriptome map, human chromosome 21, Reverse transcription polymerase chain reaction, meta-analysis, trisomy 21, lcsh:Genetics, 030104 developmental biology, Molecular Medicine, Human genome, Chromosome 21

Abstract

Down syndrome (DS) is due to the presence of an extra full or partial chromosome 21 (Hsa21). The identification of genes contributing to DS pathogenesis could be the key to any rational therapy of the associated intellectual disability. We aim at generating quantitative transcriptome maps in DS integrating all gene expression profile datasets available for any cell type or tissue, to obtain a complete model of the transcriptome in terms of both expression values for each gene and segmental trend of gene expression along each chromosome. We used the TRAM (Transcriptome Mapper) software for this meta-analysis, comparing transcript expression levels and profiles between DS and normal brain, lymphoblastoid cell lines, blood cells, fibroblasts, thymus and induced pluripotent stem cells, respectively. TRAM combined, normalized, and integrated datasets from different sources and across diverse experimental platforms. The main output was a linear expression value that may be used as a reference for each of up to 37,181 mapped transcripts analyzed, related to both known genes and expression sequence tag (EST) clusters. An independent example in vitro validation of fibroblast transcriptome map data was performed through “Real-Time” reverse transcription polymerase chain reaction showing an excellent correlation coefficient (r = 0.93, p < 0.0001) with data obtained in silico. The availability of linear expression values for each gene allowed the testing of the gene dosage hypothesis of the expected 3:2 DS/normal ratio for Hsa21 as well as other human genes in DS, in addition to listing genes differentially expressed with statistical significance. Although a fraction of Hsa21 genes escapes dosage effects, Hsa21 genes are selectively over-expressed in DS samples compared to genes from other chromosomes, reflecting a decisive role in the pathogenesis of the syndrome. Finally, the analysis of chromosomal segments reveals a high prevalence of Hsa21 over-expressed segments over the other genomic regions, suggesting, in particular, a specific region on Hsa21 that appears to be frequently over-expressed (21q22). Our complete datasets are released as a new framework to investigate transcription in DS for individual genes as well as chromosomal segments in different cell types and tissues.

Published

2017

40. Systematic identification of human housekeeping genes possibly useful as references in gene expression studies

Author

Allison Piovesan, Lorenza Vitale, Maria Chiara Pelleri, Francesca Antonaros, Maria Caracausi, Pierluigi Strippoli, Caracausi, Maria, Piovesan, Allison, Antonaros, Francesca, Strippoli, Pierluigi, Vitale, Lorenza, and Pelleri, Maria Chiara

Subjects

Adult, 0301 basic medicine, Cell type, Cancer Research, Biology, Biochemistry, Transcriptome, 03 medical and health sciences, Genetic, Databases, Genetic, Gene expression, Genetics, Humans, Human tissue, Housekeeping gene, Gene, Molecular Biology, Genes, Essential, Oncogene, Microarray analysis techniques, Gene Expression Profiling, human tissues, Reference gene, Articles, Genomics, Transcriptome mapping, Gene expression profiling, 030104 developmental biology, Oncology, Molecular Medicine

Abstract

The ideal reference, or control, gene for the study of gene expression in a given organism should be expressed at a medium‑high level for easy detection, should be expressed at a constant/stable level throughout different cell types and within the same cell type undergoing different treatments, and should maintain these features through as many different tissues of the organism. From a biological point of view, these theoretical requirements of an ideal reference gene appear to be best suited to housekeeping (HK) genes. Recent advancements in the quality and completeness of human expression microarray data and in their statistical analysis may provide new clues toward the quantitative standardization of human gene expression studies in biology and medicine, both cross‑ and within‑tissue. The systematic approach used by the present study is based on the Transcriptome Mapper tool and exploits the automated reassignment of probes to corresponding genes, intra‑ and inter‑sample normalization, elaboration and representation of gene expression values in linear form within an indexed and searchable database with a graphical interface recording quantitative levels of expression, expression variability and cross‑tissue width of expression for more than 31,000 transcripts. The present study conducted a meta‑analysis of a pool of 646 expression profile data sets from 54 different human tissues and identified actin γ 1 as the HK gene that best fits the combination of all the traditional criteria to be used as a reference gene for general use; two ribosomal protein genes, RPS18 and RPS27, and one aquaporin gene, POM121 transmembrane nucleporin C, were also identified. The present study provided a list of tissue‑ and organ‑specific genes that may be most suited for the following individual tissues/organs: Adipose tissue, bone marrow, brain, heart, kidney, liver, lung, ovary, skeletal muscle and testis; and also provides in these cases a representative, quantitative portrait of the relative, typical gene‑expression profile in the form of searchable database tables.

