Your search keyword '"Higgs D"' showing total 921 results

501. Comparison of the human and murine ATRX gene identifies highly conserved, functionally important domains.

Author

Picketts DJ, Tastan AO, Higgs DR, and Gibbons RJ

Subjects

Adenosine Triphosphatases genetics, Alternative Splicing, Animals, DNA Helicases genetics, DNA-Binding Proteins chemistry, Humans, Mice, Molecular Sequence Data, Multigene Family, Protein Structure, Tertiary, Transcription Factors chemistry, X-linked Nuclear Protein, Conserved Sequence, DNA-Binding Proteins genetics, Nuclear Proteins, Transcription Factors genetics

Published

1998

502. Understanding alpha globin gene expression: a step towards effective gene therapy.

Author

Higgs DR, Sharpe JA, and Wood WG

Subjects

Animals, Chromosome Mapping, Disease Models, Animal, Humans, Mice, Mice, Transgenic, Multigene Family, Mutation, Gene Expression, Genetic Therapy, Globins genetics, alpha-Thalassemia therapy

Abstract

During the past 20 years developments in molecular and cellular biology have kindled the hope that one might eventually ameliorate or even cure some serious genetic diseases by repairing or replacing the defective gene. Other articles deal with the formidable problems of isolating pluripotent hematopoietic stem cells; efficiently, safely, and stably transfecting them, and developing transplantation protocols to ensure that the corrected cells supplant the patient's abnormal stem cells after transplantation. Assuming that these hurdles can be overcome, it will also be important to establish the ideal segment of DNA to introduce into stem cells to ensure that, regardless of its position of integration in the genome, the gene in question will be appropriately regulated. In the case of the globin genes this is a particularly difficult task because in order to correct disorders of globin synthesis we need to obtain high levels of stable, tissue- and developmental-stage specific expression. Issues relevant to this problem arising from the analysis of the human beta globin cluster are discussed in the article in this issue by Grosveld. In this article we review our current understanding of how eukaryotic genes might be expressed from their normal chromosomal environment, using the human alpha globin cluster as a specific example. We also discuss how this information might be used in the development of strategies for gene therapy.

Published

1998

503. Chromosomal location and tissue expression of the gene encoding the adenovirus E1A-regulated transcription factor E4F in humans and mice.

Author

Rooney RJ, Daniels RR, Jenkins NA, Gilbert DJ, Rothammer K, Morris SW, Higgs DR, and Copeland NG

Subjects

Animals, Crosses, Genetic, Humans, Hybrid Cells, Mice, Mice, Inbred C57BL, Adenovirus E1A Proteins physiology, Adenovirus E4 Proteins genetics, Chromosome Mapping, Gene Expression Regulation physiology

Published

1998

504. Mutations in transcriptional regulator ATRX establish the functional significance of a PHD-like domain.

Author

Gibbons RJ, Bachoo S, Picketts DJ, Aftimos S, Asenbauer B, Bergoffen J, Berry SA, Dahl N, Fryer A, Keppler K, Kurosawa K, Levin ML, Masuno M, Neri G, Pierpont ME, Slaney SF, and Higgs DR

Subjects

Amino Acid Sequence, Animals, Conserved Sequence, Globins genetics, Humans, Intellectual Disability genetics, Mice, Molecular Sequence Data, Phenotype, Sequence Homology, Amino Acid, Syndrome, X-linked Nuclear Protein, Zinc Fingers genetics, alpha-Thalassemia genetics, DNA Helicases, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, Mutation, Nuclear Proteins, Transcription Factors chemistry, Transcription Factors genetics

Published

1997

505. Sequence comparison of human and yeast telomeres identifies structurally distinct subtelomeric domains.

Author

Flint J, Bates GP, Clark K, Dorman A, Willingham D, Roe BA, Micklem G, Higgs DR, and Louis EJ

Subjects

Base Sequence, Chromosomes, Artificial, Yeast, Humans, Molecular Sequence Data, Saccharomyces cerevisiae genetics, Telomere

Abstract

We have sequenced and compared DNA from the ends of three human chromosomes: 4p, 16p and 22q. In all cases the pro-terminal regions are subdivided by degenerate (TTAGGG)n repeats into distal and proximal sub-domains with entirely different patterns of homology to other chromosome ends. The distal regions contain numerous, short (<2 kb) segments of interrupted homology to many other human telomeric regions. The proximal regions show much longer (approximately 10-40 kb) uninterrupted homology to a few chromosome ends. A comparison of all yeast subtelomeric regions indicates that they too are subdivided by degenerate TTAGGG repeats into distal and proximal sub-domains with similarly different patterns of identity to other non-homologous chromosome ends. Sequence comparisons indicate that the distal and proximal sub-domains do not interact with each other and that they interact quite differently with the corresponding regions on other, non-homologous, chromosomes. These findings suggest that the degenerate TTAGGG repeats identify a previously unrecognized, evolutionarily conserved boundary between remarkably different subtelomeric domains.

Published

1997

506. Pulse oximetry in a cohort study of sickle cell disease.

Author

Homi J, Levee L, Higgs D, Thomas P, and Serjeant G

Subjects

Adolescent, Age Factors, Cerebrovascular Disorders blood, Cerebrovascular Disorders metabolism, Chest Pain blood, Chest Pain metabolism, Child, Cohort Studies, Female, Genotype, Growth physiology, Humans, Intelligence Tests, Male, Oxygen administration & dosage, Oxygen blood, Reference Values, Reproducibility of Results, Severity of Illness Index, Sex Factors, Anemia, Sickle Cell blood, Anemia, Sickle Cell metabolism, Oximetry standards, Oximetry statistics & numerical data

Abstract

Oxygen saturation was determined by pulse oximetry in a representative sample of Jamaican patients with steady-state sickle cell disease in a cohort study from birth. There were 220 with homozygous sickle cell (SS) disease and 142 with sickle cell-haemoglobin C (SC) disease aged 9-18 years, and 122 with a normal haemoglobin (AA) genotype aged 15-18 years. Pulse oximetry (SpO2) values were lower in SS disease (mean [95% confidence interval], 92.5 [92.0-93.0]) than in SC disease (96.7[96.5-96.9]) or AA controls (97.1 [96.8-97.3]). Inhalation of 100% oxygen in SS patients with O2 saturations below 90% consistently increased saturation to 99-100%. In SS disease, SpO2 correlated positively with haemoglobin and fetal haemoglobin and negatively with reticulocyte counts but not with MCHC, MCV or bilirubin level. Mean SpO2 in SS subjects with a normal alpha globin gene complement (mean [SD], 91.7 [3.9]%) was lower than in heterozygotes (93.4 [4.0]%) or homozygotes (96.1 [3.0]%) for alpha+ thalassaemia, the effects of alpha-thalassaemia not being explained by differences in haemoglobin or MCHC. In SS disease, SpO2 levels were not associated with age (within this age range), sex, number of sick clinic visits or number of hospital admissions. Higher SpO2 levels were associated with greater height and weight, more frequent painful crises and less frequent acute chest syndrome, but these associations were not significant after adjustment for haemoglobin level. Desaturation is common in steady-state SS disease and knowledge of the individual's steady-state value may be important in the interpreting low values during acute complications.

Published

1997

507. The relationship between chromosome structure and function at a human telomeric region.

Author

Flint J, Thomas K, Micklem G, Raynham H, Clark K, Doggett NA, King A, and Higgs DR

Subjects

Base Sequence, Chromosome Mapping, DNA chemistry, DNA genetics, Deoxyribonuclease I, Dinucleotide Repeats, Genetic Markers, Humans, Minisatellite Repeats, Molecular Sequence Data, Polymerase Chain Reaction, RNA, Messenger biosynthesis, Transcription, Genetic, Chromosomes, Human, Pair 16, Repetitive Sequences, Nucleic Acid, Telomere

Abstract

We have sequenced a contiguous 284,495-bp segment of DNA extending from the terminal (TTAGGG)n repeats of the short arm of chromosome 16, providing a full description of the transition from telomeric through subtelomeric DNA to sequences that are unique to the chromosome. To complement and extend analysis of the primary sequence, we have characterized mRNA transcripts, patterns of DNA methylation and DNase I sensitivity. Together with previous data these studies describe in detail the structural and functional organization of a human telomeric region.

