Your search keyword '"Ingo Hansmann"' showing total 95 results

1. Interstitial deletion of 22q11 in DiGeorge syndrome detected by high resolution and molecular analysis

Author

Löns P, Franke Uc, Hanefeld F, Löffler C, Ingo Hansmann, Peter J. Scambler, and B. Zoll

Subjects

Male, Monosomy, medicine.medical_specialty, Pathology, Chromosomes, Human, Pair 22, High resolution, In situ hybridization, Biology, 03 medical and health sciences, 0302 clinical medicine, 030225 pediatrics, DiGeorge syndrome, DiGeorge Syndrome, Genetics, medicine, Humans, Prospective Studies, In Situ Hybridization, Fluorescence, Genetics (clinical), 030304 developmental biology, Southern blot, 0303 health sciences, medicine.diagnostic_test, Infant, Newborn, Cytogenetics, Infant, medicine.disease, Blotting, Southern, Chromosome Deletion, Chromosome 22, Fluorescence in situ hybridization

Abstract

Two patients with DiGeorge syndrome (DGS), one with and one without characteristic dysmorphic facial features, were studied by high resolution banding, fluorescence in situ hybridization (FISH) and quantitative Southern blotting. In both patients, even in the one with no typical facial stigmata, a microdeletion within 22q11.2 was detected. FISH analysis, in particular, is most useful in screening for 22q11.2 segmental monosomy in patients with DGS and DGS-related features.

Published

2008

2. Minimal phenotype in a girl with trisomy 15q due to t(X;15)(q22.3;q11.2) translocation

Author

Svetlana A. Yatsenko, Alma Kuechler, C. Daniel Eller, Pawel Stankiewicz, Uwe Claussen, Christiane Baldermann, York Marahrens, Christiane Gläser, James R. Lupski, Trilochan Sahoo, U. Lieser, Thomas Liehr, Monika Hagemann, Ingo Hansmann, Martin Hesse, and Bernhard Horsthemke

Subjects

Male, Genotype, Aneuploidy, Trisomy, Chromosomal translocation, Biology, Autoantigens, Translocation, Genetic, snRNP Core Proteins, Fraternal twin, Chromosome 15, Genetics, medicine, Humans, Alleles, In Situ Hybridization, Fluorescence, Genetics (clinical), Chromosomes, Human, Pair 15, Chromosomes, Human, X, Autosome, Breakpoint, DNA Methylation, Ribonucleoproteins, Small Nuclear, medicine.disease, Molecular biology, Chromosome Banding, Pedigree, Long Interspersed Nucleotide Elements, Phenotype, Child, Preschool, Karyotyping, Female, Microsatellite Repeats, SNRPN Gene

Abstract

Few cases of de novo unbalanced X;autosome translocations associated with a normal or mild dysmorphic phenotype have been described. We report a 3-year-old dizygotic female twin with prenatally ascertained increased nuchal translucency. Prenatal chromosome studies revealed nearly complete trisomy 15 due to a de novo unbalanced translocation t(X;15)(q22;q11.2) confirmed postnatally. A mild phenotype was observed with normal birth measurements, minor facial dysmorphic features (hypertelorism, short broad nose, and a relatively long philtrum), and moderate developmental delay at the age of 3 years in comparison to her male fraternal twin. Replication timing utilizing BrdU and acridine-orange staining showed that the der(X) chromosome was late-replicating with variable spreading of inactivation into the translocated 15q segment. The der(X) was determined to be of paternal origin by analyses of polymorphic markers and CGG-repeat at FMR1. Methylation analysis at the SNRPN locus and analysis of microsatellites on 15q revealed paternal isodisomy with double dosage for all markers and the unmethylated SNRPN gene. The Xq breakpoint was mapped within two overlapping BAC clones RP11-575K24 and RP13-483F6 at Xq22.3 and the 15q breakpoint to 15q11.2, within overlapping clones RP11-509A17 and RP11-382A4 that are all significantly enriched for LINE-1 elements (36.6%, 43.0%, 26.6%, 22.0%, respectively). We speculate that the attenuated phenotype may be due to inactivation spreading into 15q, potentially facilitated by the enrichment of LINE-1 elements at the breakpoints. In silico analysis of breakpoint regions revealed the presence of highly identical low-copy repeats (LCRs) at both breakpoints, potentially involved in generating the translocation.

Published

2006

3. Molecular cytogenetic characterization of a familial pericentric inversion 3 associated with short stature

Author

Ingo Hansmann, Usha R. Dutta, and Dietmar Schlote

Subjects

Male, Positional cloning, Adolescent, Karyotype, Chromosome Disorders, Dwarfism, Biology, Exon, Putative gene, Databases, Genetic, Genetics, medicine, Humans, Cloning, Molecular, Child, Gene, Genetics (clinical), In Situ Hybridization, Fluorescence, Chromosomal inversion, Bacterial artificial chromosome, medicine.diagnostic_test, Breakpoint, General Medicine, Sequence Analysis, DNA, Pedigree, Chromosome Inversion, Cytogenetic Analysis, Female, Chromosomes, Human, Pair 3, Sequence Alignment, Fluorescence in situ hybridization

Abstract

Short stature refers to the height of an individual which is below expected. The causes are heterogenous and influenced by several genetic and environmental factors. Chromosomal abnormalities are a major cause of diseases and cytogenetic mapping is one of the powerful tools for the identification of novel disease genes. Here we report a three generation family with a heterozygous pericentric inversion of 46, XX, inv(3) (p24.1q26.1) associated with Short stature. Positional cloning strategy was used to physically map the breakpoint regions by Fluorescence in situ hybridization (FISH). Fine mapping was performed with Bacterial Artificial Chromosome (BAC) clones spanning the breakpoint regions. In order to further characterize the breakpoint regions extensive molecular mapping was carried out with the breakpoint spanning BACs which narrowed down the breakpoint region to 2.9 kb and 5.3 kb regions on p and q arm respectively. Although these breakpoints did not disrupt any validated genes, we had identified a novel putative gene in the vicinity of 3q26.1 breakpoint region by in silico analysis. Trying to find the presence of any transcripts of this putative gene we analyzed human total RNA by RT-PCR and identified transcripts containing three new exons confirming the existence of a so far unknown gene close to the 3q breakpoint.

Published

2014

4. Genomic structure of karyopherin ?2 ( KPNA2 ) within a low-copy repeat on chromosome 17q23-q24 and mutation analysis in patients with Russell-Silver syndrome

Author

Sylvia Dörr, Mike Schlicker, and Ingo Hansmann

Subjects

alpha Karyopherins, Molecular Sequence Data, Translocation Breakpoint, Biology, medicine.disease_cause, Exon, Genetics, medicine, Humans, Abnormalities, Multiple, Amino Acid Sequence, Cloning, Molecular, Gene, Genetics (clinical), DNA Primers, Karyopherin, Genomic organization, chemistry.chemical_classification, Mutation, Fetal Growth Retardation, Base Sequence, Sequence Homology, Amino Acid, Intron, RNA-Binding Proteins, Syndrome, Blotting, Southern, chemistry, Gene Deletion, Nuclear localization sequence, Chromosomes, Human, Pair 17

Abstract

Human karyopherin alpha2 (KPNA2), a member of the karyopherin alpha family, plays a key role in the nuclear import of proteins with a classical nuclear localization signal (NLS). KPNA2, as part of a karyopherin alpha-beta heterodimer, directly binds to the NLS of proteins and functions as an adaptor that binds NLS-containing proteins via karyopherin beta to the nuclear pore complex. The NLS protein-receptor complex is translocated through the pore by an energy-dependent mechanism. Recently, we have identified and mapped the gene for KPNA2 in close proximity to a translocation breakpoint within 17q23-q24 associated with Russell-Silver syndrome (RSS). Therefore, we considered KPNA2 as a positional candidate gene for this heterogeneous disorder. RSS is mainly characterized by pre- and postnatal growth retardation, lateral asymmetry, and other dysmorphic features. Here, we present the genomic organization of the human KPNA2 gene with 11 exons spanning approximately 10 kb on chromosome 17q23-q24. Screening for mutations within all exons and adjacent intronic sequences from 31 unrelated RSS patients revealed three single nucleotide polymorphisms (SNPs) in exons 1, 5, and 7, and five SNPs in introns 1, 4 (2 SNPs), 8, and 9, respectively. No disease-related mutation was identified by comparing the sequence data of the RSS patients with their clinically normal parents and controls.

