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2. Mutant (CCTG)n Expansion Causes Abnormal Expression of Zinc Finger Protein 9 (ZNF9) in Myotonic Dystrophy Type 2

Author

Ralf Krahe, Anna Vihola, Shodimu Emmanuel Olufemi, Mario Sirito, Yi-Ping Li, Jeanette Holmlund-Hampf, Hannu Haapasalo, Bjarne Udd, Linda L. Bachinski, and Olayinka Raheem

Subjects
Adult, Male, musculoskeletal diseases, medicine.medical_specialty, RNA-binding protein, Biology, Myotonic dystrophy, Pathology and Forensic Medicine, Young Adult, 03 medical and health sciences, 0302 clinical medicine, Internal medicine, medicine, Humans, Myotonic Dystrophy, Tissue Distribution, Muscle, Skeletal, Aged, 030304 developmental biology, Regulation of gene expression, Zinc finger, 0303 health sciences, DNA Repeat Expansion, Muscle cell differentiation, Gene Expression Profiling, Alternative splicing, Intron, RNA-Binding Proteins, Middle Aged, Microarray Analysis, medicine.disease, Molecular biology, Endocrinology, Gene Expression Regulation, Mutation, RNA splicing, Female, 030217 neurology & neurosurgery, Regular Articles, Myotonic Disorders
Abstract

The mutation that underlies myotonic dystrophy type 2 (DM2) is a (CCTG)n expansion in intron 1 of zinc finger protein 9 (ZNF9). It has been suggested that ZNF9 is of no consequence for disease pathogenesis. We determined the expression levels of ZNF9 during muscle cell differentiation and in DM2 muscle by microarray profiling, real-time RT-PCR, splice variant analysis, immunofluorescence, and Western blotting. Our results show that in differentiating myoblasts, ZNF9 protein was localized primarily to the nucleus, whereas in mature muscle fibers, it was cytoplasmic and organized in sarcomeric striations at the Z-disk. In patients with DM2, ZNF9 was abnormally expressed. First, there was an overall reduction in both the mRNA and protein levels. Second, the subcellular localization of the ZNF9 protein was somewhat less cytoplasmic and more membrane-bound. Third, our splice variant analysis revealed retention of intron 3 in an aberrant isoform, and fourth quantitative allele-specific expression analysis showed the persistence of intron 1 sequences from the abnormal allele, further suggesting that the mutant allele is incompletely spliced. Thus, the decrease in total expression appears to be due to impaired splicing of the mutant transcript. Our data indicate that ZNF9 expression in DM2 patients is altered at multiple levels. Although toxic RNA effects likely explain overlapping phenotypic manifestations between DM1 and DM2, abnormal ZNF9 levels in DM2 may account for the differences in DM1.

Published
2010
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3. Differences in aberrant expression and splicing of sarcomeric proteins in the myotonic dystrophies DM1 and DM2

Author

Olayinka Raheem, Anna Vihola, Anders Paetau, Jeanette Holmlund-Hampf, Shodimu-Emmanuel Olufemi, Giovanni Meola, Ralf Krahe, Lars Edström, Shohrae Hajibashi, Hannu Haapasalo, Bjarne Udd, Tiina Suominen, Keith A. Baggerly, Linda L. Bachinski, Rosanna Cardani, Hannu Kalimo, and Mario Sirito

Subjects
Male, musculoskeletal diseases, Gene isoform, Muscle Fibers, Skeletal, Myosins, Biology, Article, Pathology and Forensic Medicine, Cellular and Molecular Neuroscience, Troponin T, Myosin, Humans, Myotonic Dystrophy, Protein Isoforms, Gene, Adaptor Proteins, Signal Transducing, Oligonucleotide Array Sequence Analysis, Messenger RNA, Alternative splicing, LIM Domain Proteins, Phenotype, Molecular biology, Alternative Splicing, Muscular Atrophy, Gene Expression Regulation, RNA splicing, Female, Neurology (clinical), TNNT3, Transcription Factors
Abstract

Aberrant transcription and mRNA processing of multiple genes due to RNA-mediated toxic gain-of-function has been suggested to cause the complex phenotype in myotonic dystrophies type 1 and 2 (DM1 and DM2). However, the molecular basis of muscle weakness and wasting and the different pattern of muscle involvement in DM1 and DM2 are not well understood. We have analyzed the mRNA expression of genes encoding muscle-specific proteins and transcription factors by microarray profiling and studied selected genes for abnormal splicing. A subset of the abnormally regulated genes was further analyzed at the protein level. TNNT3 and LDB3 showed abnormal splicing with significant differences in proportions between DM2 and DM1. The differential abnormal splicing patterns for TNNT3 and LDB3 appeared more pronounced in DM2 relative to DM1 and are among the first molecular differences reported between the two diseases. In addition to these specific differences, the majority of the analyzed genes showed an overall increased expression at the mRNA level. In particular, there was a more global abnormality of all different myosin isoforms in both DM1 and DM2 with increased transcript levels and a differential pattern of protein expression. Atrophic fibers in DM2 patients expressed only the fast myosin isoform, while in DM1 patients they co-expressed fast and slow isoforms. However, there was no increase of total myosin protein levels, suggesting that aberrant protein translation and/or turnover may also be involved.