Published

1997

508. Benign clinical course in homozygous sickle cell disease: a search for predictors.

Author

Thomas PW, Higgs DR, and Serjeant GR

Subjects

Adolescent, Child, Child, Preschool, Cohort Studies, Fetal Hemoglobin analysis, Gene Deletion, Globins analysis, Homozygote, Humans, Infant, Infant, Newborn, Jamaica epidemiology, Prognosis, Social Class, Sickle Cell Trait epidemiology, Sickle Cell Trait genetics

Abstract

Aims: (1) To estimate the proportion of subjects with homozygous sickle cell disease who have a benign clinical course, and (2) to assess factors that may be predictive of benign disease., Material: Subjects (n = 280) were participants in a longitudinal cohort study of sickle cell disease. They were classified as benign or control based on clinical history from birth to age 13 years old. Associations with growth, hematology, and an index of social status were investigated., Results: Benign disease occurred in 43 (15%) patients. Neither growth nor social status were related to benign disease. There were only two statistically independent associations: alpha thalassemia status and average steady state fetal hemoglobin (HbF). Patients with a normal complement of alpha globin genes were 2.2 (1.0, 4.9) times more likely to have benign disease than those with gene deletion, and were less likely to have frequent painful crises, dactylitis, and bone necrosis. The odds of having benign disease were 1.09 (1.02, 1.17) times higher for each unit increase in HbF, and 44% of subjects with HbF in the top decile (HbF > 13.8%) of the distribution had benign disease. There was no evidence for a threshold effect of high HbF on benign disease., Conclusion: A benign clinical course of sickle cell disease may occur in Jamaica and is associated with a normal alpha globin gene complement, and high levels of HhF. Ability to predict benign disease at birth is limited.

Published

1997

509. ATRX encodes a novel member of the SNF2 family of proteins: mutations point to a common mechanism underlying the ATR-X syndrome.

Author

Picketts DJ, Higgs DR, Bachoo S, Blake DJ, Quarrell OW, and Gibbons RJ

Subjects

Amino Acid Sequence, Female, Gene Expression Regulation, Humans, Male, Molecular Sequence Data, Mutation, Syndrome, X-linked Nuclear Protein, DNA Helicases, DNA-Binding Proteins genetics, Intellectual Disability genetics, Nuclear Proteins, Transcription Factors genetics, alpha-Thalassemia genetics

Abstract

It was shown recently that mutations of the ATRX gene give rise to a severe, X-linked form of syndromal mental retardation associated with alpha thalassaemia (ATR-X syndrome). In this study, we have characterised the full-length cDNA and predicted structure of the ATRX protein. Comparative analysis shows that it is an entirely new member of the SNF2 subgroup of a superfamily of proteins with similar ATPase and helicase domains. ATRX probably acts as a regulator of gene expression. Definition of its genomic structure enabled us to identify four novel splicing defects by screening 52 affected individuals. Correlation between these and previously identified mutations with variations in the ATR-X phenotype provides insights into the pathophysiology of this disease and the normal role of the ATRX protein in vivo.

Published

1996

510. Chromosomal stabilisation by a subtelomeric rearrangement involving two closely related Alu elements.

Author

Flint J, Rochette J, Craddock CF, Dodé C, Vignes B, Horsley SW, Kearney L, Buckle VJ, Ayyub H, and Higgs DR

Subjects

Adolescent, Adult, Alleles, Base Sequence, Chromosome Mapping, Chromosomes, Human, Pair 16 ultrastructure, DNA genetics, DNA Primers genetics, Female, Gene Rearrangement, Genotype, Globins genetics, Haplotypes, Humans, In Situ Hybridization, Fluorescence, Male, Middle Aged, Molecular Sequence Data, Multigene Family, Polymerase Chain Reaction, Recombination, Genetic, Sequence Homology, Nucleic Acid, Telomere genetics, Telomere ultrastructure, Chromosomes, Human, Pair 16 genetics, Repetitive Sequences, Nucleic Acid, alpha-Thalassemia genetics

Abstract

We have characterised a subtelomeric rearrangement involving the short arm of chromosome 16 that gives rise to alpha-thalassaemia by deleting the major, remote regulatory element controlling alpha-globin expression. The chromosomal breakpoint lies in an Alu family repeat located only approximately 105 kb from the 16p subtelomeric region. The broken chromosome has been stabilised with a newly positioned telomere acquired by recombination between this 16p Alu element and a closely related subtelomeric Alu element of the Sx subfamily. It seems most likely that this abnormal chromosome has been rescued by the mechanism of telomere capture which may reflect a more general process by which subtelomeric sequences are normally dispersed between chromosomal ends.

Published

1996

511. Factors affecting prepubertal growth in homozygous sickle cell disease.

Author

Singhal A, Morris J, Thomas P, Dover G, Higgs D, and Serjeant G

Subjects

Anemia, Sickle Cell blood, Body Height physiology, Body Weight physiology, Cohort Studies, Female, Fetal Hemoglobin analysis, Homozygote, Humans, Infant, Newborn, Male, Sex Factors, Social Class, Anemia, Sickle Cell physiopathology, Growth physiology, Hemoglobins analysis

Abstract

Objective: To investigate the role of haematological indices, socioeconomic status, and morbidity in prepubertal growth in homozygous sickle cell (SS) disease., Method: Height, weight, and haematology were serially recorded in a cohort study of 315 children with SS disease from birth to 9 years at the sickle cell clinic of the University Hospital of the West Indies, Kingston, Jamaica., Results: Height increment between 3 and 9 years correlated positively with total haemoglobin at age 7 years in boys but not girls. Attained height and weight at age 7 years correlated positively with haemoglobin and fetal haemoglobin in boys but not girls. Only the correlation between haemoglobin and weight showed a significant gender difference. Partial correlation analysis suggested that the effect of haemoglobin was accounted for by the effect of fetal haemolglobin and further analysis indicated that height correlated with F reticulocyte count (a measure of fetal haemoglobin production) in both sexes but not with the ratio of F cells to F reticulocytes (a measure of F cell enrichment). Growth was not significantly related to mean red cell volume, proportional reticulocyte count, alpha thalassaemia, socioeconomic status, or morbidity., Conclusion: A high concentration of fetal haemoglobin in boys with SS disease is associated with greater linear growth. It is postulated that in boys, low concentrations of fetal haemoglobin increase haemolysis and hence metabolic requirements for erythropoiesis, putting them at greater risk of poor growth. Differences in the relationship of haematology and growth between boys and girls with SS disease dictate that future analyses of growth take gender into account.

Published

1996

512. The genetic basis for mental retardation.

Author

Raynham H, Gibbons R, Flint J, and Higgs D

Subjects

Gene Deletion, Humans, Intellectual Disability epidemiology, Prevalence, Chromosome Aberrations epidemiology, Chromosome Aberrations genetics, Chromosome Disorders, Intellectual Disability genetics, Intelligence genetics

Published

1996

513. The alpha-thalassemia/mental retardation syndromes.

Author

Gibbons RJ and Higgs DR

Subjects

Chromosome Disorders, Chromosome Mapping, Gene Deletion, Humans, Mutation, Pedigree, Sex Chromosome Aberrations genetics, Syndrome, Transcription, Genetic, Translocation, Genetic, Chromosome Aberrations genetics, Chromosomes, Human, Pair 16, Intellectual Disability genetics, X Chromosome, alpha-Thalassemia genetics

Abstract

The chromosome-16 and the X-chromosome forms of alpha-thalassemia--ATR-16 and ATR-X--exemplify 2 important causes of syndromal mental retardation. ATR-16 is a contiguous gene syndrome which arises from loss of DNA from the tip of chromosome 16p13.3 by truncation, interstitial deletion, or unbalanced translocation. It provided the first example of a chromosome translocation that could be detected by molecular analysis but not conventional cytogenetics. It also provided the first example of a telomeric truncation giving rise to a complex genetic syndrome. In contrast ATR-X appears to be due to mutations in a trans-acting factor that regulates gene expression. Mutations in transcription factors have recently been identified in a number of genetic diseases (for example, Denys-Drash syndrome, WT1 [19]; pituitary dwarfism, PIT1 [16]; Rubinstein-Taybi syndrome, CBP [20]. Not only is this mechanism proving to be an important cause of complex syndromes but it is providing new perspectives on certain developmental pathways. XH2 may not be a classical transcription factor but it is certainly involved in the regulation of gene expression, exerting its effects on several different genes. It seems likely that other mutations in this class of regulatory proteins will be found in patients with complex disorders including mental retardation. In broader terms the 2 mechanisms described here may prove to be responsible for a significant proportion of mental retardation. However, without a feature such as alpha-thalassemia to pinpoint the area of genome or pathways involved it may prove difficult to identify other, similarly affected genes underlying other forms of mental retardation. As the human genome project and rapid genome analysis evolve this problem should become less of an obstacle. In the meantime, it is very worthwhile to continue looking for unusual clinical associations that may point to critical genes underlying human genetic disorders.

