Your search keyword '"Quayum N"' showing total 9 results

1. Global gene expression profiling and histochemical analysis of the developing human fetal pancreas

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Author

Sarkar, S. A., Kobberup, S., Wong, R., Lopez, A. D., Quayum, N., Still, T., Kutchma, A., Jensen, J. N., Gianani, R., Beattie, G. M., Jensen, J., Hayek, A., and Hutton, J. C.

Published

2008

2. Longitudinal changes in bone mineral content and body composition in boys with Duchenne muscular dystrophy

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Author

McDevitt, H., McWilliam, R., Quayum, N., and Ahmed, S.

Published

2007

3. Nationwide, Couple-Based Genetic Carrier Screening.

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Author

Kirk EP, Delatycki MB, Archibald AD, Tutty E, Caruana J, Halliday JL, Lewis S, McClaren BJ, Newson AJ, Dive L, Best S, Long JC, Braithwaite J, Downes MJ, Scuffham PA, Massie J, Barlow-Stewart K, Kulkarni A, Ruscigno A, Kanga-Parabia A, Rodrigues B, Bennetts BH, Ebzery C, Hunt C, Cliffe CC, Lee C, Azmanov D, King EA, Madelli EO, Zhang F, Ho G, Danos I, Liebelt J, Fletcher J, Kennedy J, Beilby J, Emery JD, McGaughran J, Marum JE, Scarff K, Fisk K, Harrison K, Boggs K, Giameos L, Fitzgerald L, Thomas L, Burnett L, Freeman L, Harris M, Berbic M, Davis MR, Cifuentes Ochoa M, Wallis M, Wall M, Chow MTM, Ferrie MM, Pachter N, Quayum N, Lang N, Kasi Pandy P, Casella R, Allcock RJN, Ong R, Edwards S, Sundercombe S, Jelenich S, Righetti S, Lunke S, Kaur S, Stock-Myer S, Eggers S, Walker SP, Theodorou T, Catchpool T, Clinch T, Roscioli T, Hardy T, Zhu Y, Fehlberg Z, Boughtwood TF, and Laing NG more...

Subjects

Adult, Female, Humans, Male, Pregnancy, Australia, Feasibility Studies, Patient Acceptance of Health Care statistics & numerical data, Decision Making, Heterozygote, Family Characteristics, Reproductive Behavior, Genetic Carrier Screening methods, Genetic Carrier Screening statistics & numerical data, Genetic Diseases, Inborn genetics, Genetic Diseases, Inborn prevention & control, Genetic Diseases, Inborn psychology

Abstract

Background: Genomic sequencing technology allows for identification of reproductive couples with an increased chance, as compared with that in the general population, of having a child with an autosomal recessive or X-linked genetic condition., Methods: We investigated the feasibility, acceptability, and outcomes of a nationwide, couple-based genetic carrier screening program in Australia as part of the Mackenzie's Mission project. Health care providers offered screening to persons before pregnancy or early in pregnancy. The results obtained from testing at least 1281 genes were provided to the reproductive couples. We aimed to ascertain the psychosocial effects on participants, the acceptability of screening to all participants, and the reproductive choices of persons identified as having an increased chance of having a child with a condition for which we screened., Results: Among 10,038 reproductive couples enrolled in the study, 9107 (90.7%) completed screening, and 175 (1.9%) were newly identified as having an increased chance of having a child with a genetic condition for which we screened. These conditions involved pathogenic variants in 90 different genes; 74.3% of the conditions were autosomal recessive. Three months after receiving the results, 76.6% of the couples with a newly identified increased chance had used or planned to use reproductive interventions to avoid having an affected child. Those newly identified as having an increased chance had greater anxiety than those with a low chance. The median level of decisional regret was low in all result groups, and 98.9% of participants perceived screening to be acceptable., Conclusions: Couple-based reproductive genetic carrier screening was largely acceptable to participants and was used to inform reproductive decision making. The delivery of screening to a diverse and geographically dispersed population was feasible. (Funded by the Medical Research Future Fund of the Australian government; ClinicalTrials.gov number, NCT04157595.)., (Copyright © 2024 Massachusetts Medical Society.) more...