Published

2017

41. A quantitative transcriptome reference map of the normal human brain

Author

Maria Caracausi, Lorenza Vitale, Pierluigi Strippoli, Samantha Bruno, Allison Piovesan, Maria Chiara Pelleri, Caracausi M, Vitale L, Pelleri MC, Piovesan A, Bruno S, and Strippoli P

Subjects

Adult, Male, Databases, Factual, In silico, Biology, Transcriptome, Cellular and Molecular Neuroscience, Fetus, Sex Factors, Gene expression, Genetics, medicine, Humans, Microarray databases, TRANSCRIPTOME, Gene, Genetics (clinical), GENE EXPRESSION PROFILE, Gene Expression Profiling, Brain, Human brain, META-ANALYSIS, HUMAN BRAIN, Human genetics, Gene expression profiling, medicine.anatomical_structure, Female

Abstract

We performed an innovative systematic meta-analysis of 60 gene expression profiles of whole normal human brain, to provide a quantitative transcriptome reference map of it, i.e. a reference typical value of expression for each of the 39,250 known, mapped and 26,026 uncharacterized (unmapped) transcripts. To this aim, we used the software named Transcriptome Mapper (TRAM), which is able to generate transcriptome maps based on gene expression data from multiple sources. We also analyzed differential expression by comparing the brain transcriptome with those derived from human foetal brain gene expression, from a pool of human tissues (except the brain) and from the two normal human brain regions cerebellum and cerebral cortex, which are two of the main regions severely affected when cognitive impairment occurs, as happens in the case of trisomy 21. Data were downloaded from microarray databases, processed and analyzed using TRAM software and validated in vitro by assaying gene expression through several magnitude orders by 'real-time' reverse transcription polymerase chain reaction (RT-PCR). The excellent agreement between in silico and experimental data suggested that our transcriptome maps may be a useful quantitative reference benchmark for gene expression studies related to the human brain. Furthermore, our analysis yielded biological insights about those genes which have an intrinsic over-/under-expression in the brain, in addition offering a basis for the regional analysis of gene expression. This could be useful for the study of chromosomal alterations associated to cognitive impairment, such as trisomy 21, the most common genetic cause of intellectual disability.

Published

2014

42. Systematic reanalysis of partial trisomy 21 cases with or without Down syndrome suggests a small region on 21q22.13 as critical to the phenotype

Author

Alessandro Rocca, Lorenza Vitale, Guido Cocchi, Allison Piovesan, Giulia Poletti, Marco Seri, Maria Chiara Pelleri, Elena Cicchini, Pierluigi Strippoli, Chiara Locatelli, Maria Caracausi, Pelleri, Maria Chiara, Cicchini, Elena, Locatelli, Chiara, Vitale, Lorenza, Caracausi, Maria, Piovesan, Allison, Rocca, Alessandro, Poletti, Giulia, Seri, Marco, Strippoli, Pierluigi, and Cocchi, Guido

Subjects

0301 basic medicine, Male, Down syndrome, DNA Copy Number Variations, Genotype, Chromosomes, Human, Pair 21, Trisomy, Biology, Homology (biology), Chimpanzee genome project, 03 medical and health sciences, Gene duplication, Genetics, medicine, Down Syndrome Critical Region - Partial trisomy 21 - Copy Number Variant - Human genome, Humans, Copy-number variation, Molecular Biology, Genetics (clinical), Genetic Association Studies, Chromosome Mapping, General Medicine, Articles, medicine.disease, Phenotype, 030104 developmental biology, Female, Down Syndrome, Chromosome 21