Published
2010
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4. Intestinal Ischemic Preconditioning After Ischemia/Reperfusion Injury in Rat Intestine: Profiling Global Gene Expression Patterns

Author

Rosemary A. Kozar, Steven T. Lott, Bruce C. Kone, Ravi S. Radhakrishnan, Stacey D. Moore-Olufemi, Shodimu Emmanuel Olufemi, Shinil K. Shah, Frederick A. Moore, Norio Sato, Fernando Jimenez, and Charles S. Cox

Subjects
Male, Pathology, medicine.medical_specialty, Necrosis, Physiology, Ischemia, Rats, Sprague-Dawley, Random Allocation, Intestinal mucosa, Ileum, Reference Values, parasitic diseases, Gene expression, medicine, Animals, Cluster Analysis, cardiovascular diseases, Intestinal Mucosa, Ischemic Preconditioning, Oligonucleotide Array Sequence Analysis, Probability, Regulation of gene expression, Analysis of Variance, Reverse Transcriptase Polymerase Chain Reaction, business.industry, Gene Expression Profiling, Gastroenterology, Microarray Analysis, medicine.disease, Rats, Gene expression profiling, Disease Models, Animal, Gene Expression Regulation, Reperfusion Injury, RNA, Ischemic preconditioning, medicine.symptom, business, Reperfusion injury
Abstract

Intestinal ischemia/reperfusion (IR) injury involves activation of inflammatory mediators, mucosal necrosis, ileus, and alteration in a variety of gene products. Ischemic preconditioning (IPC) reduced all the effects of intestinal injury seen in IR. In an effort to investigate the molecular mechanisms responsible for the protective effects afforded by IPC, we sought to characterize the global gene expression pattern in rats subjected to IPC in the setting of IR injury.Rats were randomized into five groups: (1) Sham, (2) IPC only (3) IR, (4) Early IPC + IR (IPC --IR), and (5) Late IPC + IR (IPC --24 h --IR). At 6 h after reperfusion, ileum was harvested for total RNA isolation, pooled, and analyzed on complementary DNA (cDNA) microarrays with validation using real-time polymerase chain reaction (PCR). Significance Analysis of Microarray (SAM) software was used to determine statistically significant changes in gene expression.Early IPC + IR had 5,167 induced and 4 repressed genes compared with the other groups. SAM analysis revealed 474 out of 10,000 genes differentially expressed among the groups. Early and Late IPC + IR had more genes involved in redox hemostasis, the immune/inflammatory response, and apoptosis than either the IPC only or IR alone groups.The transcriptional profile suggests that IPC exerts its protective effects by regulating the gene response to injury in the intestine.

Published
2009
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5. Intestinal Edema: Effect of Enteral Feeding on Motility and Gene Expression

Author

Stacey D. Moore-Olufemi, Hasen Xue, Glen A. Laine, Frederick A. Moore, Randy Stewart, S.J. Allen, Dwight H Oliver, Charles S. Cox, Ravi S. Radhakrishnan, Shodimu Emmanuel Olufemi, and Jeff Padalecki

Subjects
Male, medicine.medical_specialty, Apoptosis, Ileum, Biology, Inflammatory bowel disease, Enteral administration, Gastroenterology, Article, Rats, Sprague-Dawley, Enteral Nutrition, Internal medicine, Edema, Gene expression, medicine, Animals, Intestinal Mucosa, Cytoskeleton, Oligonucleotide Array Sequence Analysis, Regulation of gene expression, Gene Expression Profiling, Dextrans, medicine.disease, Actin cytoskeleton, Actins, Rats, Intestines, Disease Models, Animal, Intestinal Diseases, medicine.anatomical_structure, Endocrinology, Parenteral nutrition, Gene Expression Regulation, Surgery, medicine.symptom, Gastrointestinal Motility, Fluorescein-5-isothiocyanate, Signal Transduction
Abstract