Published

2024

4. Clinically Responsive Genomic Analysis Pipelines: Elements to Improve Detection Rate and Efficiency.

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Sundercombe SL, Berbic M, Evans CA, Cliffe C, Elakis G, Temple SEL, Selvanathan A, Ewans L, Quayum N, Nixon CY, Dias KR, Lang S, Richards A, Goh S, Wilson M, Mowat D, Sachdev R, Sandaradura S, Walsh M, Farrar MA, Walsh R, Fletcher J, Kirk EP, Teunisse GM, Schofield D, Buckley MF, Zhu Y, and Roscioli T more...

Subjects

Cost-Benefit Analysis, Exome, Genetic Testing economics, Genome, Human, Genomics economics, High-Throughput Nucleotide Sequencing economics, Humans, INDEL Mutation, Phenotype, Polymorphism, Single Nucleotide, Sensitivity and Specificity, Exome Sequencing economics, Genetic Diseases, Inborn genetics, Genetic Testing methods, Genomics methods, Germ-Line Mutation, High-Throughput Nucleotide Sequencing methods, Exome Sequencing methods

Abstract

Massively parallel sequencing has markedly improved mendelian diagnostic rates. This study assessed the effects of custom alterations to a diagnostic genomic bioinformatic pipeline in response to clinical need and derived practice recommendations relative to diagnostic rates and efficiency. The Genomic Annotation and Interpretation Application (GAIA) bioinformatics pipeline was designed to detect panel, exome, and genome sample integrity and prioritize gene variants in mendelian disorders. Reanalysis of selected negative cases was performed after improvements to the pipeline. GAIA improvements and their effect on sensitivity are described, including addition of a PubMed search for gene-disease associations not in the Online Mendelian Inheritance of Man database, inclusion of a process for calling low-quality variants (known as QPatch), and gene symbol nomenclature consistency checking. The new pipeline increased the diagnostic rate and reduced staff costs, resulting in a saving of US$844.34 per additional diagnosis. Recommendations for genomic analysis pipeline requirements are summarized. Clinically responsive bioinformatics pipeline improvements increase diagnostic sensitivity and increase cost-effectiveness., (Crown Copyright © 2021. Published by Elsevier Inc. All rights reserved.) more...

Published

2021

5. Effect of alginate encapsulation on the cellular transcriptome of human islets.

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Author

Vaithilingam V, Quayum N, Joglekar MV, Jensen J, Hardikar AA, Oberholzer J, Guillemin GJ, and Tuch BE

Subjects

Alginates chemistry, Animals, Base Sequence, Blotting, Western, DNA Primers, Down-Regulation drug effects, Gene Expression Profiling, Glucuronic Acid chemistry, Glucuronic Acid pharmacology, Hexuronic Acids chemistry, Hexuronic Acids pharmacology, Humans, Insulin metabolism, Insulin Secretion, Islets of Langerhans metabolism, Islets of Langerhans Transplantation, Mice, Mice, Inbred NOD, Mice, SCID, Oligonucleotide Array Sequence Analysis, Principal Component Analysis, Real-Time Polymerase Chain Reaction, Up-Regulation drug effects, Alginates pharmacology, Islets of Langerhans drug effects, Transcriptome

Abstract

Encapsulation of human islets may prevent their immune rejection when transplanted into diabetic recipients. To assist in understanding why clinical outcomes with encapsulated islets were not ideal, we examined the effect of encapsulation on their global gene (mRNA) and selected miRNAs (non-coding (nc)RNA) expression. For functional studies, encapsulated islets were transplanted into peritoneal cavity of diabetic NOD-SCID mice. Genomics analysis and transplantation studies demonstrate that islet origin and isolation centres are a major source of variation in islet quality. In contrast, tissue culture and the encapsulation process had only a minimal effect, and did not affect islet viability. Microarray analysis showed that as few as 29 genes were up-regulated and 2 genes down-regulated (cut-off threshold 0.1) by encapsulation. Ingenuity analysis showed that up-regulated genes were involved mostly in inflammation, especially chemotaxis, and vascularisation. However, protein expression of these factors was not altered by encapsulation, raising doubts about the biosignificance of the gene changes. Encapsulation had no effect on levels of islet miRNAs. In vivo studies indicate differences among the centres in the quality of the islets isolated. We conclude that microencapsulation of human islets with barium alginate has little effect on their transcriptome., (Copyright © 2011 Elsevier Ltd. All rights reserved.) more...

Published

2011

6. Sox6 is necessary for efficient erythropoiesis in adult mice under physiological and anemia-induced stress conditions.