Published

2001

5. Parental mosaicism of JAG1 mutations in families with Alagille syndrome

Author

David J. Amor, Ingo Hansmann, Joannis Giannakudis, Albrecht Röpke, Jean-Pierre Fryns, Mike Schlicker, Agnes Bankier, Annegret Kujat, Małgorzata Krajewska-Walasek, and Helen E. Hughes

Subjects

Male, JAG1, Biology, medicine.disease_cause, Variable Expression, Alagille syndrome, Genetics, medicine, Humans, Serrate-Jagged Proteins, Genetics (clinical), DNA Primers, Mutation, Base Sequence, Mosaicism, Calcium-Binding Proteins, Membrane Proteins, Proteins, Autosomal dominant trait, medicine.disease, Penetrance, Pedigree, Alagille Syndrome, Phenotype, Intercellular Signaling Peptides and Proteins, Jagged-1 Protein, Female, Congenital disorder

Abstract

The Alagille syndrome (AGS), a congenital disorder affecting liver, heart, skeleton and eye in association with a typical face, is an autosomal dominant disease with nearly complete penetrance and variable expression. AGS is caused by mutations in the developmentally important JAG1 gene. In our mutation screening, where 61 mutations in JAG1 were detected, we identified five cases where mosaicism is present. Our results point to a significant frequency of mosaicism for JAG1 mutations in AGS of more than 8.2%. Because mosaicism may be associated with a very mild phenotype, the appropriate diagnosis of AGS and consequently the determination of the recurrence risk can be complicated.

Published

2001

6. Alagille syndrome associated with a paracentric inversion 20p12.2p13 disrupting theJAG1 gene

Author

Jolanta Rujner, Bożena Piłacik, Christiane Löffler, Ioannis Giannakudis, Anna Gutkowska, Paweł Stankiewicz, Małgorzata Krajewska-Walasek, Manjunath Nimmakayalu, Ingo Hansmann, and Antje Krüger

Subjects

Male, JAG1, Chromosomes, Human, Pair 20, Biology, medicine.disease_cause, Exon, Gene mapping, Alagille syndrome, medicine, Humans, Serrate-Jagged Proteins, Gene, In Situ Hybridization, Fluorescence, Genetics (clinical), Chromosomal inversion, Genetics, Mutation, Calcium-Binding Proteins, Infant, Membrane Proteins, Proteins, DNA, medicine.disease, Chromosome Banding, Alagille Syndrome, Blotting, Southern, Child, Preschool, Chromosome Inversion, Intercellular Signaling Peptides and Proteins, Chromosome 20, Jagged-1 Protein

Abstract

Mutations in the human gene Jagged1 (JAG1) localized in 20p12 have been recently identified as causal for the anomalies found in patients with Alagille syndrome (AGS). This gene encodes a ligand for the Notch1 transmembrane receptor, which plays a key role in cell-to-cell signaling during differentiation and is conserved from C. elegans to human. We report a paracentric inversion (PAI) of chromosome 20p12.2p13 in an individual with AGS who also had α-1-antitrypsin deficiency. To our knowledge, this is the first published case of PAI involving the short arm of chromosome 20. Using FISH, fiberFISH, and molecular studies with a ∼40 kb cosmid clone encompassing the entire 36 kb JAG1 gene, we demonstrate that the gene was disrupted by the inversion breakpoint between exons 5 and 6. An unusual association between two most common causes of chronic liver disease in childhood, AGS and α-1-antitrypsin deficiency, as well as their influence on the proband's abnormal phenotype are discussed. © 2001 Wiley-Liss, Inc.

Published

2001

7. Phenotypic findings due to trisomy 7p15.3-pter including theTWIST locus

Author

Jürgen Kunz, Hannelore Thiele, Christiane Baldermann, Ingo Hansmann, Paweł Stankiewicz, Nadeshda Werner, Sylvia Dörr, Gudrun A. Rappold, Ioannis Giannakudis, and Antje Krüger

Subjects

Male, Microcephaly, Adolescent, Pseudoautosomal region, Trisomy, Chromosomal translocation, Postnatal microcephaly, Biology, Translocation, Genetic, Fingers, Y Chromosome, medicine, Humans, Abnormalities, Multiple, Hypertelorism, Child, Growth Disorders, In Situ Hybridization, Fluorescence, Genetics (clinical), Twist-Related Protein 1, Breakpoint, Infant, Nuclear Proteins, Anatomy, Toes, Choanal stenosis, medicine.disease, Phenotype, Karyotyping, medicine.symptom, Chromosomes, Human, Pair 7, Transcription Factors

Abstract

We report on a three-month-old boy with a 46,XY,der(Y)t(Y;7)(p11.32;p15.3) karyotype and growth deficiency, postnatal microcephaly with large fontanels, wide sagittal and metopic sutures, hypertelorism, choanal stenosis, micrognathia, bilateral cryptorchidism, hypospadias, abnormal fingers and toes, and severe developmental delay. FISH studies showed partial trisomy 7p resulting from a de novo unbalanced translocation. The application of molecular probes from the TWIST gene region (7p15.3-p21.1) and probes from the pseudoautosomal region (PAR) demonstrated that the 7p15.3-pter fragment was translocated onto Yp with the breakpoint within approximately 20 kb from the Yp telomere. We discuss the possible role of the TWIST gene in abnormal skull development and suggest that trisomy 7p cases with delayed closure of fontanels can be a result of TWIST gene dosage effect.