Published

1996

514. Ontogeny of visual and mechanosensory structure and function in Atlantic menhaden Brevoortia tyrannus

Author

Higgs D and Fuiman L

Abstract

The importance of visual, mechanoreceptive and auditory inputs to escape responses was examined in larvae of the Atlantic menhaden (Brevoortia tyrannus) presented with a simulated predatory stimulus. Ontogenetic changes in the retina, superficial neuromasts and auditory bullae were examined in concert with behavioral trials in which sensory inputs were selectively blocked. Menhaden larvae showed a decrease in cone photoreceptor density and first developed rod photoreceptors when their total length (TL) reached 8&shy;10 mm; they began summing photoreceptive inputs at 12&shy;14 mm TL. Inflation of the auditory bullae was complete by 15 mm TL. The proliferation of superficial neuromasts varied depending on their location, with cephalic superficial neuromasts decreasing in number beginning at 19 mm TL and numbers of trunk neuromasts continuing to increase throughout the larval period. In behavioral trials, responsiveness and the reactive distance to the approaching probe increased with increasing larva total length when all sensory inputs were available (control larvae). When visual inputs were blocked, responsiveness was lower than in control larvae, but still increased ontogenetically, while reactive distance showed no difference between control larvae and those lacking visual information. When neuromasts were ablated, ontogenetic increases in responsiveness and reactive distance were absent. Inflation of the auditory bullae had no discernible effect on behavior. The anatomical and behavioral results suggest that both vision and mechanoreception are used to trigger a response to a looming predatory stimulus and that mechanoreception, but not vision, contributes to the timing of the response. Ontogenetic improvements in performance are attributed mainly to neuromast proliferation and not to ontogenetic changes in the retina.

Published

1996

515. Determinants of haemoglobin level in steady-state homozygous sickle cell disease.

Author

Serjeant G, Serjeant B, Stephens A, Roper D, Higgs D, Beckford M, Cook J, and Thomas P

Subjects

Adult, Blood Volume, Erythrocyte Aging, Erythrocyte Indices, Female, Fetal Hemoglobin analysis, Humans, Iron blood, Male, Reticulocyte Count, Transferrin analysis, alpha-Thalassemia blood, Anemia, Sickle Cell blood, Hemoglobins analysis

Abstract

High total haemoglobin levels in homozygous sickle cell (SS) disease are a risk factor for painful crises, avascular necrosis of the femoral head, proliferative sickle retinopathy, and the acute chest syndrome. Since lowering the haemoglobin level may ameliorate these features, understanding the determinants of total haemoglobin may be of practical importance. A range of possible determinants including red cell characteristics, reticulocytes, serum iron, transferrin saturation, serum ferritin, alpha thalassaemia status, red cell mass and plasma volume, oxygen affinity, red cell survival, transferrin receptor and erythropoietin levels have been measured in 62 patients selected to provide a range of total haemoglobin and fetal haemoglobin levels. There were weak negative associations of haemoglobin with mean cell volume and mean cell haemoglobin concentration, strong negative associations with proportional reticulocyte counts, oxygen affinity, plasma volume, serum transferrin receptors, and erythropoietin levels and strong positive associations with red cell mass. Weighted analysis suggested that the statistically independent determinants of haemoglobin level were alpha thalassaemia, sex, red cell mass/body weight, plasma volume/body weight, fetal haemoglobin, and red cell count. The apparent contributions of red cell survival, P50, reticulocyte count, serum transferrin receptor and erythropoietin levels were explained by the effects of these other variables. The independent determinants as a group explained 91% of the variation in haemoglobin level.

Published

1996

516. Conservation of position and sequence of a novel, widely expressed gene containing the major human alpha-globin regulatory element.

Author

Vyas P, Vickers MA, Picketts DJ, and Higgs DR

Subjects

Amino Acid Sequence, Animals, Base Composition, Base Sequence, Birds, Cell Line, Chickens, Conserved Sequence, DNA Primers, DNA, Complementary, Exons, Globins biosynthesis, Humans, Introns, Mammals, Molecular Sequence Data, Polymerase Chain Reaction, Recombinant Proteins biosynthesis, Sequence Homology, Nucleic Acid, TATA Box, Transfection, Tumor Cells, Cultured, Biological Evolution, Gene Expression Regulation, Globins genetics, Multigene Family, Promoter Regions, Genetic, Regulatory Sequences, Nucleic Acid

Abstract

We have determined the cDNA and genomic structure of a gene (-14 gene) that lies adjacent to the human alpha-globin cluster. Although it is expressed in a wide range of cell lines and tissues, a previously described erythroid-specific regulatory element that controls expression of the alpha-globin genes lies within intron 5 of this gene. Analysis of the -14 gene promoter shows that it is GC rich and associated with a constitutively expressed DNase 1 hypersensitive site; unlike the alpha-globin promoter, it does not contain a TATA or CCAAT box. These and other differences in promoter structure may explain why the erythroid regulatory element interacts specifically with the alpha-globin promoters and not the -14 gene promoter, which lies between the alpha promoters and their regulatory element. Interspecies comparisons demonstrate that the sequence and location of the -14 gene adjacent to the alpha cluster have been maintained since the bird/mammal divergence, 270 million years ago.

Published

1995

517. Abundance and half-life of the distinct oat phytochrome A3 and A4 mRNAs.

Author

Higgs DC, Barnes LJ, and Colbert JT

Subjects

Avena radiation effects, Base Sequence, Conserved Sequence, Half-Life, Light, Molecular Sequence Data, Oligonucleotide Probes, Phytochrome A, Poaceae genetics, RNA, Messenger analysis, RNA, Messenger genetics, Sequence Homology, Nucleic Acid, Transcription, Genetic radiation effects, Avena genetics, Phytochrome genetics, RNA, Messenger metabolism

Abstract

Gene-preferential oligonucleotide probes were used to determined the relative abundance and half-lives of distinct oat phytochrome A (PHYA) mRNAs. Oat PHYA mRNAs are highly conserved in the 5'-untranslated region and the coding region, but the 3'-untranslated region has an overall lower sequence conservation and was the source of gene-preferential probes. PHYA3 mRNA was estimated to be ca. 61% of the oat PHYA mRNA pool present in poly(A)+ RNA from dark-grown seedlings. The half-lives for PHYA3 and PHYA4 mRNAs were both estimated to be ca. 30 min, and a similar short half-life was estimated for the average PHYA mRNA. Sequence comparisons of PHYA mRNAs from four grass species identified conserved sequences within the 5'- and 3'-untranslated regions that might be important for PHYA mRNA degradation.

Published

1995

518. The IL-9 receptor gene (IL9R): genomic structure, chromosomal localization in the pseudoautosomal region of the long arm of the sex chromosomes, and identification of IL9R pseudogenes at 9qter, 10pter, 16pter, and 18pter.