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Author

Dumitriu B, Bhattaram P, Dy P, Huang Y, Quayum N, Jensen J, and Lefebvre V

Subjects

Anemia metabolism, Anemia pathology, Animals, Biomarkers metabolism, Cell Survival, Erythrocytes cytology, Erythrocytes metabolism, Erythrocytes pathology, Erythropoietin metabolism, Mice, Signal Transduction, Up-Regulation, bcl-X Protein genetics, Anemia physiopathology, Erythropoiesis, SOXD Transcription Factors metabolism, Stress, Physiological

Abstract

Background: Definitive erythropoiesis is a vital process throughout life. Both its basal activity under physiological conditions and its increased activity under anemia-induced stress conditions are highly stimulated by the hormone erythropoietin. The transcription factor Sox6 was previously shown to enhance fetal erythropoiesis together and beyond erythropoietin signaling, but its importance in adulthood and mechanisms of action remain unknown. We used here Sox6 conditional null mice and molecular assays to address these questions., Methodology/principal Findings: Sox6fl/flErGFPCre adult mice, which lacked Sox6 in erythroid cells, exhibited compensated anemia, erythroid cell developmental defects, and anisocytotic, short-lived red cells under physiological conditions, proving that Sox6 promotes basal erythropoiesis. Tamoxifen treatment of Sox6fl/flCaggCreER mice induced widespread inactivation of Sox6 in a timely controlled manner and resulted in erythroblast defects before reticulocytosis, demonstrating that impaired erythropoiesis is a primary cause rather than consequence of anemia in the absence of Sox6. Twenty five percent of Sox6fl/flErGFPCre mice died 4 or 5 days after induction of acute anemia with phenylhydrazine. The others recovered slowly. They promptly increased their erythropoietin level and amplified their erythroid progenitor pool, but then exhibited severe erythroblast and reticulocyte defects. Sox6 is thus essential in the maturation phase of stress erythropoiesis that follows the erythropoietin-dependent amplification phase. Sox6 inactivation resulted in upregulation of embryonic globin genes, but embryonic globin chains remained scarce and apparently inconsequential. Sox6 inactivation also resulted in downregulation of erythroid terminal markers, including the Bcl2l1 gene for the anti-apoptotic factor Bcl-xL, and in vitro assays indicated that Sox6 directly upregulates Bcl2l1 downstream of and beyond erythropoietin signaling., Conclusions/significance: This study demonstrates that Sox6 is necessary for efficient erythropoiesis in adult mice under both basal and stress conditions. It is primarily involved in enhancing the survival rate and maturation process of erythroid cells and acts at least in part by upregulating Bcl2l1. more...

Published

2010

7. Establishment of extracellular signal-regulated kinase 1/2 bistability and sustained activation through Sprouty 2 and its relevance for epithelial function.

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Author

Liu W, Tundwal K, Liang Q, Goplen N, Rozario S, Quayum N, Gorska M, Wenzel S, Balzar S, and Alam R

Subjects

Active Transport, Cell Nucleus physiology, Adaptor Proteins, Signal Transducing, Animals, Asthma metabolism, Asthma physiopathology, Cell Survival physiology, Cells, Cultured, Endosomes metabolism, Enzyme Activation, Epithelial Cells cytology, Gene Expression Profiling, Humans, Intracellular Signaling Peptides and Proteins genetics, Membrane Proteins genetics, Mice, Microarray Analysis, Mitogen-Activated Protein Kinase 1 genetics, Mitogen-Activated Protein Kinase 3 genetics, Protein Serine-Threonine Kinases, RNA, Small Interfering genetics, RNA, Small Interfering metabolism, Rats, Signal Transduction physiology, rab GTP-Binding Proteins genetics, rab GTP-Binding Proteins metabolism, src-Family Kinases antagonists & inhibitors, src-Family Kinases metabolism, Enzyme Stability, Epithelial Cells physiology, Intracellular Signaling Peptides and Proteins metabolism, Membrane Proteins metabolism, Mitogen-Activated Protein Kinase 1 metabolism, Mitogen-Activated Protein Kinase 3 metabolism