Published

2001

8. Chromosome mapping of Rett syndrome: a likely candidate region on the telomere of Xq

Author

Pereira Joseluiz, Angus John Clarke, Lars Edström, Naidu Sakkubai, Ingo Hansmann, Maria Anvret, Fengqing Xiang, Zhiping Zhang, Budden Sarojini, and C. D. DeLozier-Blanchet

Subjects

Male, X Chromosome, Rett syndrome, Locus (genetics), Biology, Genetic determinism, 03 medical and health sciences, 0302 clinical medicine, Germline mutation, Gene mapping, Rett Syndrome, Genetics, medicine, Humans, Skewed X-inactivation, Genetics (clinical), X chromosome, 0303 health sciences, 030305 genetics & heredity, Chromosome Mapping, Telomere, medicine.disease, Pedigree, Xq28, Female, 030217 neurology & neurosurgery, Microsatellite Repeats, Research Article

Abstract

Rett syndrome (RS) is a disease of neurological development. First reported 30 years ago in 1966, its biological and genetic basis remains obscure. RS is commonly thought of as an X linked dominant disorder lethal to hemizygous males. The few familial cases would arise through mosaicism or because of occasional females failing to manifest the disorder through skewed X inactivation in relevant cell types. We have one family where the mother and daughter are affected with RS, and which can be explained according to this hypothesis. If the alternative proposal of Thomas (1996) is correct, that the lack of males affected by such disorders is the result of a high male to female ratio of germline mutations rather than of gestational lethality, then the RS gene should be located on the grandpaternal chromosome. Genomic screening with markers covering the whole X chromosome has been performed. Studies using multiple informative markers indicate that the RS locus is likely to be located close to one of the X chromosome telomeres. Further investigations in eight additional families suggest the most likely region for the RS gene to be is the distal part of Xq (Xq28).

Published

1998

9. Molecular structure and chromosomal mapping of the human homolog of the agouti gene

Author

Richard P. Woychik, Ingo Hansmann, Paul J. Furdon, John G. Powell, Wen Ji Chen, Scott J. Bultman, Heajoon Y. Kwon, William O. Wilkison, Christiane Löffler, and Anton-Lewis Usala

Subjects

Male, Transcription, Genetic, Sequence analysis, Molecular Sequence Data, Restriction Mapping, Chromosomes, Human, Pair 20, 030209 endocrinology & metabolism, Locus (genetics), Biology, Polymerase Chain Reaction, Mice, 03 medical and health sciences, 0302 clinical medicine, Gene mapping, Pregnancy, Animals, Humans, Coding region, Amino Acid Sequence, Cloning, Molecular, Gene, Peptide sequence, Conserved Sequence, DNA Primers, 030304 developmental biology, Genetics, Genomic Library, 0303 health sciences, Multidisciplinary, integumentary system, Base Sequence, Sequence Homology, Amino Acid, Gene map, digestive, oral, and skin physiology, Intron, Chromosome Mapping, Proteins, Hominidae, Molecular biology, Introns, Organ Specificity, Protein Biosynthesis, Agouti Signaling Protein, Intercellular Signaling Peptides and Proteins, Female, Research Article

Abstract

The agouti (a) locus in mouse chromosome 2 normally regulates coat color pigmentation. The mouse agouti gene was recently cloned and shown to encode a distinctive 131-amino acid protein with a consensus signal peptide. Here we describe the cloning of the human homolog of the mouse agouti gene using an interspecies DNA-hybridization approach. Sequence analysis revealed that the coding region of the human agouti gene is 85% identical to the mouse gene and has the potential to encode a protein of 132 amino acids with a consensus signal peptide. Chromosomal assignment using somatic-cell-hybrid mapping panels and fluorescence in situ hybridization demonstrated that the human agouti gene maps to chromosome band 20q11.2. This result revealed that the human agouti gene is closely linked to several traits, including a locus called MODY (for maturity onset diabetes of the young) and another region that is associated with the development of myeloid leukemia. Initial expression studies with RNA from several adult human tissues showed that the human agouti gene is expressed in adipose tissue and testis.

Published

1994

10. 2. A Multilocus DNA Fingerprint with Built-in Security Devices

Author

Ingo Hansmann, Ulrike Thies, Jörg T. Epplen, Jörg Schmidtke, and Michael Krawczak

Subjects

Proband, Health Policy, Genetic counseling, Fingerprint (computing), Biology, Y chromosome, Issues, ethics and legal aspects, DNA profiling, Evolutionary biology, Mutation (genetic algorithm), Forensic engineering, Abnormality, Genetic diagnosis, Law

Abstract

An unusual case of paternity testing is reported in which determination of paternity was an essential part of a genetic diagnosis. A.Y-chromosomal abnormality, observed in a 33-year-old male whose wife had experienced a series of spontaneous abortions, was not found in his alleged father. DNA fingerprinting with the oligonucleotide multilocus probe (CAC)5 yielded two aberrant bands for the proband, i.e. bands exhibited by neither parent. This finding resulted in a comparatively low paternity probability of 0.02934 which is suggestive of, but does not unequivocally prove, false paternity. Subsequent analysis with other multi- and single-locus systems, however, failed to confirm this preliminary result. The paternity probability computed on the basis of the single-locus systems was 0.99997, providing compelling evidence in favour of true paternity. The present case thus demonstrates that even when two mutations turn up in a DNA fingerprint, these may be readily recognized as such.

Published

1994

11. Prenatal diagnosis of the Pallister-Killian mosaic aneuploidy syndrome by CVS

Author

Helga Rehder, Barbara Zoll, Jürgen Bernert, Ingo Hansmann, Gudrun Gatz, Paul Dieter Niedmann, Martina Heyat, Iris Bartels, and Claus Waldenmaier

Subjects

Adult, Genetic Markers, Isochromosome, Chorionic villus sampling, Aneuploidy, Prenatal diagnosis, Biology, Fingers, 03 medical and health sciences, Pallister–Killian syndrome, Pregnancy, medicine, Humans, Abnormalities, Multiple, Genitalia, Genetics (clinical), 030304 developmental biology, 0303 health sciences, medicine.diagnostic_test, Mosaicism, 030305 genetics & heredity, Aborted Fetus, Chromosome, Karyotype, Syndrome, medicine.disease, Molecular biology, 3. Good health, Chorionic Villi Sampling, Face, Karyotyping, Female

Abstract

Prenatal cytogenetic analysis at 11 weeks of gestation revealed an abnormal karyotype 47,XX,+mar in all metaphases obtained from a chorionic villi sample after 24 h culture. Karyotyping of amniotic fluid cells in the second trimester showed mosaicism 47,XX,+i(12p)/46,XX with 10% aneuploid cells. The pregnancy was terminated at 20 weeks of gestation on the patient's request. The aborted fetus showed typical manifestations of the Pallister-Killian mosaic aneuploidy syndrome. The identity of the supernumerary isochromosome 12p was proven by LDH isozyme electrophoresis using cultured fibroblasts and by nonradioactive in situ hybridization using a biotinylated set of chromosome 12-specific DNA probes.

Published

1992

12. Contents, Vol. 61, 1992

Author

John S. Mattick, H. Winking, E. Petit, W.L. Neuman, Raju Kucherlapati, U. Hirning-Folz, Roger A. Schultz, Carol A. Westbrook, V.M. Chapman, Kenneth W. Harder, T. Shiomi, Roy Layfield, D. Benova, Howard P. Levy, Frank R. Jirik, Yoichi Matsuda, Maimon M. Cohen, Bernard H. Brownstein, Ian W. Craig, I.G. Melhado, Alessandra M.V. Duncan, Wendy Stock, Settara C. Chandrasekharappa, Robert M. Gemmill, Peter F. Nixon, M M Le Beau, Bernard Dutrillaux, M. Koleva, Y.-N. Harada, W. L. Neuman, N. Lemieux, Hélène Hayes, Christiane Löffler, G.R. Sutherland, Robert Williamson, Kyeryoung Lee, M. Abedinia, J. Battey, S. Natsuume-Sakai, L.L. Anderson, David F. Callen, Elizabeth Baker, V.V.N. Gopal Rao, Horst Hameister, N.M. Lapsys, and Ingo Hansmann