Author

Kermouni A, Van Roost E, Arden KC, Vermeesch JR, Weiss S, Godelaine D, Flint J, Lurquin C, Szikora JP, and Higgs DR

Subjects

Alternative Splicing, Base Sequence, Cell Line, Chromosome Mapping, Chromosomes, Human, Pair 10, Chromosomes, Human, Pair 16, Chromosomes, Human, Pair 18, Chromosomes, Human, Pair 9, Cloning, Molecular, DNA, Neoplasm genetics, DNA, Neoplasm isolation & purification, Exons, Humans, In Situ Hybridization, Fluorescence, Introns, Molecular Sequence Data, RNA, Messenger biosynthesis, Random Amplified Polymorphic DNA Technique, Receptors, Interleukin biosynthesis, Receptors, Interleukin-9, Recombinant Proteins biosynthesis, Tumor Cells, Cultured, Pseudogenes, Receptors, Interleukin genetics, X Chromosome, Y Chromosome

Abstract

Cosmids containing the human IL-9 receptor (R) gene (IL9R) have been isolated from a genomic library using the IL9R cDNA as a probe. We have shown that the human IL9R cDNA as a probe. We have shown that hte human IL9R gene is composed of 11 exons and 10 introns, stretching over approximately 17 kb, and is located within the pseudoautosomal region of the Xq and Yq chromosome, in the vicinity of the telomere. Analysis f the 5' flanking region revealed multiple transcription initiation sites as well as potential binding motifs for AP1, AP2, AP3, Sp1, and NF-kB, although this region lacks a TATA box. Using the human IL9R cosmid as a probe to perform fluorescence in situ hybridization, additional signals were identified in the subtelomeric regions of chromosomes 9q, 10p, 16p, and 18p. IL9R homologs located on chromosomes 16 and 10 were completely sequenced. Although they are similar to the IL9R gene (approximately 90% identity), none of these copies encodes a functional receptor: none of them contains sequences homologous to the 5' flanking region or exon 1 of the IL9R gene, and the remaining ORFs have been inactivated by various point mutations and deletions. Taken together, our results indicate that the IL9R gene is located at Xq28 and Yq12, in the long arm pseudoautosomal region, and that four IL9R pseudogenes are located on 9q34, 10p15, 16p13.3, and 18p11.3, probably dispersed as the result of translocations during evolution.

Published

1995

519. Targeted inactivation of the major positive regulatory element (HS-40) of the human alpha-globin gene locus.

Author

Bernet A, Sabatier S, Picketts DJ, Ouazana R, Morlé F, Higgs DR, and Godet J

Subjects

Cell Line, Deoxyribonuclease I, Gene Expression Regulation, Humans, In Vitro Techniques, Mutagenesis, Insertional, RNA, Messenger genetics, Restriction Mapping, Globins genetics, Regulatory Sequences, Nucleic Acid

Abstract

We have examined the role of the major positive upstream regulatory element of the human alpha-globin gene locus (HS-40) in its natural chromosomal context. Using homologous recombination, HS-40 was replaced by a neo marker gene in a mouse erythroleukemia hybrid cell line containing a single copy of human chromosome 16. In clones from which HS-40 had been deleted, human alpha-globin gene expression was severely reduced, although basal levels of alpha 1 and alpha 2-globin mRNA expression representing less than 3% of the level in control cell lines were detected. Deletion of the neo marker gene, by using FLP recombinase/FLP recombinase target system, proved that the phenotype observed was not caused by the regulatory elements of this marker gene. In the targeted clones, deletion of HS-40 apparently does not affect long-range or local chromatin structure at the alpha promoters. Therefore, these results indicate that, in the experimental system used, HS-40 behaves as a strong inducible enhancer of human alpha-globin gene expression.

Published

1995

520. The mouse alpha-globin locus regulatory element.

Author

Gourdon G, Sharpe JA, Higgs DR, and Wood WG

Subjects

Animals, Base Sequence, Cloning, Molecular, Globins biosynthesis, HeLa Cells, Humans, Mice, Transgenic, Molecular Sequence Data, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins genetics, Sequence Alignment, Sequence Homology, Nucleic Acid, Species Specificity, Tumor Cells, Cultured, Gene Expression Regulation, Genes, Globins genetics, Mice genetics, Regulatory Sequences, Nucleic Acid

Abstract

We have identified and cloned the major alpha globin locus regulatory element in the mouse (m alpha RE). This element shows a high level of sequence homology to its human counterpart (HS -40) and lies between the same two exons of an upstream, widely expressed gene in both species. Footprinting and band shift studies of the core element show conservation of many (but not all) of the protein binding sites identified as functionally important in HS -40. The functional equivalence of the mouse element was shown by attaching it to a human alpha globin gene and examining expression in transgenic mice. Readily detectable levels of human alpha mRNA were produced in these mice but they were lower than the endogenous gene expression and did not show copy number dependence. These results suggest that sequences additional to this major regulatory element may be necessary to obtain complete regulation of the alpha globin genes in both species.

Published

1995

521. Contrasting effects of alpha and beta globin regulatory elements on chromatin structure may be related to their different chromosomal environments.

Author

Craddock CF, Vyas P, Sharpe JA, Ayyub H, Wood WG, and Higgs DR

Subjects

Animals, Base Sequence, Chromatin ultrastructure, Chromosomes, Human, Pair 16 ultrastructure, DNA metabolism, Deoxyribonuclease I metabolism, Globins biosynthesis, Humans, Hybrid Cells, Mice, Mice, Transgenic, Molecular Sequence Data, Multigene Family genetics, Promoter Regions, Genetic genetics, Sequence Deletion, Chromatin genetics, Chromosomes, Human, Pair 16 genetics, Gene Expression Regulation, Globins genetics, Regulatory Sequences, Nucleic Acid genetics

Abstract

Expression of the human alpha and beta globin gene clusters is regulated by remote sequences, referred to as HS -40 and the beta-locus control region (beta-LCR) that lie 5-40 kb upstream of the genes they activate. Because of their common ancestry, similar organization and coordinate expression it has often been assumed that regulation of the globin gene clusters by HS -40 and the beta-LCR occurs via similar mechanisms. Using interspecific hybrids containing chromosomes with naturally occurring deletions of HS -40 we have shown that, in contrast to the beta-LCR, this element exerts no discernible effect on long-range chromatin structure and in addition does not influence formation of DNase I hypersensitive sites at the alpha globin promoters. These differences in the behaviour of HS -40 and the beta-LCR may reflect their contrasting influence on gene expression in transgenic mice and may result from the differing requirements of these elements in their radically different, natural chromosomal environments; the alpha cluster lying within a region of constitutively 'open' chromatin and the beta cluster in a segment of chromatin which opens in a tissue-specific manner. Differences in the hierarchical control of the alpha and beta globin clusters may exemplify more general differences in the regulation of eukaryotic genes which lie in similar open or closed chromosomal regions.

Published

1995

522. Mutations in a putative global transcriptional regulator cause X-linked mental retardation with alpha-thalassemia (ATR-X syndrome).

Author

Gibbons RJ, Picketts DJ, Villard L, and Higgs DR

Subjects

Amino Acid Sequence, Base Sequence, Brain metabolism, Chromosome Mapping, Conserved Sequence, DNA Primers, Fetus, Gene Library, Genetic Linkage, Humans, Lod Score, Molecular Sequence Data, Phenotype, Polymerase Chain Reaction, Sequence Homology, Amino Acid, Syndrome, Abnormalities, Multiple genetics, DNA Helicases genetics, DNA Repair, Gene Expression Regulation, Intellectual Disability genetics, Multigene Family, Sequence Deletion, Transcription, Genetic, X Chromosome, alpha-Thalassemia genetics

Abstract

The ATR-X syndrome is an X-linked disorder comprising severe psychomotor retardation, characteristic facial features, genital abnormalities, and alpha-thalassemia. We have shown that ATR-X results from diverse mutations of XH2, a member of a subgroup of the helicase superfamily that includes proteins involved in a wide range of cellular functions, including DNA recombination and repair (RAD16, RAD54, and ERCC6) and regulation of transcription (SW12/SNF2, MOT1, and brahma). The complex ATR-X phenotype suggests that XH2, when mutated, down-regulates expression of several genes, including the alpha-globin genes, indicating that it could be a global transcriptional regulator. In addition to its role in the ATR-X syndrome, XH2 may be a good candidate for other forms of X-linked mental retardation mapping to Xq13.

Published

1995

523. X-linked alpha-thalassemia/mental retardation (ATR-X) syndrome: a new kindred with severe genital anomalies and mild hematologic expression.