Abstract

Our objective was to establish an experimental model of a self-sustained and bistable extracellular signal-regulated kinase 1/2 (ERK1/2) signaling process. A single stimulation of cells with cytokines causes rapid ERK1/2 activation, which returns to baseline in 4 h. Repeated stimulation leads to sustained activation of ERK1/2 but not Jun N-terminal protein kinase (JNK), p38, or STAT6. The ERK1/2 activation lasts for 3 to 7 days and depends upon a positive-feedback mechanism involving Sprouty 2. Overexpression of Sprouty 2 induces, and its genetic deletion abrogates, ERK1/2 bistability. Sprouty 2 directly activates Fyn kinase, which then induces ERK1/2 activation. A genome-wide microarray analysis shows that the bistable phospho-ERK1/2 (pERK1/2) does not induce a high level of gene transcription. This is due to its nuclear exclusion and compartmentalization to Rab5+ endosomes. Cells with sustained endosomal pERK1/2 manifest resistance against growth factor withdrawal-induced cell death. They are primed for heightened cytokine production. Epithelial cells from cases of human asthma and from a mouse model of chronic asthma manifest increased pERK1/2, which is associated with Rab5+ endosomes. The increase in pERK1/2 was associated with a simultaneous increase in Sprouty 2 expression in these tissues. Thus, we have developed a cellular model of sustained ERK1/2 activation, which may provide a mechanistic understanding of self-sustained biological processes in chronic illnesses such as asthma. more...

Published

2010

8. GeneSpeed Beta Cell: an online genomics data repository and analysis resource tailored for the islet cell biologist.

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Author

Quayum N, Kutchma A, Sarkar SA, Juhl K, Gradwohl G, Mellitzer G, Hutton JC, and Jensen J

Subjects

Animals, Computational Biology trends, Gene Expression Profiling, Humans, Internet, Islets of Langerhans physiology, Oligonucleotide Array Sequence Analysis, Pancreas physiology, Databases, Genetic, Genomics methods, Insulin-Secreting Cells physiology

Abstract

Objective: We here describe the development of a freely available online database resource, GeneSpeed Beta Cell, which has been created for the pancreatic islet and pancreatic developmental biology investigator community., Research Design and Methods: We have developed GeneSpeed Beta Cell as a separate component of the GeneSpeed database, providing a genomics-type data repository of pancreas and islet-relevant datasets interlinked with the domain-oriented GeneSpeed database., Results: GeneSpeed Beta Cell allows the query of multiple published and unpublished select genomics datasets in a simultaneous fashion (multiexperiment viewing) and is capable of defining intersection results from precomputed analysis of such datasets (multidimensional querying). Combined with the protein-domain categorization/assembly toolbox provided by the GeneSpeed database, the user is able to define spatial expression constraints of select gene lists in a relatively rigid fashion within the pancreatic expression space. We provide several demonstration case studies of relevance to islet cell biology and development of the pancreas that provide novel insight into islet biology., Conclusions: The combination of an exhaustive domain-based compilation of the transcriptome with gene array data of interest to the islet biologist affords novel methods for multidimensional querying between individual datasets in a rapid fashion, presently not available elsewhere. more...

Published

2008

9. GeneSpeed: protein domain organization of the transcriptome.

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Author

Kutchma A, Quayum N, and Jensen J

Subjects

Animals, Caenorhabditis elegans Proteins chemistry, Drosophila Proteins chemistry, Gene Expression Profiling, Humans, Internet, Mice, Sequence Alignment, Sequence Homology, Amino Acid, Transcription Factors chemistry, Transcription, Genetic, User-Computer Interface, Databases, Protein, Protein Structure, Tertiary genetics

Abstract

The GeneSpeed database (http://genespeed.uchsc.edu/) is an online database and resource tool facilitating the detailed study of protein domain homology in the transcriptomes of Homo sapiens, Mus musculus, Drosophila melanogaster and Caenorhabditis elegans. The population schema for the GeneSpeed database takes advantage of HOWARD parallel cluster technology (http://www.massivelyparallel.com/) and performs exhaustive tBLASTn searches covering all pre-assigned PFAM domain classes in all species (currently 7973 domain families) against the respective Unigene EST databases of the selected four transcriptomes. The resulting database provides a complete annotation of presumed protein domain presence for each Unigene cluster. To complement this domain annotation we have also performed a custom transcription factor-family curation of all Pfam domains, incorporated the Gene Ontology classifications for these domains as well as integrated the Novartis SymAtlas2 dataset for both human and mouse which provides rapid and easy access to tissue-based expression analysis. Consequently, the GeneSpeed database provides the user with the capability to browse or search the database by any of these specialized criteria as well as more traditional means (gene identifier, gene symbol, etc.), thereby enabling a supervised analysis of gene families through a top-down hierarchical basis defined by domain content, all directly linked to an optimized gene expression dataset. more...

Published

2007