Abstract

A 'Down Syndrome critical region' (DSCR) sufficient to induce the most constant phenotypes of Down syndrome (DS) had been identified by studying partial (segmental) trisomy 21 (PT21) as an interval of 0.6-8.3 Mb within human chromosome 21 (Hsa21), although its existence was later questioned. We propose an innovative, systematic reanalysis of all described PT21 cases (from 1973 to 2015). In particular, we built an integrated, comparative map from 125 cases with or without DS fulfilling stringent cytogenetic and clinical criteria. The map allowed to define or exclude as candidates for DS fine Hsa21 sequence intervals, also integrating duplication copy number variants (CNVs) data. A highly restricted DSCR (HR-DSCR) of only 34 kb on distal 21q22.13 has been identified as the minimal region whose duplication is shared by all DS subjects and is absent in all non-DS subjects. Also being spared by any duplication CNV in healthy subjects, HR-DSCR is proposed as a candidate for the typical DS features, the intellectual disability and some facial phenotypes. HR-DSCR contains no known gene and has relevant homology only to the chimpanzee genome. Searching for HR-DSCR functional loci might become a priority for understanding the fundamental genotype-phenotype relationships in DS.

Published

2016

43. Letter to the Editor: On osteocytes density in the human body

Author

Alina Beraudi, Silvia Canaider, Pierluigi Strippoli, Simone Tassani, Eva Bianconi, Beraudi, Alina, Tassani, Simone, Bianconi, Eva, Strippoli, Pierluigi, and Canaider, Silvia

Subjects

0301 basic medicine, Communication, Histology, Letter to the editor, Physiology, Computer science, business.industry, Endocrinology, Diabetes and Metabolism, Cell number, Bone, cell number, osteocytes, 030209 endocrinology & metabolism, Human body, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, business

Abstract

not available

Published

2016

44. Genome-scale analysis of human mRNA 5′ coding sequences based on expressed sequence tag (EST) database

Author

Lorenza Vitale, Eva Bianconi, Silvia Canaider, Federica Facchin, Maria Chiara Pelleri, Allison Piovesan, Pierluigi Strippoli, Raffaella Casadei, Flavia Frabetti, Piovesan A, Casadei R, Vitale L, Facchin F, Pelleri MC, Canaider S, Bianconi E, Frabetti F, Strippoli P., Casadei R., Piovesan A., Vitale L., Facchin F., Pelleri M.C., Canaider S., Bianconi E., and Frabetti F.

Subjects

DNA, Complementary, Five prime untranslated region, Molecular Sequence Data, Codon, Initiator, Biology, Open Reading Frames, Start codon, Databases, Genetic, Genetics, Humans, HUMAN GENOME, Coding region, MRNA 5&#8242, CODING SEQUENCE, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Genetic Association Studies, Expressed Sequence Tags, Expressed sequence tag, Genome, Human, 5&#8242, UNTRANSLATED REGION (5&#8242, UTR), mRNA 5′ coding sequence, Computational Biology, Shine-Dalgarno sequence, 5′ Untranslated region (5′ UTR), Sequence Analysis, DNA, EXPRESSED SEQUENCE TAG (EST), Stop codon, TRANSLATION START CODON, Open reading frame, Genetic Loci, Human genome, 5' Untranslated Regions, Sequence Alignment