Subjects

Botany, Genetics, Zoology, Biology, Molecular Biology, Genetics (clinical)

Published

1992

13. Silver-Russell syndrome and cystic fibrosis associated with maternal uniparental disomy 7

Author

Uwe Preiss, Monika Hagemann, Ute Hehr, Sabine Brömme, Sylvia Dörr, and Ingo Hansmann

Subjects

Pregnancy, Pathology, medicine.medical_specialty, biology, business.industry, Silver–Russell syndrome, Dwarfism, medicine.disease, Cystic fibrosis, Cystic fibrosis transmembrane conductance regulator, law.invention, Exon, law, medicine, biology.protein, business, Genomic imprinting, Genetics (clinical), Polymerase chain reaction

Published

2000

14. G protein Gsα (GNAS1), the probable candidate gene for albright hereditary osteodystrophy, is assigned to human chromosome 20q12–q13.2

Author

Ingo Hansmann, Susanne Schnittger, and V.V.N. Gopal Rao

Subjects

Male, Candidate gene, G protein, Chromosomes, Human, Pair 20, Biology, Fibrous Dysplasia, Polyostotic, 03 medical and health sciences, 0302 clinical medicine, Gene mapping, GTP-Binding Proteins, Genetics, GNAS complex locus, medicine, Humans, Gene, Pseudohypoparathyroidism, 030304 developmental biology, 0303 health sciences, Chromosome Mapping, medicine.disease, Molecular biology, Chromosome Banding, 030220 oncology & carcinogenesis, Mutation, biology.protein, Signal transduction, Chromosome 20, Signal Transduction

Abstract

Guanine nucleotide-binding proteins, also known as G proteins, mediate intracellular responses to a wide variety of extracellular stimuli. A variety of genes that specify the synthesis of the components of guanine nucleotide proteins have been identified. One of these proteins, termed Gs alpha (GNAS1), is the G protein component of the olfactory signal transduction cascade. Mutations in the GNAS1 gene leading to Gs alpha protein deficiency are known to be associated with pseudohypoparathyroidism Ia (Albright hereditary osteodystrophy) and certain pituitary tumors with acromegaly. Studies on the human--mouse somatic cell hybrids provisionally assigned this gene to chromosome 20. We have now confirmed this localization on chromosome 20 and regionally assigned the GNAS1 gene to 20q12-q13.2 by in situ hybridization.

Published

1991

15. Paramutation-like effects at the mouse scapinin (Phactr3) locus

Author

Dietmar Schlote, Ingo Hansmann, and Sebastian Worch

Subjects

Non-Mendelian inheritance, Locus (genetics), Mice, Inbred Strains, Biology, Regulatory Sequences, Nucleic Acid, Polymorphism, Single Nucleotide, Paramutation, Exon, Genomic Imprinting, Mice, Structural Biology, Genotype, Animals, Allele, Promoter Regions, Genetic, Molecular Biology, Gene, Alleles, Genetics, Nuclear Proteins, Exons, Chromosomes, Mammalian, Alternative Splicing, Animals, Newborn, Knockout mouse, Polymorphism, Restriction Fragment Length

Abstract

Paramutation-like phenomena have been extensively studied in plants and so far described for a very few engineered loci in the mouse. Here we report an allele-specific expression analysis of the Phactr3 (phosphatase and actin regulator 3) locus by identifying the first internal mouse transcripts with a paramutation-like effect not associated with transgenic or knockout mice. In our previous work, we showed that the Phactr3 gene was mainly transcribed in the brain, exhibiting a complex genomic organisation with four alternatively spliced leader exons. Due to the location of the Phactr3 gene in the distal imprinting region on mouse chromosome 2, we generated a mouse model to investigate the possible parental influence on the allelic expression pattern by reciprocally mating NMRI mice and Mus musculus castaneus. We were able to identify a single-nucleotide polymorphism in leader exon 1C representing restriction fragment length polymorphism. After reverse transcription PCR, NMRI and M. musculus castaneus showed a homozygous restriction pattern according to their genotype. Unlike this, reverse transcription PCR products of the F1 hybrids of both crosses were transcribed from the NMRI allele only. Therefore, the Phactr3 exon 1C splice variant is potentially strain specific regulated, leading to the expression of only one allele of the reciprocal crosses. So far, this has not yet been described for an internal mouse gene. These results potentially provide new insight into non-Mendelian inheritance in mammals and may serve also as a model for investigating the regulation of allele-specific expression.

Published

2007

16. Gene symbol: JAG1. Disease: tetralogy of Fallot

Author

C, Glaeser, Dieter, Kotzot, Almuth, Caliebe, Renate, Kottke, Susanne, Schulz, Ullrich, Schweigmann, and Ingo, Hansmann

Subjects

Mutagenesis, Insertional, Calcium-Binding Proteins, Tetralogy of Fallot, Humans, Intercellular Signaling Peptides and Proteins, Membrane Proteins, Serrate-Jagged Proteins, Jagged-1 Protein

Published

2006

17. Duplication of Xq26.2-q27.1, including SOX3, in a mother and daughter with short stature and dyslalia

Author

Andrea Cseke-Friedrich, James R. Lupski, Pawel Stankiewicz, Svetlana A. Yatsenko, Hannelore Thiele, Mike Schlicker, Sylva Bartel-Friedrich, and Ingo Hansmann

Subjects

Proband, Adult, Male, medicine.medical_specialty, Adolescent, media_common.quotation_subject, Mothers, Biology, Short stature, X-inactivation, Speech Disorders, Internal medicine, Gene Duplication, Gene duplication, Genetics, medicine, Humans, Abnormalities, Multiple, Insulin-Like Growth Factor I, Genetics (clinical), X chromosome, Growth Disorders, In Situ Hybridization, Fluorescence, Sex Chromosome Aberrations, media_common, Daughter, Chromosomes, Human, X, SOXB1 Transcription Factors, High Mobility Group Proteins, Karyotype, Chromosome Banding, Pedigree, DNA-Binding Proteins, Endocrinology, Receptors, Androgen, Karyotyping, Speech delay, Female, medicine.symptom, Transcription Factors

Abstract

Duplications of the distal long arm of the X chromosome are rare and carrier females are usually phenotypically normal. We report on a 14-year-old short statured (height and weight

Published

2005

18. Renal failure and hypertension in Alagille syndrome with a novel JAG1 mutation

Author

Sigrid, Harendza, Christian A, Hübner, Christiane, Gläser, Martin, Burdelski, Friedrich, Thaiss, Ingo, Hansmann, Andreas, Gal, and Rolf A K, Stahl

Subjects

Adult, Male, Ultrasonography, Doppler, Duplex, Hypertension, Renal, Calcium-Binding Proteins, Membrane Proteins, Angiotensin-Converting Enzyme Inhibitors, Blood Pressure, Pedigree, Renal Circulation, Alagille Syndrome, Phenotype, Humans, Intercellular Signaling Peptides and Proteins, Kidney Failure, Chronic, Serrate-Jagged Proteins, Frameshift Mutation, Jagged-1 Protein, Follow-Up Studies

Abstract

Renal failure and hypertension in Alagille syndrome with a novel JAG1 mutation: Alagille syndrome is an autosomal dominant disorder involving liver, heart, eyes, face, skeleton, and other organs. Various renal abnormalities have also been associated with Alagille syndrome, whereas renal vascular hypertension combined with renal insufficiency has been reported in several cases. We describe a patient with a novel frameshift mutation (c.1880_1881insA) in the JAG1 gene who presented with chronic renal failure and hypertension but without evidence of renal vascular or aortic stenosis. The patient's chronic renal failure had persisted for several years. His high blood pressure seemed to be due to renal parenchymal changes and was treated with ACE-inhibitors without worsening his renal function. This novel JAG1 mutation revealed great variability of the phenotype. The patient's daughter suffered from severe paucity of intrahepatic bile ducts and received a liver transplant at the age of two years. These findings are discussed including a review of the literature.