Author

McPherson EW, Clemens MM, Gibbons RJ, and Higgs DR

Subjects

Abnormalities, Multiple genetics, Child, Preschool, Dosage Compensation, Genetic, Face abnormalities, Female, Genetic Linkage, Hemoglobin H analysis, Heterozygote, Humans, Male, Middle Aged, Pedigree, Disorders of Sex Development genetics, Intellectual Disability genetics, X Chromosome, alpha-Thalassemia genetics

Abstract

We report a new kindred containing 4 patients with X-linked alpha-thalassemia/mental retardation syndrome ((ATR-X). Like previously reported ATR-X patients, these children are all genetic males with severe developmental delay and characteristic facial appearance. The genital anomalies are more severe than in most previous cases and have led to a female sex of rearing for 3 of the 4 patients. The hematologic expression is extremely mild and was not demonstrable on routine hematologic studies including hemoglobin electrophoresis, but the three living patients all had hemoglobin H inclusions on brilliant cresyl blue stained peripheral smears. The combination of skewed X-inactivation and haplotype analysis at Xq12-q21.3 confirmed carrier status in the 3 obligate carriers in the kindred and led to identification of an additional carrier. Two other women in the kindred appear to be noncarriers on the basis of normal X-inactivation and/or inheritance of a different Xq12-21.3 haplotype. More widespread use of brilliant cresyl blue staining for HbH inclusions in individuals with the facial phenotype of ATR-X and/or ambiguous genitalia may lead to the identification of more affected patients and improved understanding of the clinical spectrum of ATR-X.

Published

1995

524. Syndromal mental retardation due to mutations in a regulator of gene expression.

Author

Gibbons RJ, Picketts DJ, and Higgs DR

Subjects

Child, Chromosome Mapping, Genetic Linkage, Humans, Male, Mutation, Syndrome, Gene Expression Regulation genetics, Intellectual Disability genetics, X Chromosome, alpha-Thalassemia genetics

Abstract

Mental handicap is a common clinical problem that has been a relatively neglected area of research. Though the causes are varied and complex, molecular biologists are making progress in understanding the mechanisms in some cases, particularly where there are distinguishing phenotypic or genetic markers. The fortuitous association of alpha thalassaemia with a form of mental retardation has allowed us to define a specific X-linked syndrome (ATR-X). Positional cloning was used to define a disease interval and examination of candidate genes demonstrated that mutations in a gene, XH2, showing homology to the SNF2 superfamily were responsible for this syndrome. The complex ATR-X phenotype suggests that this gene, when mutated, down-regulates the expression of several genes including the alpha-globin genes indicating that it could be a global transcriptional regulator. It is conceivable that this mechanism is involved in other forms of syndromal mental retardation.

Published

1995

525. Helix pomatia agglutinin binding is a useful prognostic indicator in colorectal carcinoma.

Author

Schumacher U, Higgs D, Loizidou M, Pickering R, Leathem A, and Taylor I

Subjects

Acetylgalactosamine metabolism, Aged, Animals, Binding Sites, Colorectal Neoplasms mortality, Female, Helix, Snails, Humans, Male, Neoplasm Metastasis, Neoplasm Staging, Prognosis, Regression Analysis, Survival Rate, Colorectal Neoplasms metabolism, Colorectal Neoplasms pathology, Lectins metabolism

Abstract

Background: Most deaths from colorectal carcinoma are due to metastases. A relatively reliable prognostic indicator at surgery to date is the Dukes' stage, but this is a morphologic approach that does not elucidate biochemical changes to explain why cells became metastatic. The binding sites for the lectin from the Roman snail Helix pomatia (HPA) were shown to be good prognostic indicators in breast and gastric cancer, and accordingly, this study was performed to evaluate the use of HPA binding sites as prognostic markers in colorectal carcinoma., Methods: The histochemically detected expression of HPA binding sites in colorectal carcinomas (n = 130) was increased. The results of the histochemical findings were correlated with patient survival and tumor recurrence., Results: The results indicated that the prognosis for the groups of patients whose colorectal cancer cells binded to HPA in tissue sections was almost as bad as those with Dukes' Stage C disease., Conclusion: Because HPA binds to N-acetylgalactosamine, the authors' results indicate that this sugar residue is at least partly involved in the process of human colorectal carcinoma cells metastasizing to regional lymph nodes and possibly also to distant sites.

Published

1994

526. Analysis of a 70 kb segment of DNA containing the human zeta and alpha-globin genes linked to their regulatory element (HS-40) in transgenic mice.

Author

Gourdon G, Sharpe JA, Wells D, Wood WG, and Higgs DR

Subjects

Animals, Base Sequence, Chromatin chemistry, Cosmids, DNA chemistry, Deoxyribonuclease EcoRI, Gene Expression, Gene Expression Regulation, Humans, Mice, Mice, Inbred CBA, Mice, Transgenic, Molecular Sequence Data, RNA, Messenger metabolism, DNA metabolism, Globins genetics, Regulatory Sequences, Nucleic Acid

Abstract

We have ligated two cosmids through an oligonucleotide linker to produce a single fragment spanning 70 kb of the human alpha-globin cluster, in which the alpha-like globin genes (zeta 2, alpha 2 and alpha 1), their regulatory element (HS-40) and erythroid-specific DNase I hypersensitive sites accurately retain their normal genomic organization. The zeta (embryonic) and alpha (embryonic, fetal and adult) globin genes were expressed in all 17 transgenic embryos. Similarly, all fetal and adult mice from seven transgenic lines that contained one or more copies of the fragment, produced up to 66% of the level of endogenous mouse alpha-globin mRNA. However, as for smaller constructs containing these elements, human alpha-globin expression was not copy number dependent and decreased by 1.5-9.0 fold during development. These findings suggest that either it is not possible to obtain full regulation of human alpha-globin expression in transgenic mice or, more likely, that additional alpha-globin regulatory elements lie beyond the 70 kb segment of DNA analysed.

Published

1994

527. A mutation in the polyadenylation signal of the alpha 2 globin gene (AATAAA-->AATA--) as a cause of alpha thalassaemia in Asian indians.

Author

Hall GW, Higgs DR, Murphy P, Villegas A, and de Miguel A

Subjects

Adult, Base Sequence, Humans, India epidemiology, Male, Molecular Sequence Data, alpha-Thalassemia ethnology, Globins genetics, Mutation, Poly A genetics, alpha-Thalassemia genetics

Published

1994

528. Healing of broken human chromosomes by the addition of telomeric repeats.

Author

Flint J, Craddock CF, Villegas A, Bentley DP, Williams HJ, Galanello R, Cao A, Wood WG, Ayyub H, and Higgs DR

Subjects

Base Sequence, Chromosome Deletion, DNA Nucleotidylexotransferase biosynthesis, DNA Primers, DNA Replication, DNA, Complementary metabolism, Globins biosynthesis, Globins genetics, Humans, Molecular Sequence Data, Polymerase Chain Reaction, RNA metabolism, Templates, Genetic, alpha-Thalassemia genetics, Chromosomes, Human, Pair 16 enzymology, Chromosomes, Human, Pair 16 physiology, DNA Nucleotidylexotransferase physiology, Repetitive Sequences, Nucleic Acid

Abstract

We have characterized and compared a series of naturally occurring chromosomal truncations involving the terminal region of the short arm of human chromosome 16 (16p13.3). All six broken chromosomes appear to have been stabilized by the direct addition of telomeric repeats (TTAGGG)n to nontelomeric DNA. In five of the six chromosomes, sequence analysis shows that the three of four nucleotides preceding the point of telomere addition are complementary to and in phase with the putative RNA template of human telomerase. Otherwise we have found no common structural features around the breakpoint regions. These findings, together with previously reported in vitro data, suggest that chromosome-healing events in man can be mediated by telomerase and that a small region of complementarity to the RNA template of telomerase at the end of a broken chromosome may be sufficient to prime healing in vivo.

Published

1994

529. Oat phytochrome A mRNA degradation appears to occur via two distinct pathways.

Author

Higgs DC and Colbert JT

Subjects

Base Sequence, Exoribonucleases metabolism, Glucuronidase biosynthesis, Molecular Sequence Data, Oligodeoxyribonucleotides, Phytochrome A, Poly A metabolism, Ribonuclease H metabolism, Edible Grain metabolism, Phytochrome biosynthesis, RNA, Messenger metabolism

Abstract

We have identified possible mechanisms for the degradation of oat phytochrome A (PHYA) mRNA. The majority of PHYA mRNA molecules appeared to be degraded prior to removal of the poly(A) tail, a pathway that differs from that reported for the degradation of other eukaryotic mRNAs. Polyadenylated PHYA mRNA contained a pattern of putative degradation products that is consistent with a 5'-->3' exoribonuclease, although the participation of a stochastic endoribonuclease cannot be excluded. The poly(A) tail of PHYA mRNA was heterogeneous in size and ranged from approximately 14 to 220 nucleotides. Early PHYA mRNA degradation events did not appear to involve site-specific endoribonucleases. Approximately 25% of the apparently full-length PHYA mRNA was poly(A) deficient. Oat H4 histone, beta-tubulin, and actin mRNA populations had lower amounts of apparently full-length mRNAs that were poly(A) deficient. Degradation of the poly(A)-deficient PHYA mRNA, a second pathway, appeared to be initiated by a 3'-->5' exoribonucleolytic removal of the poly(A) tail followed by both 5'-->3' and 3'-->5' exoribonuclease activities. Polysome-associated RNA contained putative PHYA mRNA degradation products and was a mixture of polyadenylated and deadenylated PHYA messages, suggesting that the two distinct degradation pathways are polysome associated.