Abstract

The term "5´ end mRNA artifact" refers to the incorrect assignment of the first AUG codon in an mRNA, due to the incomplete determination of its 5´ end sequence (Casadei et al., 2003). Since the '70s, the amino acid sequence of gene products has been routinely deduced from the nucleotide sequence of the relative cloned cDNA (DNA complementary to mRNA), according to rules for recognition of the start codon (first-AUG rule, optimal sequence context) and the genetic code (Kozak, 2002). All standard methods for the cloning of cDNA are affected by a potential inability to effectively clone the 5´ region of mRNA. This is due to the reverse transcriptase failure to extend first-strand cDNA along the full length of the mRNA template toward its 5´ end (Sambrook, 2001). The identification of a more complete mRNA 5´ end could reveal an additional upstream AUG – in-frame with the previously determined one – thus extending the predicted amino terminus sequence of the product and avoiding subsequent relevant errors in the experimental study of the relative cDNA (Casadei et al., 2003). The continuous incorporation of information derived from individual and large-scale cDNA sequencing projects, including those specifically designed to characterize mRNA 5´ end (Carninci et al., 1996; Suzuki et al., 2000; Porcel et al., 2004), in the last few years led to continuous improvement of completeness of mRNA reference sequences (e.g., RefSeq), and also to the corresponding protein coding sequences. However, genome browsers do not appear to systematically extract useful information from the ever-increasing vast quantity of EST (expressed sequence tag) data. To date, EST data remain invaluable due to significantly longer continuous RNA sequences they may provide in comparison with the very short fragments typically deposited in current high-throughput nucleotide sequencing databases. We previously used individual EST-based gene model refinement by classic in silico sequence analysis to revise the mRNA sequence of 109 human chromosome 21 protein-coding genes (Casadei et al., 2003). The success of this approach encouraged us to develop a piece of software ("5'_ORF_Extender" software) in order to automate the steps that were previously performed manually, applying it to the Danio rerio (zebrafish) genome (Frabetti et al., 2007). In the present work, we present a modified strategy able to analyze the much more numerous human sequences. Firstly, we fully revised the software algorithm by using pre-computed coordinates of the UCSC-downloaded RefSeqs and ESTs genome alignment data and specific UCSC-downloaded EST sequence entries. Furthermore, we adopted an original quality filter which was able to test if each single EST candidate with sequence information of possible use for extending a known mRNA, was attributed to the same locus of that mRNA by an updated, complete and embedded version of UniGene. Lastly, we automated data summarization for an analyzed genome. Following these improvements, parsing more than 7 million BLAT alignment, 5'_ORF_Extender 2.0 recognized a total of 477 loci, out of the 18,665 human loci represented in the mRNA reference set, as bona fide candidates for extension. Proof-of-concept confirmation was obtained by in vitro cloning and sequencing for GNB2L1 (guanine nucleotide binding protein (G protein), beta polypeptide 2-like 1), QARS (glutaminyl-tRNA synthetase) and TDP2 (tyrosyl-DNA phosphodiesterase 2) cDNAs, and the consequences for the functional studies of these loci are discussed. In addition, we generated a list of 20,775 human mRNAs in which the presence of an in-frame stop codon upstream of the known start codon indicates completeness of the coding sequence at 5´ in the current form. Bibliografia: R. Casadei et al., mRNA 5’ region sequence incompleteness: a potential source of systematic errors in translation initiation codon assignment in human mRNAs, Gene 321 (2003) 185–193. M. Kozak, Pushing the limits of the scanning mechanism for initiation of translation, Gene 99 (2002) 1–34. P. Carninci et al., High-efficiency fulllength cDNA cloning by biotinylated CAP trapper, Genomics 37 (1996) 327–336. F. Frabetti et al., Systematic analysis of mRNA 5’ coding sequence incompleteness in Danio rerio: an automated EST-based approach, Biol. Direct 2 (2007) 34.

Published

2012

45. Identification of minimal eukaryotic introns through GeneBase, a user-friendly tool for parsing the NCBI Gene databank

Author

Maria Chiara Pelleri, Pierluigi Strippoli, Lorenza Vitale, Allison Piovesan, Marco Ricci, Maria Caracausi, Piovesan, Allison, Caracausi, Maria, Ricci, Marco, Strippoli, Pierluigi, Vitale, Lorenza, and Pelleri, Maria Chiara

Subjects

Genomics, Computational biology, Biology, Exon, User-Computer Interface, computational biology, Data retrieval, Proto-Oncogene Proteins, Databases, Genetic, Genetics, Humans, gene data parsing, Molecular Biology, Gene, personal computer software, minimal intron, Hepatocyte Growth Factor, Intron, General Medicine, Full Papers, Introns, Identification (information), ComputingMethodologies_PATTERNRECOGNITION, RNA splicing, Databases, Nucleic Acid, NCBI Gene, MST1L Gene, Algorithms

Abstract

We have developed GeneBase, a full parser of the National Center for Biotechnology Information (NCBI) Gene database, which generates a fully structured local database with an intuitive user-friendly graphic interface for personal computers. Features of all the annotated eukaryotic genes are accessible through three main software tables, including for each entry details such as the gene summary, the gene exon/intron structure and the specific Gene Ontology attributions. The structuring of the data, the creation of additional calculation fields and the integration with nucleotide sequences allow users to make many types of comparisons and calculations that are useful for data retrieval and analysis. We provide an original example analysis of the existing introns across all the available species, through which the classic biological problem of the 'minimal intron' may find a solution using available data. Based on all currently available data, we can define the shortest known eukaryotic GT-AG intron length, setting the physical limit at the 30 base pair intron belonging to the human MST1L gene. This 'model intron' will shed light on the minimal requirement elements of recognition used for conventional splicing functioning. Remarkably, this size is indeed consistent with the sum of the splicing consensus sequence lengths.