Published

2005

19. Twelve novel JAG1 gene mutations in Polish Alagille syndrome patients

Author

Dorota, Jurkiewicz, Ewa, Popowska, Christiane, Gläser, Ingo, Hansmann, and Małgorzata, Krajewska-Walasek

Subjects

Male, Genotype, Calcium-Binding Proteins, DNA Mutational Analysis, Mutation, Missense, Membrane Proteins, Polymerase Chain Reaction, Protein Structure, Tertiary, Alagille Syndrome, Codon, Nonsense, Humans, Intercellular Signaling Peptides and Proteins, Point Mutation, Female, Serrate-Jagged Proteins, Poland, RNA Splice Sites, Frameshift Mutation, Jagged-1 Protein

Abstract

Alagille syndrome (AGS) is an autosomal dominant disorder with developmental abnormalities of the liver, heart, eyes, vertebrae, and face. Mutations in the JAG1 (Jagged 1) gene, coding a ligand in the evolutionarily conserved Notch signaling pathway, are responsible for AGS. Here we present sixteen different JAG1 gene mutations, among them twelve novel, not described previously. Seven frameshift: c. 172_178del7 (p.Ala58fs), c.509delT (p.Leu170fs), c.1197delG (p.Val399fs), c.1485_1486delCT (p.Pro495fs), c.1809_1810insTGGG (p.Lys604fs), c.2122_2125delCAGT (p.Gln708fs), c.2753delT (p.Ile918fs); five nonsense: c.383GA (p.Trp128X), c.496CT (p.Glu166X), c.841CT (p.Gln281X), c.1207CT (p.Gln403X), c.1603CT (p.Gln535X); two splice site: c.388-1GC, c.3048+1_3048+2insG and two missense mutations: c.359TA (p.Ile120Asn), c.560GA (p.Cys187Tyr) were found. Forty percent of the changes were identified in exons 2 and 4, the remaining mutations are distributed along the entire coding sequence of the gene. Seventy-five percent of the mutations lead to creation of premature termination codons. Family studies revealed that the specific mutations were inherited in 3 out of 11 investigated cases. No correlation between genotype and phenotype was observed.

Published

2005

20. An excess of chromosome 1 breakpoints in male infertility

Author

Lisbeth Tranebjerg, Zeynep Tümer, Iben Bache, Maria Orera, Vera M. Kalscheuer, Elisabeth Blennow, Val Davison, Klaus Wagner, David R. FitzPatrick, Isidora Lopez-Pajares, Laurence Duprez, Maj Hultén, Sultan Cingoz, Sophie Dahoun, Niels Tommerup, Margarita Stefanova, Ingo Hansmann, Jan Murken, Maryse Bonduelle, Bruno Dallapiccola, M.-F. Croquette, Tony Parkin, Kirsten Winther, Kim Smith, Fiorella Shabtai, Kirsten Rasmussen, Catherine Turleau, Claes Lundsteen, Anita Niebuhr, Elvire Van Assche, Gotthold Barbi, Eberhard Schwinger, Carl Birger van der Hagen, Bruno Delobel, Philippe Jonveaux, Nadja Kokalj Vokac, Peter Jensen, Inge Liebaers, Mads F. Hjorth, Georges Bourrouillou, Merete Bugge, Carmen Ramos, Regine Schubert, Leopoldo Zelante, Werner Schempp, Eberhard Passarge, Carmen Ayuso, Herman Tournaye, James Lespinasse, Malcolm A. Ferguson-Smith, Ulf Kristoffersson, Jan Wahlstroem, Gert Bruun-Petersen, Hans-Christoph Duba, Karen Brøndum-Nielsen, Michel Vekemans, Elizabeth Grace, Raymond L. Stallings, and Jean McGowan-Jordan

Subjects

Infertility, Genetics, Chromosome Aberrations, Male, medicine.medical_specialty, Cytogenetics, Chromosome, Chromosomal translocation, Karyotype, Locus (genetics), Oligospermia, Biology, medicine.disease, Translocation, Genetic, Male infertility, Chromosomes, Human, Pair 1, Chromosome Inversion, medicine, Humans, Genetics (clinical), Infertility, Male, Chromosomal inversion

Abstract

In a search for potential infertility loci, which might be revealed by clustering of chromosomal breakpoints, we compiled 464 infertile males with a balanced rearrangement from Mendelian Cytogenetics Network database (MCNdb) and compared their karyotypes with those of a Danish nation-wide cohort. We excluded Robertsonian translocations, rearrangements involving sex chromosomes and common variants. We identified 10 autosomal bands, five of which were on chromosome 1, with a large excess of breakpoints in the infertility group. Some of these could potentially harbour a male-specific infertility locus. However, a general excess of breakpoints almost everywhere on chromosome 1 was observed among the infertile males: 26.5 versus 14.5% in the cohort. This excess was observed both for translocation and inversion carriers, especially pericentric inversions, both for published and unpublished cases, and was significantly associated with azoospermia. The largest number of breakpoints was reported in 1q21; FISH mapping of four of these breakpoints revealed that they did not involve the same region at the molecular level. We suggest that chromosome 1 harbours a critical domain whose integrity is essential for male fertility.

Published

2004

21. Phenotypic variability in Hey2 -/- mice and absence of HEY2 mutations in patients with congenital heart defects or Alagille syndrome

Author

Hartmut Fenge, Andreas Fischer, Barbara Klamt, Manfred Gessler, Christiane Glaeser, Nina Schumacher, and Ingo Hansmann

Subjects

Heart Defects, Congenital, JAG1, Adolescent, Biology, medicine.disease_cause, Polymerase Chain Reaction, Polymorphism, Single Nucleotide, Atrial septal defects, Exon, Mice, Alagille syndrome, Genetics, medicine, Basic Helix-Loop-Helix Transcription Factors, Animals, Humans, Point Mutation, Serrate-Jagged Proteins, HEY2, Child, Tetralogy of Fallot, Mice, Knockout, Mutation, Calcium-Binding Proteins, Infant, Membrane Proteins, DNA, Sequence Analysis, DNA, medicine.disease, Phenotype, Alagille Syndrome, Mice, Inbred C57BL, Repressor Proteins, Child, Preschool, Intercellular Signaling Peptides and Proteins, Jagged-1 Protein, Microsatellite Repeats

Abstract

The genetic alterations leading to congenital heart defects (CHD) are still poorly understood. We and others have recently shown that in mice loss of Hey2 results in a high incidence of fatal ventricular and atrial septal defects, combined with tricuspid stenosis or atresia in some cases. The phenotype has been postulated to resemble human tetralogy of Fallot. Our analysis of CD1 outbred mice suggests that phenotypic consequences of Hey2 loss can be quite variable and dependent on modifier genes as we detected only isolated VSDs with lower prevalence and a significantly reduced mortality rate in this strain. Since Hey2 is one of the few Notch target genes, it is also conceivable that HEY2 mutations may account for cases of Alagille syndrome (AGS: variable combinations of heart, skeleton, eye, and facial malformations and cholestasis), in which the typical mutations of the Notch ligand JAG1 cannot be found. To clarify the role of HEY2 in human CHD and AGS, we screened by direct sequencing 23 children with CHD and 38 patients diagnosed with AGS, which lack mutations in the JAG1 gene. We found two types of silent changes in the coding region: a CTT--CTG transition in exon 3 and a CTG--CTC polymorphism in exon 5. Furthermore, a heterozygous SNP in the splice donor site of exon 4 was detected that is unlikely to disrupt splicing. Although the high incidence and variability of human congenital heart defects implies a multifactorial genetic basis, our results suggest that mutation of HEY2 is not a major contributing factor.