Objective Edema formation, inflammation, and ileus in the intestine are commonly seen in conditions like gastroschisis, inflammatory bowel disease, and cirrhosis. We hypothesized that early enteral feeding would improve intestinal transit. We also wanted to study the impact of early enteral feeding on global gene expression in the intestine. Design Rats were divided into Sham or Edema ± immediate enteral nutrition (IEN). At 12 h, small intestinal transit via FITC-Dextran and tissue water were measured. Ileum was harvested for total RNA to analyze gene expression using cDNA microarray with validation using real-time PCR. Data are expressed as mean ± SEM, n = 4–6 and ∗, ∗∗ = P Results IEN markedly improved intestinal transit with minimal genetic alterations in Edema animals. Major alterations in gene expression were detected in primary, cellular and macromolecular metabolic activities. Edema also altered more genes involved with the regulation of the actin cytoskeleton. Conclusions Intestinal edema results in impaired small intestinal transit and globally increased gene expression. Early enteral nutrition improves edema-induced impaired transit and minimizes gene transcriptional activity.

Published
2009
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6. Common ancestral mutations in theMEN1 gene is likely responsible for the prolactinoma variant of MEN1 (MEN1Burin) in four kindreds from Newfoundland

Author

Shodimu Emmanuel Olufemi, Allen M. Spiegel, Francis S. Collins, Sunita K. Agarwal, Settara C. Chandrasekharappa, Stephen J. Marx, A. Lee Burns, Jane Green, Qihan Dong, Siradanahalli C. Guru, Mary Beth Kester, and Pachiappan Manickam

Subjects
Genetics, Haplotype, Nonsense mutation, Locus (genetics), Biology, medicine.disease, Genetic marker, medicine, MEN1, Multiple endocrine neoplasia, Genetics (clinical), Prolactinoma, Founder effect
Abstract

Familial multiple endocrine neoplasia type 1 (MEN1) is an autosomal dominant disorder with affected individuals developing parathyroid, gastrointestinal (GI) endocrine, and anterior pituitary tumors. Four large kindreds from the Burin peninsula/Fortune Bay area of Newfoundland with prominent features of prolactinomas, carcinoids, and parathyroid tumors (referred to as MEN1Burin) have been described, and they show linkage to 11q13, the same locus as that of MEN1. Haplotype analysis with 16 polymorphic markers now reveals that representative affected individuals from all four families share a common haplotype over a 2.5 Mb region. A nonsense mutation in the MEN1 gene has been found to be responsible for the disease in the affected members in all four of the MEN1Burin families, providing convincing evidence of a common founder. Hum Mutat 11:264–269, 1998. Published 1998 Wiley-Liss, Inc.

Published
1998
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8. A Transcript Map for the 2.8-Mb Region Containing the Multiple Endocrine Neoplasia Type 1 Locus

Author

Lance A. Liotta, Francis S. Collins, Burns Lee, Bruce A. Roe, Settara C. Chandrasekharappa, Pachiappan Manickam, Siradanahalli C. Guru, Yingping Wang, Shodimu Emmanuel Olufemi, Allen M. Spiegel, Jane M. Weisemann, Sunita K. Agarwal, Young Sik Kim, Mark S. Boguski, Michael R. Emmert-Buck, Stephen J. Marx, Mary Beth Kester, and Judy S. Crabtree

Subjects
Genetics, Transcription, Genetic, Tumor suppressor gene, Genetic Linkage, Genome, Human, Chromosomes, Human, Pair 11, Molecular Sequence Data, Chromosome Mapping, Locus (genetics), Biology, medicine.disease, Molecular biology, Paraspeckles, Loss of heterozygosity, Multiple Endocrine Neoplasia Type 1, Mutation testing, medicine, Humans, MEN1, Letters, Multiple endocrine neoplasia, Gene, Genetics (clinical)
Abstract

Multiple endocrine neoplasia type 1 (MEN 1) is an inherited cancer syndrome in which affected individuals develop multiple parathyroid, enteropancreatic, and pituitary tumors. The locus for MEN1 is tightly linked to the marker PYGM on chromosome 11q13, and linkage analysis places the MEN1 gene within a 2-Mb interval flanked by the markers D11S1883 and D11S449. Loss of heterozygosity studies in MEN 1 and sporadic tumors suggest that theMEN1 gene encodes a tumor suppressor and have helped to narrow the location of the gene to a 600-kb interval between PYGM andD11S449. Focusing on this smaller MEN1 interval, we have identified and mapped 12 transcripts to this 600-kb region. A precise ordered map of 33 transcripts, including 12 genes known to map to this region, was generated for the 2.8-Mb D11S480–D11S913interval. Fifteen candidate genes (of which 10 were examined exhaustively) were evaluated by Southern blot and/or dideoxy fingerprinting analysis to identify the gene harboring disease-causing mutations.[The sequence data described in this paper have been submitted to GenBank under accession nos. EST06996, U93236,AF001540–AF001547, AF001433–AF001436, AF001891–AF001893,N55476, R19205, and W37647 (see Table 1 for listing of transcripts). The BAC clone sequences have been submitted to GenBank under accession nos. AC000134, AC000159, and AC000353.]