Published

2015

46. An integrated route to identifying new pathogenesis-based therapeutic approaches for trisomy 21 (Down Syndrome) following the thought of Jérôme Lejeune

Author

Pierluigi Strippoli, Maria Caracausi, Doris Ricotta, Donatella Barisani, Marco Seri, Chiara Locatelli, Alessandro Ghezzo, Mark Basik, Anna Concetta Berardi, Allison Piovesan, Annalisa Radeghieri, Lorenza Vitale, Guido Cocchi, Maria Chiara Mimmi, Maria Chiara Pelleri, Maria Chiara Monaco, Pierluigi Strippoli, Maria Chiara Pelleri, Maria Caracausi, Lorenza Vitale, Allison Piovesan, Chiara Locatelli, Maria Chiara Mimmi, Anna Concetta Berardi, Doris Ricotta, Annalisa Radeghieri, Donatella Barisani, Mark Basik, Maria Chiara Monaco, Alessandro Ghezzo, Marco Seri, Guido Cocchi, Strippoli, P, Pelleri, M, Caracausi, M, Vitale, L, Piovesan, A, Locatelli, C, Mimmi, M, Berardi, A, Ricotta, D, Radeghieri, A, Barisani, D, Basik, M, Monaco, M, Ghezzo, A, Seri, M, and Cocchi, G

Subjects

lcsh:GE1-350, Down syndrome, Pathology, medicine.medical_specialty, therapy, lcsh:R, PATHOGENESIS, lcsh:Medicine, General Medicine, Biology, medicine.disease, Bioinformatics, Pathogenesis, Trisomy 21 (Down syndrome), medicine, Trisomy, lcsh:Environmental sciences

Abstract

Down Syndrome (DS) is the most frequent human chromosomal disorder. Main symptoms include intellectual disability (ID), cardiovascular defects and craniofacial dysmorphisms. Despite ID being measured by a test of symbolic logic skills, it is common for children with DS to arouse a climate of affective intensity greater than the norm. In 1959, Jérôme Lejeune (1926-1994) and coll. described an additional chromosome 21 (Hsa21) in children with DS (trisomy 21), giving origin to the field of medical genetics. Remarkably, the discovery of trisomy 21 had relevant social consequences for the affected children, in that their parents were no longer suspected to be alcoholics or infected with syphilis. Although it is broadly agreed that the DS phenotype originates from the altered expression of the genes located on Hsa21, its molecular pathogenesis is still unknown. To date, no therapy is recognized and recommended by guidelines as being effective in improving the cognitive abilities of persons with DS. The aim of this article is to categorize main therapeutical approaches or pathways to new approaches reported in the biomedical literature, to extract critical methodological points from the works of Lejeune and then to propose a new research project aimed to generate and integrate clinical, biochemical, genetic and bioinformatic data in order to identify novel therapeutic targets for this form of trisomy. We show here that nearly all the current lines of research were pursued, theorized or foreseen by Lejeune, and that central points of his method remain current: positive hypothesis about the existence of a solution, envision of systematic investigation of cell machinery, anchoring of clinical and biochemical finding to the chromosome physical map, and continuing clinical observation of the affected children. We therefore propose a project aimed at producing both experimentally and by meta-analysis state-of-the-art maps and databases related to clinical/phenotype, cytogenetics, exome, transcriptome, methylome, molecular biology, metabolome and mutations data. The primary expected outcome of this research project is the identification of a restricted list of strong candidate genes and mechanisms for ID in persons with DS in order to devise new rational therapeutic approaches.