Published

1994

530. Alpha thalassaemia mental retardation (ATR-X): an atypical family.

Author

Logie LJ, Gibbons RJ, Higgs DR, Brown JK, and Porteous ME

Subjects

Adolescent, Facial Bones abnormalities, Genetic Linkage, Hemoglobin H analysis, Humans, Infant, Newborn, Male, Pedigree, Skull abnormalities, alpha-Thalassemia genetics, Intellectual Disability genetics, X Chromosome, alpha-Thalassemia psychology

Abstract

A novel form of severe, X linked mental retardation associated with alpha thalassaemia (ATR-X syndrome) has recently been described. Two affected cousins are described, one of whom has an unusually mild haematological phenotype. HbH inclusions, which are the hallmark of this disease, were only detected in the peripheral red blood cells after repeated observations.

Published

1994

531. The detection of amylase on swabs from sexual assault cases.

Author

Keating SM and Higgs DF

Subjects

Breast enzymology, Female, Forensic Medicine, Humans, Male, Penis enzymology, Time Factors, Vagina enzymology, Amylases isolation & purification, Body Fluids enzymology, Saliva enzymology, Sex Offenses

Abstract

Results are presented of amylase tests performed on more than 400 casework swabs using Phadebas tablets. Amylase levels indicative of saliva were obtained from 25% of the penile swabs tested, 32% of the vaginal swabs and 50% of the breast swabs. The longest time interval between the offence and sampling when such levels were detected was 16 hours for penile swabs, 55 hours for vaginal swabs and 30 hours for breast swabs.

Published

1994

532. Analysis of the human alpha-globin gene cluster in transgenic mice.

Author

Sharpe JA, Wells DJ, Whitelaw E, Vyas P, Higgs DR, and Wood WG

Subjects

Animals, Gene Expression Regulation, Genes, Gestational Age, Humans, Mice, Multigene Family, RNA, Messenger genetics, Regulatory Sequences, Nucleic Acid, Restriction Mapping, Globins genetics, Mice, Transgenic embryology

Abstract

A 350-bp segment of DNA associated with an erythroid-specific DNase I-hypersensitive site (HS-40), upstream of the alpha-globin gene cluster, has been identified as the major tissue-specific regulator of the alpha-globin genes. However, this element does not direct copy number-dependent or developmentally stable expression of the human genes in transgenic mice. To determine whether additional upstream hypersensitive sites could provide more complete regulation of alpha gene expression we have studied 17 lines of transgenic mice bearing various DNA fragments containing HSs -33, -10, -8, and -4, in addition to HS -40. Position-independent, high-level expression of the human zeta- and alpha-globin genes was consistently observed in embryonic erythroid cells. However, the additional HSs did not confer copy-number dependence, alter the level of expression, or prevent the variable down-regulation of expression in adults. These results suggest that the region upstream of the human alpha-globin genes is not equivalent to that upstream of the beta locus and that although the two clusters are coordinately expressed, there may be differences in their regulation.

Published

1993

533. A base substitution (T-->C) in codon 29 of the alpha 2-globin gene causes alpha thalassaemia.

Author

Hall GW, Thein SL, Newland AC, Chisholm M, Traeger-Synodinos J, Kanavakis E, Kattamis C, and Higgs DR

Subjects

Adult, Anemia, Hypochromic etiology, Base Sequence, Child, Preschool, DNA chemistry, Female, Humans, Infant, Male, Molecular Sequence Data, Polymerase Chain Reaction, alpha-Thalassemia complications, Codon genetics, Globins genetics, Mutation genetics, alpha-Thalassemia genetics

Abstract

We have identified three individuals of Greek or Greek Cypriot origin with an atypical form of HbH disease characterized by a severe hypochromic microcytic anaemia associated with relatively small amounts of HbH in the peripheral blood. Molecular analysis has shown that each is a compound heterozygote for a previously described mutation affecting the poly A addition signal (AATAAA-->AATAAG) and a previously undescribed mutation involving a T-->C transition in codon 29 of the alpha 2 gene causing a leucine-->proline substitution. Although this mutation would be expected to produce an unstable haemoglobin and hence a haemolytic anaemia, simple heterozygotes for the alpha 29Leu-->Pro mutation have the phenotype of alpha-thalassaemia trait.

Published

1993

534. Dental care--matching training with need.

Author

Higgs DM

Subjects

Dental Care standards, Education, Dental standards, Faculty, Dental supply & distribution, General Practice, Dental standards, Health Services Needs and Demand, Humans, Quality Assurance, Health Care, Schools, Dental, Training Support, United Kingdom, Dental Auxiliaries education, Education, Dental methods, General Practice, Dental education, Specialties, Dental education

Abstract

When dentistry was first incorporated into the new National Health Service the amount of untreated dental disease was enormous. A system was required which would provide a high volume of simple dental treatment. This was successfully achieved but what is now long overdue is a transfer to low volume, high quality, well-maintained treatment based on a foundation of effective public education in prevention.

Published

1993

535. Role of upstream DNase I hypersensitive sites in the regulation of human alpha globin gene expression.

Author

Sharpe JA, Summerhill RJ, Vyas P, Gourdon G, Higgs DR, and Wood WG

Subjects

Animals, Base Sequence, Chromosome Mapping, Clone Cells, DNA analysis, Gene Expression, Gene Expression Regulation, Enzymologic, Humans, Mice, Mice, Transgenic, Molecular Sequence Data, Promoter Regions, Genetic, RNA analysis, Transfection, Tumor Cells, Cultured, Deoxyribonuclease I genetics, Deoxyribonuclease I physiology, Globins genetics

Abstract

Erythroid-specific DNase 1 hypersensitive sites have been identified at the promoters of the human alpha-like genes and within the region from 4 to 40 kb upstream of the gene cluster. One of these sites, HS-40, has been shown previously to be the major regulator of tissue-specific alpha-globin gene expression. We have now examined the function of other hypersensitive sites by studying the expression in mouse erythroleukemia (MEL) cells of various fragments containing these sites attached to HS-40 and an alpha-globin gene. High level expression of the alpha gene was observed in all cases. When clones of MEL cells bearing a single copy of the alpha-globin gene fragments were examined, expression levels were similar to those of the endogenous mouse alpha genes and similar to MEL cells bearing beta gene constructs under the control of the beta-globin locus control region. However, there was no evidence that the additional hypersensitive sites increased the level of expression or conferred copy number dependence on the expression of a linked alpha gene in MEL cells.

Published

1993

536. The thalassaemia syndromes.

Author

Higgs DR

Subjects

Forecasting, Hemoglobins metabolism, Humans, alpha-Thalassemia genetics, beta-Thalassemia genetics, Thalassemia genetics, Thalassemia prevention & control, Thalassemia therapy

Published

1993

537. Understanding erythroid differentiation.

Author

Higgs DR and Wood WG

Published

1993

538. Frequency and clinical significance of erythrocyte genetic abnormalities in Omanis.

Author

White JM, Christie BS, Nam D, Daar S, and Higgs DR

Subjects

Adolescent, Adult, Aged, Child, Erythrocyte Indices, Erythrocytes chemistry, Female, Ferritins analysis, Fetal Blood cytology, Glucosephosphate Dehydrogenase blood, Glucosephosphate Dehydrogenase Deficiency epidemiology, Hemoglobins analysis, Heterozygote, Humans, Infant, Newborn, Male, Middle Aged, Oman epidemiology, Phenotype, Sickle Cell Trait epidemiology, alpha-Thalassemia epidemiology, beta-Thalassemia epidemiology, Gene Frequency, Glucosephosphate Dehydrogenase Deficiency genetics, Sickle Cell Trait genetics, alpha-Thalassemia genetics, beta-Thalassemia genetics

Abstract

The frequencies of four malaria associated erythrocyte genetic abnormalities have been established in 1000 Omani subjects. They are: homozygous alpha+ thalassaemia (-alpha/-alpha) 0.45; high Hb A2 beta thalassaemia trait 0.015; sickle trait (Hb A/S) 0.061; and glucose 6 phosphate dehydrogenase deficiency (Gd-): males 0.27, females 0.11. From our data the alpha+ (-alpha/) thal gene (confirmed by Southern blotting) is pandemic in this population. Moreover, in spite of the very high frequency of Gd-, oxidative haemolytic syndromes are very uncommon. Also preliminary data indicate that among the Omani population with sickle cell disease, homozygosity of the alpha+ gene markedly modifies the clinical picture.