Published

2004

22. Association of a specific haplotype across the genes MMP1 and MMP3 with radiographic joint destruction in rheumatoid arthritis

Author

Sylvia, Dörr, Nadine, Lechtenböhmer, Rolf, Rau, Gertraud, Herborn, Ulf, Wagner, Bertram, Müller-Myhsok, Ingo, Hansmann, and Gernot, Keyszer

Subjects

Adult, Aged, 80 and over, Male, rheumatoid arthritis, Polymorphism, Genetic, matrix metalloproteinase, HLA-DR1 Antigen, Middle Aged, Linkage Disequilibrium, Arthritis, Rheumatoid, Radiography, Haplotypes, allelic polymorphism, radiographic progression, HLA-DR4 Antigen, Humans, Female, Genetic Predisposition to Disease, Joints, Matrix Metalloproteinase 3, Matrix Metalloproteinase 1, Promoter Regions, Genetic, Alleles, Aged, Research Article

Abstract

The genetic background of rheumatoid arthritis (RA) is only partly understood, and several genes seem to be involved. The matrix metalloproteinases MMP1 (interstitial collagenase) and MMP3 (stromelysin 1) are thought to be important in destructive joint changes seen in RA. In the present study, functional relevant promoter polymorphisms of MMP1 and MMP3 were genotyped in 308 patients and in 110 controls, to test whether the polymorphisms contribute to the severity of the disease measured by radiographic progression of joint destruction. For comparison, the shared epitope of HLA DR4 and DR1 (SE) was determined by polymerase chain reaction. There was no association of MMP polymorphisms with susceptibility to RA. However, a strong linkage disequilibrium was observed between the 1G/2G (MMP1) and the 5A/6A (MMP3) polymorphisms (P << 10-6; linkage disequilibrium index D' = 0.46). In factorial regression, the degree of radiographic joint destruction correlated significantly with the 1G-5A haplotype (P = 0.0001) and the interaction term 'estimated number of 1G-5A haplotypes × duration of disease' (P = 0.0007). This association was phasic, indicating that possession of the 1G-5A haplotype has a protective effect over a period of about 15 years of RA, but might be associated with a more pronounced radiographic progression later on. Similar results were also found with the 1G allele of MMP1 alone (P = 0.015) and with the interaction term 'estimated number of 1G alleles × duration of disease' (P = 0.014). The correlation of SE with the Ratingen score was comparable (0.044). The regression model of MMP haplotypes explained 35% of the variance of the radiographic score, whereas the SE explained 29%. The 1G-5A haplotype across the closely linked MMP1 and MMP3 gene loci is a newly described genetic factor strongly associated with the progression of joint damage in RA. Our findings suggest that there are haplotypes in a MMP cluster region that modify the joint destruction in RA in a phasic manner.

Published

2003

23. Identification of 36 novel Jagged1 (JAG1) mutations in patients with Alagille syndrome

Author

Albrecht, Röpke, Annegret, Kujat, Mechthild, Gräber, Joannis, Giannakudis, and Ingo, Hansmann

Subjects

Alagille Syndrome, Calcium-Binding Proteins, DNA Mutational Analysis, Mutation, Humans, Intercellular Signaling Peptides and Proteins, Membrane Proteins, Proteins, Serrate-Jagged Proteins, Exons, Jagged-1 Protein

Abstract

Alagille syndrome (AGS) is an autosomal dominant disorder characterized by five major symptoms: cholestasis, vertebral deformity, heart malformations, ocular defects and peculiar facial appearance. The previously described Jagged1 (JAG1) gene on chromosome 20p12 has been identified as being responsible for AGS. JAG1 encodes a transmembrane protein acting as ligand for the evolutionarily conserved Notch signaling pathway. Here we report 36 novel mutations in the JAG1 gene. We identified 12 novel deletions, 4 insertions, 8 missense, 7 nonsense and 5 splice site mutations. All mutations map to the sequence encoding the extracellular part of the Jagged1 protein. The mutations spread over the entire gene with slightly increased rates in exons 2 to 6 and exon 23 and 24. Eight novel missense mutations map to the Delta-Serrate-Lag2 (DSL) domain and adjacent sequences which are important for ligand-receptor interaction. Inheritance was determined in 27 families. Sixteen mutations (55%) were de novo and eleven mutations (45%) were transmitted. Altogether 226 different JAG1 mutations have been described in association with AGS, including our novel 36 mutations. AGS variants are spread over the entire gene with only a few mutations in exon 26. A relatively high number of mutations are clustered in exons 2 to 6. This sequence region shows high interspecies conservation and encodes the Notch receptor-binding region (DSL domain).

Published

2002

24. Paternal isodisomy 7q secondary to monosomy 7 at recurrence in a Down syndrome child with acute myelogenous leukemia

Author

M. A. Esparza-Flores, Melva Gutiérrez-Angulo, Ingo Hansmann, G.J.R. González, Verónica Judith Picos-Cárdenas, María de la Luz Ayala-Madrigal, and J. P. Meza-Espinoza

Subjects

Male, Cancer Research, Down syndrome, Aneuploidy, Biology, Genetics, medicine, Humans, Molecular Biology, In Situ Hybridization, Fluorescence, Chromosome 7 (human), Polymorphism, Genetic, Karyotype, Uniparental Disomy, medicine.disease, Molecular biology, Uniparental disomy, Chromosome Banding, Leukemia, Myeloid, Acute, Uniparental Isodisomy, Child, Preschool, Down Syndrome, Haploinsufficiency, Trisomy, Chromosomes, Human, Pair 7

Abstract

We report a boy with Down syndrome and leukemia who acquired uniparental isodisomy of chromosome 7q as a secondary chromosomal change during recurrence of the disease. His karyotype before therapy was 46,XY,der(1)t(1;1)(p36;q32),−7,+21c[17]/46,idem,del(9)(p22)[10], whereas at recurrence it was 46,XY,der(1)t(1;1)(p36;q32,−7,der(7)(qter→p22∼pter::q10→qter),del(9)(p22),+21c[13]/47,XY,+21c[2]. By using polymerase chain reaction amplification of D7S493 and D7S527 markers, we identified the loss of the maternal chromosome 7 with a consequent paternal isodisomy in the clone with dup7q. This rearrangement could be implicated in the progression of the disease by causing (1) nullisomy for a gene or genes located on 7p22→pter, (2) functional double doses of exclusively paternal expressed genes, and (3) restoration of the effects produced by haploinsufficiency of biparental expressed genes.