Published

2013

47. An estimation of the number of cells in the human body

Author

Flavia Frabetti, Alina Beraudi, Allison Piovesan, Lorenza Vitale, Federica Facchin, Raffaella Casadei, Soledad Perez-Amodio, Simone Tassani, Eva Bianconi, Silvia Canaider, Pierluigi Strippoli, Maria Chiara Pelleri, Francesco Piva, Eva Bianconi, Allison Piovesan, Federica Facchin, Alina Beraudi, Raffaella Casadei, Flavia Frabetti, Lorenza Vitale, Maria Chiara Pelleri, Simone Tassani, Francesco Piva, Amodio Soledad Perez, Pierluigi Strippoli, and Silvia Canaider

Subjects

Adult, Aging, Physiology, Epidemiology, Cell Count, Computational biology, Biology, Human cell number, Models, Biological, Cell size, 03 medical and health sciences, 0302 clinical medicine, Type (biology), Genetics, Humans, Total cell count, Organism, 030304 developmental biology, 0303 health sciences, Public Health, Environmental and Occupational Health, Human body, Organ Specificity, Organ, 030220 oncology & carcinogenesis

Abstract

Background: All living organisms are made of individual and identifiable cells, whose number, together with their size and type, ultimately defines the structure and functions of an organism. While the total cell number of lower organisms is often known, it has not yet been defined in higher organisms. In particular, the reported total cell number of a human being ranges between 1012 and 1016 and it is widely mentioned without a proper reference. Aim: To study and discuss the theoretical issue of the total number of cells that compose the standard human adult organism. Subjects and methods: A systematic calculation of the total cell number of the whole human body and of the single organs was carried out using bibliographical and/or mathematical approaches. Results: A current estimation of human total cell number calculated for a variety of organs and cell types is presented. These partial data correspond to a total number of 3.72 × 1013. Conclusions: Knowing the total cell number of the human body as well as of individual organs is important from a cultural, biological, medical and comparative modelling point of view. The presented cell count could be a starting point for a common effort to complete the total calculation.

Published

2013

48. Universal tight correlation of codon bias and pool of RNA codons (codonome): The genome is optimized to allow any distribution of gene expression values in the transcriptome from bacteria to humans

Author

Maria Chiara Pelleri, Lorenza Vitale, Allison Piovesan, Pierluigi Strippoli, Allison Piovesan, Lorenza Vitale, Maria Chiara Pelleri, and Pierluigi Strippoli

Subjects

DNA codon table, Erythrocytes, Codon bias, Pool of RNA codon, Saccharomyces cerevisiae, Biology, Genome, Transcriptome, Amino Acyl-tRNA Synthetases, Codonome, Gene expression, Genetics, Escherichia coli, Animals, Humans, Caenorhabditis elegans, Codon, Gene, Zebrafish, Codon bia, Base Sequence, Models, Genetic, Genome, Human, Brain, Open reading frame, Gene Expression Regulation, Codon usage bias, Pool of RNA codons, Synonymous substitution, Databases, Nucleic Acid, Genome, Bacterial, Software

Abstract

Codon bias is the phenomenon in which distinct synonymous codons are used with different frequencies. We define here the “codonome value” as the total number of codons present across all the expressed mRNAs in a given biological condition. We have developed the “CODONOME” software, which calculates the codon bias and, following integration with a gene expression profile, estimates the actual frequency of each codon at the transcriptome level (codonome bias) of a given tissue. Systematic analysis across different human tissues and multiple species shows a surprisingly tight correlation between the codon bias and the codonome bias. An aneuploidy and cancer condition such as that of Down Syndrome-related acute megakaryoblastic leukemia (DS-AMKL), does not appear to alter this relationship. The law of correlation between codon bias and codonome emerges as a property of the distribution and range of the number, sequence and expression level of the genes in a genome.

Published

2013

49. Proteins encoded by human Down syndrome critical region gene 1-like 2 (DSCR1L2) mRNA and by a novel DSCR1L2 mRNA isoform interact with cardiac troponin I (TNNI3)

Author

Paolo Carinci, Maria Zannotti, Federica Facchin, Silvia Canaider, Luca Lenzi, Pierluigi Strippoli, Flavia Frabetti, Raffaella Casadei, Pietro D'Addabbo, Lorenza Vitale, Cristiana Griffoni, Canaider S, Facchin F, Griffoni C, Casadei R, Vitale L, Lenzi L, Frabetti F, D'Addabbo P, Carinci P, Zannotti M, and Strippoli P

Subjects

Adult, Gene isoform, DNA, Complementary, Protein family, Recombinant Fusion Proteins, Molecular Sequence Data, Biology, TNNI3, Open Reading Frames, Two-hybrid system techniques, Troponin complex, Yeasts, Troponin I, Genetics, Humans, Protein Isoforms, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, education, Adaptor Proteins, Signal Transducing, education.field_of_study, Reverse Transcriptase Polymerase Chain Reaction, Alternative splicing, Proteins, General Medicine, Glutathione, Molecular biology, Fusion protein, Human heart, DOWN SYNDROME CRITICAL REGION GENE 1, Sequence Alignment, Protein Binding