Published

1993

539. β-glucuronidase gene expression and mRNA stability in oat protoplasts.

Author

Higgs DC and Colbert JT

Abstract

Protoplasts derived from oat (Avena sativa L.) suspension culture cells (7 days after subculturing) were electroporated with plasmid DNA containing the Escherichia coli uidA gene encoding the ß-glucuronidase reporter enzyme. Consistently high enzyme activity was observed with electroporation conditions of 500 μF and 1125 volts/cm. Enzyme activity and mRNA accumulation time courses were determined. The maximum enzyme activity was detected at 24 hours after electroporation, while the maximum mRNA level was detected at 12 hours after electroporation. ß-glucuronidase mRNA was in vitro synthesized with and without a 5' methylated cap and then electroporated into protoplasts. Only capped mRNA produced significant enzyme activity. By electroporating radiolabeled, in vitro synthesized mRNA, the ß-glucuronidase mRNA half-life was estimated to be ∼35 minutes in oat protoplasts.

Published

1993

540. Structure of the human 3-methyladenine DNA glycosylase gene and localization close to the 16p telomere.

Author

Vickers MA, Vyas P, Harris PC, Simmons DL, and Higgs DR

Subjects

Amino Acid Sequence, Base Sequence, Cell Line, Chromosome Mapping, DNA Repair, Exons, Globins genetics, Humans, Introns, Molecular Sequence Data, Multigene Family, Restriction Mapping, Chromosomes, Human, Pair 16, DNA Glycosylases, N-Glycosyl Hydrolases genetics, Telomere

Abstract

We recently reported the presence of four genes lying between the human alpha-globin gene cluster and the telomere of the short arm of chromosome 16 (16p). We now report that one of these genes encodes 3-methyladenine DNA glycosylase, an enzyme important in the repair of DNA after damage by alkylating agents. The gene comprises five exons, representation of which differs in independently isolated cDNA clones. Although the gene is widely expressed, the abundance of its mRNA is considerably higher in a colon adenocarcinoma cell line (HT29) than in other cell lines that were tested. The major positive erythroid-specific regulatory element controlling alpha-globin gene expression lies equidistant between the promoters of the alpha-globin genes and the 3-methyladenine DNA glycosylase gene. Interestingly, in contrast to the alpha-globin genes, expression of the 3-methyladenine DNA glycosylase gene is not influenced by the regulatory element in the human erythroleukemia cell line K562.

Published

1993

541. Transcriptional activation of human zeta 2 globin promoter by the alpha globin regulatory element (HS-40): functional role of specific nuclear factor-DNA complexes.

Author

Zhang Q, Reddy PM, Yu CY, Bastiani C, Higgs D, Stamatoyannopoulos G, Papayannopoulou T, and Shen CK

Subjects

Base Sequence, Binding Sites, DNA Mutational Analysis, DNA-Binding Proteins metabolism, Erythroid-Specific DNA-Binding Factors, GATA1 Transcription Factor, Humans, In Vitro Techniques, Molecular Sequence Data, Mutagenesis, Site-Directed, NF-E2 Transcription Factor, NF-E2 Transcription Factor, p45 Subunit, Nuclear Proteins physiology, Oligodeoxyribonucleotides chemistry, RNA, Messenger genetics, Sequence Deletion, Transcription, Genetic, Tumor Cells, Cultured, Enhancer Elements, Genetic, Erythroid Precursor Cells physiology, Gene Expression Regulation, Globins genetics, Promoter Regions, Genetic, Transcription Factors metabolism

Abstract

We studied the functional interaction between human embryonic zeta 2 globin promoter and the alpha globin regulatory element (HS-40) located 40 kb upstream of the zeta 2 globin gene. It was shown by transient expression assay that HS-40 behaved as an authentic enhancer for high-level zeta 2 globin promoter activity in K562 cells, an erythroid cell line of embryonic and/or fetal origin. Although sequences located between -559 and -88 of the zeta 2 globin gene were dispensable for its expression on enhancerless plasmids, they were required for the HS-40 enhancer-mediated activity of the zeta 2 globin promoter. Site-directed mutagenesis demonstrated that this HS-40 enhancer-zeta 2 globin promoter interaction is mediated by the two GATA-1 factor binding motifs located at -230 and -104, respectively. The functional domains of HS-40 were also mapped. Bal 31 deletion mapping data suggested that one GATA-1 motif, one GT motif, and two NF-E2/AP1 motifs together formed the functional core of HS-40 in the erythroid-specific activation of the zeta 2 globin promoter. Site-directed mutagenesis further demonstrated that the enhancer function of one of the two NF-E2/AP1 motifs of HS-40 is mediated through its binding to NF-E2 but not AP1 transcription factor. Finally, we did genomic footprinting of the HS-40 enhancer region in K562 cells, adult nucleated erythroblasts, and different nonerythroid cells. All sequence motifs within the functional core of HS-40, as mapped by transient expression analysis, appeared to bind a nuclear factor(s) in living K562 cells but not in nonerythroid cells. On the other hand, only one of the apparently nonfunctional sequence motifs was bound with factors in vivo. In comparison to K562, nucleated erythroblasts from adult human bone marrow exhibited a similar but nonidentical pattern of nuclear factor binding in vivo at the HS-40 region. These data suggest that transcriptional activation of human embryonic zeta 2 globin gene and the fetal/adult alpha globin genes is mediated by erythroid cell-specific and developmental stage-specific nuclear factor-DNA complexes which form at the enhancer (HS-40) and the globin promoters.

Published

1993

542. De novo truncation of chromosome 16p and healing with (TTAGGG)n in the alpha-thalassemia/mental retardation syndrome (ATR-16).

Author

Lamb J, Harris PC, Wilkie AO, Wood WG, Dauwerse JG, and Higgs DR

Subjects

Adult, Base Sequence, Blotting, Southern, DNA analysis, DNA Mutational Analysis, DNA Nucleotidylexotransferase metabolism, DNA Repair, Electrophoresis, Gel, Pulsed-Field, Fathers, Globins genetics, Humans, Male, Molecular Sequence Data, Polymerase Chain Reaction, Restriction Mapping, Syndrome, Chromosome Deletion, Chromosomes, Human, Pair 16, Intellectual Disability genetics, Telomere metabolism, alpha-Thalassemia genetics

Abstract

We have previously described a series of patients in whom the deletion of 1-2 megabases (Mb) of DNA from the tip of the short arm of chromosome 16 (band 16p13.3) is associated with alpha-thalassemia/mental retardation syndrome (ATR-16). We now show that one of these patients has a de novo truncation of the terminal 2 Mb of chromosome 16p and that telomeric sequence (TTAGGG)n has been added at the site of breakage. This suggests that the chromosomal break, which is paternal in origin and which probably arose at meiosis, has been stabilized in vivo by the direct addition of the telomeric sequence. Sequence comparisons of this breakpoint with that of a previously described chromosomal truncation (alpha alpha)TI do not reveal extensive sequence homology. However, both breakpoints show minimal complementarity (3-4 bp) to the proposed RNA template of human telomerase at the site at which telomere repeats have been added. Unlike previously characterized individuals with ATR-16, the clinical features of this patient appear to be solely due to monosomy for the terminal portion of 16p13.3. The identification of further patients with "pure" monosomy for the tip of chromosome 16p will be important for defining the loci contributing to the phenotype of this syndrome.

Published

1993

543. alpha-Thalassaemia.