Published

2002

25. Homologous sequences at human chromosome 9 bands p12 and q13-21.1 are involved in different patterns of pericentric rearrangements

Author

Markus Stumm, Christine Behrend, Heike Starke, Sylvia Reichardt, Wolfram Henn, Marianne Volleth, Thomas Liehr, Klaus R Sandig, Gabriele Senger, J. Seidel, Uwe Claussen, Beate Albrecht, Christine Kelbova, Anita Heller, and Ingo Hansmann

Subjects

Genetics, Chromosome Aberrations, Male, Derivative chromosome, Heterochromatin, Breakpoint, Chromosome, Chromosome 9, Biology, Homology (biology), Chromosome Banding, Sequence Homology, Nucleic Acid, Centromere, Humans, Female, Chromosomes, Human, Pair 9, Genetics (clinical), Recombination, In Situ Hybridization, Fluorescence

Abstract

A thorough study of the heterochromatin organisation in the pericentromeric region and the proximal long (q) and short (p) arms of human chromosome 9 (HSA 9) revealed homology between 9p12 and 9q13-21.1, two regions that are usually not distinguishable by molecular cytogenetic techniques. Furthermore, the chromosomal regions 9p12 and 9q13-21.1 showed some level of homology with the short arms of the human acrocentric chromosomes. We studied five normal controls and 51 clinical cases: 48 with chromosome 9 heteromorphisms, one with an exceptionally large inversion and two with an additional derivative chromosome 9. Using fluorescence in situ hybridisation (FISH) with three differentially labelled chromosome 9-specific probes we were able to distinguish 12 heteromorphic patterns in addition to the most frequent pattern (defined as normal). In addition, we studied one inversion 9 case with the recently described multicolour banding (MCB) technique. Our results, and previously published findings, suggest several hotspots for recombination in the pericentromeric heterochromatin of HSA 9. They also demonstrate that constitutional inversions affecting the pericentromeric region of chromosome 9 carry breakpoints located preferentially in 9p12 or 9q13-21.1 and less frequently in 9q12.

Published

2002

26. Kabuki syndrome-like features associated with a small ring chromosome X and XIST gene expression

Author

Hannelore Thiele, Paweł Stankiewicz, Ioannis Giannakudis, Heike Starke, Antje Krüger, Mike Schlicker, Ingo Hansmann, Sylvia Dörr, and Christiane Baldermann

Subjects

medicine.medical_specialty, RNA, Untranslated, X Chromosome, Ring chromosome, Gene Expression, Biology, Craniofacial Abnormalities, Intellectual Disability, medicine, Humans, Abnormalities, Multiple, Ring Chromosomes, Child, Genetics (clinical), X chromosome, Growth Disorders, In Situ Hybridization, Fluorescence, Genetics, medicine.diagnostic_test, Cytogenetics, Karyotype, Syndrome, medicine.disease, Uniparental disomy, Chromosome Banding, Cytogenetic Analysis, XIST, Female, RNA, Long Noncoding, Kabuki syndrome, Fluorescence in situ hybridization, Microsatellite Repeats, Transcription Factors

Abstract

Although clinical features in Kabuki syndrome (KS; Niikawa-Kuroki syndrome) have been well defined, the underlying genetic mechanism still remains unclear. We report a 9-year-old girl with typical KS-like facial appearance, skeletal and dermatoglyphic abnormalities, severe mental retardation, and growth deficiency. In 60 of 100 GTG-banded metaphases from peripheral blood lymphocytes, a ring chromosome smaller than a G group chromosome was found, which, according to reverse painting, consisted of Xq11.1q13. The proband's karyotype was described as mos45,X/46,X,+r(X). Several loci were analyzed with fluorescence in situ hybridization (FISH) and microsatellite markers revealing that one r(X) breakpoint mapped proximal to DXS422 (Xp11.21) and the second mapped distal to XIST gene, between loci DXS128E and DXS441 (Xq13.2). Uniparental disomy for X and r(X) was excluded and the paternal origin of r(X) was identified. XIST expression was demonstrated by nested reverse transcription polymerase chain reaction (RT-PCR) using primers spanning exons 5, 6i, and 6 in RNA prepared from lymphocytes. The observation of XIST expression is in contrast to two other cases in which the XIST gene was either not present on r(X) or not expressed. To our knowledge, this is the first case of Kabuki-like syndrome manifestations with r(X) and XIST expression.

Published

2001

27. Construction of a detailed physical and transcript map of the candidate region for Russell-Silver syndrome on chromosome 17q23-q24

Author

Claudia Färber, Alina T. Midro, Joannis Giannakudis, Sylvia Dörr, and Ingo Hansmann

Subjects

Genetics, Yeast artificial chromosome, Genetic Markers, alpha Karyopherins, Bacterial artificial chromosome, Contig, Translocation Breakpoint, Locus (genetics), Human artificial chromosome, Syndrome, Biology, Physical Chromosome Mapping, Translocation, Genetic, Chromosome 17 (human), Chromosomal region, Humans, Abnormalities, Multiple, Carrier Proteins, Growth Disorders, Chromosomes, Human, Pair 17, Gene Library

Abstract

Russell-Silver syndrome (RSS) is a heterogeneous disorder characterized mainly by pre- and postnatal growth retardation and characteristic dysmorphic features. The genetic cause of this syndrome is unknown. However, two autosomal translocations involving chromosome 17q25 were reported in association with RSS. Molecular analysis of the breakpoint on chromosome 17 of the de novo translocation previously described as t(1;17)(q31;q25) enabled us to refine the localization of the chromosome 17 breakpoint to 17q23-q24. Since no detailed mapping data were available for this region, we established a contig of yeast artificial chromosomes, P1 artificial chromosomes, bacterial artificial chromosomes, and cosmid clones for a 17q segment flanked by the sequence-tagged site (STS) markers D17S1557 and D17S940. This contig covers a physical distance of 4-5 Mb encompassing several novel markers. A transcript map was constructed by assigning genes and expressed sequence tags to the clone contig, and altogether 74 STS markers were mapped. Furthermore, the locus order and content provide insight into several duplication events that have occurred in the chromosomal region 17q23-q24. On the basis of our refined map, we have reduced the translocation breakpoint region to 65 kb between the newly derived markers 58T7 and CF20b. These data provide the molecular tools for the final identification of the RSS gene in 17q23-q24.

Published

2001

28. Maternal UPD 20 in a hyperactive child with severe growth retardation

Author

Gabriele Senger, Ilse Chudoba, S Demuth, Volkmar Beensen, G Sauerbrei, Uwe Claussen, Y Franke, Ingo Hansmann, and Annett Neumann

Subjects

Genetics, Chromosome Aberrations, Male, Growth retardation, Developmental Disabilities, Chromosomes, Human, Pair 20, Mothers, Karyotype, Child Behavior Disorders, Biology, Genomic Imprinting, Hyperactive child, Child, Preschool, Karyotyping, Centromere, Microsatellite, Humans, Chromosome 20, Genomic imprinting, Genetics (clinical), Microdissection, In Situ Hybridization, Fluorescence

Abstract

Maternal uniparental disomy was observed in a 4-year-old boy with severe pre- and postnatal growth retardation (body height: 85 cm = 12 cm < third percentile, head circumference: 48 cm = 10 cm < third percentile), a few minor facial findings, and with apparent hyperactivity. His intelligence is within the normal range for his age. Karyotype analysis revealed two cell lines, one apparently normal with 46,XY, the other with a tiny marker (47,XY, + mar). Microdissection and reverse chromosome painting using the marker DNA library as a probe, as well as PCR analysis revealed that the marker is from chromosome 20 and contains only the centromere and pericentromeric segments, but none of the pericentromeric loci for microsatellites. Microsatellite analysis of 25 chromosome 20 loci disclosed maternal uniparental disomy for all 16 informative markers. Maternal heterodisomy was evident for seven loci of the short arm segment 20p11.2-pter. Maternal isodisomy was found at five loci, three of them map to the proximal 20p11.2 segment and two to 20q. To our knowledge, this is the first case of maternal disomy 20 in humans.