Abstract

Down syndrome critical region gene 1-like 2 (DSCR1L2) belongs to the human DSCR1-like gene family, which also includes DSCR1 and DSCR1L1. Both DSCR1 and DSCR1L1 proteins interact with calcineurin, a calcium/calmodulin-dependent phosphatase. To date, no interactor has been described for DSCR1L2. The aim of this work was to perform a first functional study of DSCR1L2 using yeast two-hybrid analysis conducted on a human heart cDNA library. Here, we report the interaction between DSCR1L2 and the human cardiac troponin I (TNNI3), the heart-specific inhibitory subunit of the troponin complex, a central component of the contractile apparatus. This interaction was confirmed by both yeast cotransformation and GST (glutathione-sepharose transferase) fusion protein assay. Moreover, a new DSCR1L2 mRNA isoform, generated by alternative splicing, was identified and cloned in different tissues: it lacks two central exons, encoding the most conserved domains among the DSCR1-like protein family. A quantitative relative reverse transcription-polymerase chain reaction (RT-PCR) assay showed that in heart tissue the normalized expression level ratio for DSCR1L2 and DSCR1L2-E2E5 mRNA isoforms is 3.5 : 1, respectively. The yeast cotransformation and GST fusion protein assay demonstrated the interaction between this new DSCR1L2 variant and the human cardiac troponin I and the prominent role of DSCR1L2 exon 2 in determining binding between both DSCR1L2 isoforms and TNNI3. These data indicate an entirely new role for a DSCR1-like family gene, suggesting a possible involvement of DSCR1L2 in cardiac contraction.

Published

2006

50. Cysteine and tyrosine-rich 1 (CYYR1), a novel unpredicted gene on human chromosome 21 (21q21.2), encodes a cysteine and tyrosine-rich protein and defines a new family of highly conserved vertebrate-specific genes

Author

Pietro D'Addabbo, Paolo Carinci, Silvia Canaider, Luca Lenzi, Lorenza Vitale, Pierluigi Strippoli, Maria Zannotti, Sandra Giannone, and Raffaella Casadei

Subjects

DNA, Complementary, Protein family, Chromosomes, Human, Pair 21, Molecular Sequence Data, Gene Expression, Biology, Evolution, Molecular, Mice, Complementary DNA, Gene cluster, Genetics, Animals, Humans, Coding region, Amino Acid Sequence, RNA, Messenger, Gene, Phylogeny, Expressed Sequence Tags, Radiation Hybrid Mapping, Expressed sequence tag, Sequence Homology, Amino Acid, Intron, Membrane Proteins, Proteins, Sequence Analysis, DNA, General Medicine, Blotting, Northern, Molecular biology, Vertebrates, Female, Databases, Nucleic Acid, Chromosome 21, Sequence Alignment

Abstract

A novel human gene has been identified by in-depth bioinformatics analysis of chromosome 21 segment 40/105 (21q21.1), with no coding region predicted in any previous analysis. Brain-derived DNA complementary to RNA (cDNA) sequencing predicts a 154-amino acid product with no similarity to any known protein. The gene has been named cysteine and tyrosine-rich protein 1 gene (symbol cysteine and tyrosine-rich 1, CYYR1). The CYYR1 messenger RNA was found by Northern blot analysis in a broad range of tissues (two transcripts of 3.4 and 2.2 kb). The gene consists of four exons and spans about 107 kb, including a very large intron of 85.8 kb. Analysis of expressed sequence tags shows high CYYR1 expression in cells belonging to the amine precursor uptake and decarboxylation system. We also cloned the cDNA of the murine ortholog Cyyr1, which was mapped by a radiation hybrid panel on chromosome 16 within the region corresponding to that containing the respective human homolog on chromosome 21. Sequence and phylogenetic analysis led to identification of several genes encoding CYYR1 homologous proteins. The most prominent feature identified in the protein family is a central, unique cysteine and tyrosine-rich domain, which is strongly conserved from lower vertebrates (fishes) to humans but is absent in bacteria and invertebrates.

Published

2002