Author

Higgs DR

Subjects

Base Sequence, Consensus Sequence, Gene Expression Regulation, Globins genetics, Hemoglobin H genetics, Hemoglobins, Abnormal genetics, Humans, Hydrops Fetalis genetics, Intellectual Disability genetics, Molecular Sequence Data, Multigene Family, Mutation, alpha-Thalassemia genetics

Abstract

The large number of naturally occurring mutants of this well-characterized locus provides an excellent opportunity for elucidating the relationship between its structure and function. Comparisons of what has been learned about the alpha-globin locus with complementary observations on the beta-globin locus, provide a strategy for understanding the co-ordinate regulation of eukaryotic gene expression. From a practical point of view it is important to remember that millions of individuals throughout the world are carriers of alpha-thalassaemia and every year many thousands of pregnancies are at risk of producing children with the severe alpha-thalassaemia syndromes. The data summarized here provide the basis for accurately predicting the genotype in such cases and thus enabling appropriate prenatal testing. However, because this is a genetic disease that predominantly affects individuals from countries with limited health resources, simpler and cheaper methods of screening and diagnosis will have to be developed before this information has a significant impact on the attendant morbidity and mortality (see Chapter 9, this volume).

Published

1993

544. The regulation of human globin gene expression.

Author

Grosveld F, Dillon N, and Higgs D

Subjects

Animals, Chromatin metabolism, Gene Expression Regulation, Globins genetics, Growth physiology, Humans, Methylation, Mice, Mice, Transgenic, Mutation, Transcription Factors metabolism, Globins biosynthesis

Abstract

The haemopoietic system provides a well-characterized and accessible system for studying the mechanisms of developmental regulation and differentiation in higher eukaryotes. Our current understanding of the steps involved in the early stages of differentiation are poorly understood but a great deal is now known about the mechanisms by which globin expression is regulated in cells committed to the erythroid lineage. Many of the critical cis-acting sequences and some of the important trans-acting factors involved have been identified and current work is focusing on how these interact to produce high levels of tissue-specific and developmentally regulated expression of the human globin genes.

Published

1993

545. Influence of alpha thalassaemia on the retinopathy of homozygous sickle cell disease.

Author

Fox PD, Higgs DR, and Serjeant GR

Subjects

Adolescent, Adult, Age Factors, Aged, Anemia, Sickle Cell genetics, Female, Fluorescein Angiography, Homozygote, Humans, Male, Middle Aged, Sex Factors, Anemia, Sickle Cell complications, Retinal Diseases etiology, alpha-Thalassemia complications

Abstract

Homozygous alpha+ thalassaemia (alpha-/alpha-) ameliorates some of the clinical manifestations of homozygous sickle cell (SS) disease but its effect on retinal complications remains unknown. This has been assessed by visual examination and fluorescein angiography in 39 subjects with SS disease and homozygous alpha+ thalassaemia and in 39 age/sex matched controls with SS disease but with a normal alpha globin genotype (alpha alpha/alpha alpha). The results indicate that homozygous alpha+ thalassaemia reduces the extent of peripheral retinal vessel closure but has no apparent effect on the frequency of proliferative sickle retinopathy.

Published

1993

546. Utilization of dietary starch and glucose tolerance in juvenile chinook salmon (Oncorhynchus tshawytscha) of different strains in seawater.

Author

Mazur CN, Higgs DA, Plisetskaya E, and March BE

Abstract

Juvenile chinook salmon of three strains responded to inclusion of 28.7% of gelatinized starch in the diet with different degrees of reduction in growth rate and feed efficiency relative to control fish of the respective strains fed a low-starch, high-lipid diet of similar protein (46%) and estimated metabolizable energy content (16 mJ/kg). The productive protein value of the diet was not reduced to the same extent by the high intake of starch. Carcasses of fish fed the high-starch diet contained higher concentrations of protein and lower concentrations of lipid than control fish. The accumulation of liver glycogen in response to the high-starch diet differed among strains. Glucose tolerance curves also varied among strains but were poorly correlated with plasma concentrations of insulin. Tolerance to glucose loading was improved in fish previously fed the high-starch diet.

Published

1992

547. Analysis of the human alpha globin upstream regulatory element (HS-40) in transgenic mice.

Author

Sharpe JA, Chan-Thomas PS, Lida J, Ayyub H, Wood WG, and Higgs DR

Subjects

Animals, DNA genetics, Female, Homozygote, Humans, Male, Mice, Mice, Inbred C57BL, Mice, Inbred CBA, Mice, Transgenic, Plasmids, RNA, Messenger genetics, Restriction Mapping, Globins genetics, Regulatory Sequences, Nucleic Acid

Abstract

We have analysed the effect of a 1.4 kb segment of DNA containing the upstream alpha globin regulatory element (HS-40) on human alpha globin gene expression in fetal mice and lines of transgenic mice. High levels of tissue-specific, human alpha mRNA expression were seen in all transgenic animals and in this sense expression was position independent. However, the level of human alpha mRNA expression per integrated gene copy decreased during development and was inversely related to copy number. The limitation in expression with increasing gene copy number was shown to be in cis since homozygotes for the transgene produced twice as much human alpha mRNA as hemizygotes. In many respects HS -40 appears similar to single elements within the previously described beta globin locus control region and in cross breeding experiments we have shown that HS -40 behaves in a similar manner to such elements in transgenic mice.

Published

1992

548. X-linked alpha-thalassemia/mental retardation (ATR-X) syndrome: localization to Xq12-q21.31 by X inactivation and linkage analysis.

Author

Gibbons RJ, Suthers GK, Wilkie AO, Buckle VJ, and Higgs DR

Subjects

Female, Genetic Carrier Screening, Genetic Linkage, Genetic Markers genetics, Globins genetics, Humans, Lod Score, Male, Pedigree, Risk, Syndrome, Dosage Compensation, Genetic, Intellectual Disability genetics, X Chromosome, alpha-Thalassemia genetics

Abstract

We have examined seven pedigrees that include individuals with a recently described X-linked form of severe mental retardation associated with alpha-thalassemia (ATR-X syndrome). Using hematologic and molecular approaches, we have shown that intellectually normal female carriers of this syndrome may be identified by the presence of rare cells containing HbH inclusions in their peripheral blood and by an extremely skewed pattern of X inactivation seen in cells from a variety of tissues. Linkage analysis has localized the ATR-X locus to an interval of approximately 11 cM between the loci DXS106 and DXYS1X (Xq12-q21.31), with a peak LOD score of 5.4 (recombination fraction of 0) at DXS72. These findings provide the basis for genetic counseling, assessment of carrier risk, and prenatal diagnosis of the ATR-X syndrome. Furthermore, they represent an important step in developing strategies to understand how the mutant ATR-X allele causes mental handicap, dysmorphism, and down-regulation of the alpha-globin genes.

Published

1992

549. RNase protection assays and RNA gel blots: a direct comparison of sensitivity.

Author

Higgs DC and Colbert JT

Subjects

Edible Grain, Electrophoresis, Polyacrylamide Gel, Glucuronidase genetics, Nucleic Acid Denaturation, RNA Probes, Ribonucleases metabolism, Sensitivity and Specificity, Molecular Probe Techniques, RNA, Bacterial analysis, RNA, Messenger analysis

Abstract

RNase protection assays are commonly thought to be a more sensitive means of detecting and quantitating specific mRNAs than are RNA gel blots (Northern blots). We have directly compared the sensitivity of these two approaches by assaying for known amounts of in vitro synthesized beta-glucuronidase mRNA. With the probes and protocols employed here, the ability to detect a specific mRNA was similar whether RNase protection or RNA gel blot analyses were performed.

Published

1992

550. Oral sex--further information from sexual assault cases.

Author

Keating SM and Higgs DF

Subjects

Adolescent, Adult, Age Factors, Child, Cross-Sectional Studies, England epidemiology, Ethnicity, Female, Humans, Incidence, Male, Middle Aged, Sex Factors, Sex Offenses statistics & numerical data

Abstract

A survey was carried out of sexual assault cases submitted to the Metropolitan Police Forensic Science Laboratory during 1988 and 1989. There were 104 cases with male victims, and 1403 with females. In the all-male offences, fellatio was reported in 34%; nearly two-thirds of the acts were by the offender, one-third by the victim. In the offences on females, oral-genital acts were alleged in 22%, 78% of which were fellatio, and 22% cunnilingus. The majority of offenders were white. The few Afro-Caribbeans studied rarely performed oral sex on males or very young females.

Published

1992