Published
1997
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9. Genetic mapping of a third Li-Fraumeni syndrome predisposition locus to human chromosome 1q23

Author

Linda L. Bachinski, Shodimu-Emmanuel Olufemi, Xiaojun Zhou, Chih-Chieh Wu, Linwah Yip, Sanjay Shete, Guillermina Lozano, Christopher I. Amos, Louise C. Strong, and Ralf Krahe

Subjects
Male, Cancer Research, Genetic Linkage, Chromosome Mapping, Protein Serine-Threonine Kinases, Genes, p53, Pedigree, Li-Fraumeni Syndrome, Checkpoint Kinase 2, Oncology, Chromosomes, Human, Pair 1, Humans, Female, Genetic Predisposition to Disease
Abstract

Li-Fraumeni syndrome (LFS) is a clinically and genetically heterogeneous inherited cancer syndrome. Most cases (∼70%) identified and characterized to date are associated with dominantly inherited germ line mutations in the tumor suppressor gene TP53 (p53) in chromosome 17p13.1. In a subset of non-p53 patients with LFS, CHEK2 in chromosome 22q11 has been identified as another predisposing locus. Studying a series of non-p53 LFS kindred, we have shown that there is additional genetic heterogeneity in LFS kindred with inherited predisposition at loci other than p53 or CHEK2. Using a genome-wide scan for linkage with complementing parametric and nonparametric analysis methods, we identified linkage to a region of approximately 4 cM in chromosome 1q23, a genomic region not previously implicated in this disease. Identification ofa third predisposing gene and its underlying mutation(s) should provide insight into other genetic events that predispose to the genesis of the diverse tumor types associated with LFS and its variants.

Published
2005

10. 11q13 allelotype analysis in 27 northern American MEN1 kindreds identifies two distinct founder chromosomes

Author

Sunita K. Agarwal, Stephen J. Marx, Larisa V. Debelenko, Mary Beth Kester, A. Lee Burns, Michael R. Emmert-Buck, Irina A. Lubensky, Shodimu Emmanuel Olufemi, Allen M. Spiegel, Lance A. Liotta, Francis S. Collins, Zhengping Zhuang, Siradanahalli C. Guru, Settara C. Chandrasekharappa, Monica C. Skarulis, and Pachiappan Manickam

Subjects
Genetic Markers, Linkage disequilibrium, endocrine system diseases, Endocrinology, Diabetes and Metabolism, Biology, Biochemistry, Polymerase Chain Reaction, Allelotype Analysis, Endocrinology, Genetics, Multiple Endocrine Neoplasia Type 1, Humans, MEN1, Allele, Molecular Biology, Alleles, Polymorphism, Genetic, Chromosomes, Human, Pair 11, Haplotype, Phenotype, Founder Effect, Pedigree, Haplotypes, North America, Allelic loss
Abstract

We analyzed constitutional and tumor DNA from 27 MEN1 kindreds not known to be related to each other. Disease allele haplotypes were constructed for each pedigree based on shared alleles from two or more affected members and from determination of allelic loss patterns in their tumors. Analysis of disease allele haplotypes showed unexpected linkage disequilibrium at marker PYGM. Further haplotype analysis indicated this could be explained by the presence of two founder chromosomes, one in four families, the other in three. A shared disease haplotype was not observed among two MEN1 kindreds with the prolactinoma phenotype of MEN1.

Published
1998

11. G.P.14.14 Differences in aberrant expression and splicing of genes involved in Ca2+ metabolism between myotonic dystrophy type 2 (DM2) and type 1 (DM1)

Author

Olayinka Raheem, Linda L. Bachinski, Shodimu Emmanuel Olufemi, Mario Sirito, Ralf Krahe, Anna Vihola, B. Udd, and Tiina Suominen

Subjects
Genetics, 0303 health sciences, Myotonic dystrophy type 2, Metabolism, Biology, 03 medical and health sciences, 0302 clinical medicine, Neurology, Pediatrics, Perinatology and Child Health, RNA splicing, Neurology (clinical), Gene, 030217 neurology & neurosurgery, Genetics (clinical), 030304 developmental biology
Published
2007
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