Published

1999

29. Localization of Alagille syndrome to 20p11.2-p12 by linkage analysis of a three-generation family

Author

O. Daniëls, M.P.A. Geurds, Edwin C. M. Mariman, Ingo Hansmann, F.A.E. Nabben, Frans A. Hol, and Ben C.J. Hamel

Subjects

Male, Candidate gene, Chromosomes, Human, Pair 20, Chromosomal translocation, Locus (genetics), Biology, Translocation, Genetic, 03 medical and health sciences, Genetic linkage, Alagille syndrome, Genetics, medicine, Humans, 10. No inequality, Genetics (clinical), 030304 developmental biology, Netherlands, Sequence Deletion, 0303 health sciences, 030305 genetics & heredity, Breakpoint, Haplotype, Autosomal dominant trait, Chromosome Mapping, medicine.disease, Pedigree, Alagille Syndrome, Indonesia, Female, Lod Score

Abstract

Alagille syndrome (AGS) or arteriohepatic dysplasia is a rare but well-defined clinical entity that is usually inherited as an autosomal dominant trait. A limited number of patients carry a deletion in chromosome 20p, with 20p11.23-p12.2 as the area of minimal overlap. Recently, a family has been identified in which a balanced translocation with a breakpoint in 20p12 co-segregates with the AGS phenotype. Here, we report a three-generation family with AGS and in which the affected members have a normal karyotype. Linkage analysis was performed with markers from the 20p candidate region. A lod score of Z = 2.96 was obtained with D20S27 at no recombination. Combining D20S27 and D20S61 to a single highly informative locus resulted in a maximum lod score of Z = +3.56 at theta = 0.0. Haplotype analysis positioned AGS between D20S59 and D20S65, markers that define an interval of about 40 cM. Allelic loss was not observed for the tested markers and no abnormalities in the PAX1 candidate gene were detected. These findings demonstrate that the locus on chromosome 20p could be responsible for AGS in cytogenetically normal patients and argues for a general role of this locus in the aetiology of AGS.

Published

1995

30. Cystatin C (CST3), the candidate gene for hereditary cystatin C amyloid angiopathy (HCCAA), and other members of the cystatin gene family are clustered on chromosome 20p11.2

Author

Magnus Abrahamson, Ingo Hansmann, Susanne Schnittger, and Vvn Gopal Rao

Subjects

Chromosomes, Human, Pair 20, Locus (genetics), 03 medical and health sciences, 0302 clinical medicine, Gene mapping, Gene cluster, Genetics, Gene family, Humans, Cystatin C, In Situ Hybridization, Fluorescence, 030304 developmental biology, Southern blot, 0303 health sciences, biology, Chromosome Mapping, Hereditary cystatin C amyloid angiopathy, Molecular biology, Cystatins, Electrophoresis, Gel, Pulsed-Field, Blotting, Southern, Cerebral Amyloid Angiopathy, Multigene Family, biology.protein, Cystatin, DNA Probes, 030217 neurology & neurosurgery

Abstract

The cystatin C gene (CST3) encodes a low-molecular-weight cysteine proteinase inhibitor belonging to family II of the cystatin super family and is mutated in cases of hereditary cystatin C amyloid angiopathy (HCCAA). CST3, which along with other family II cystatin genes is a member of the cystatin gene family, has been assigned to chromosome 20. To investigate the genomic organization on chromosome 20, the CST3 gene and related sequences were regionally mapped by fluorescence in situ hybridization (FISH), Southern blot, and pulsed-field gel electrophoresis (PFGE) analysis using the cDNA cystatin C probe C6a and three genomic probes, C3E1, C3E2, and C3E2-2. Probe C3E2-2, which like probe C3E2 is specific for CST3, hybridized to only one Hind III and one XbaI fragment on Southern blots and to a 300-kb Bss HII PFGE fragment. FISH with probe C3E2 mapped this locus to chromosome 20p11.2, with an FL-pter value of 0.37 ± 0.07 on the physical map. Probe C3E1 containing the most conserved cystatin gene exon (exon 1) and its flanking sequences hybridized with more fragments, e.g., to eight Xba I and nine HindIII fragments on conventional Southern blots and to eight SmaI, two BssHII (900 and 300 kb), and two Not I fragments after PFGE. FISH with C3E1 revealed only one single site at 20p11.2 with an FL-pter value of 0.37 ± 0.04, identical to that obtained with C3E2. From these results it is concluded that (1) exon 1 and its flanking sequences are preferentially conserved within the cystatin gene family and that (2) CST3 and probably seven other members of the cystatin gene family are clustered within an at maximum 1.2-Mb segment on chromosome 20p11.2.

Published

1993

31. Pax1, a member of the paired box-containing class of developmental control genes, is mapped to human chromosome 20p11.2 by in situ hybridization (ISH and FISH)

Author

V.V.N.G. Rao, Ingo Hansmann, Peter Gruss, Rudi Balling, Urban Deutsch, and Susanne Schnittger

Subjects

Chromosomes, Human, Pair 20, Locus (genetics), Biology, Hybrid Cells, 03 medical and health sciences, Gene mapping, Cricetinae, Genetics, medicine, Animals, Humans, Paired Box Transcription Factors, In Situ Hybridization, In Situ Hybridization, Fluorescence, 030304 developmental biology, Chromosome 7 (human), 0303 health sciences, medicine.diagnostic_test, 030305 genetics & heredity, Genes, Homeobox, Chromosome Mapping, Molecular biology, Chromosome 17 (human), DNA-Binding Proteins, Chromosome 20, Chromosome 21, Chromosome 22, Fluorescence in situ hybridization, Transcription Factors

Abstract

Pax-1 , a member of a murine multigene family, belongs to the paired box-containing class of developmental control genes first identified in Drosophila . The Pax-1 gene encodes a sequence-specific DNA-binding protein with transcriptional activating properties and has been found to be mutated in the autosomal recessive mutation undulated (un) on mouse chromosome 2 with vertebral anomalies along the entire rostrocaudal axis. By radioactive in situ hybridization (ISH) using a fragment from the murine Pax-1 paired box that is almost identical to the respective sequences from the cognate human gene HuP48 and fluorescence in situ hybridization (FISH) using a complete mouse Pax-1 cDNA, we have assigned the human homologue of murine Pax-1 , the PAX1 locus, to chromosome 20p. The map position of PAX1 after FISH (FL-pter value of 0.34 ± 0.04) corresponds to band p11.2. These results confirm the exceptional homology between human chromosome 20 and the distal segment of mouse chromosome 2, extending from bands F to G, and add PAX1 to the group of genes on 20p like PTPA, PRNP, SCG1, BMP2A, which are located in proximity on both chromosomes.

Published

1992

32. The gene for bone morphogenetic protein 2A (BMP2A) is localized to human chromosome 20pl2 by radioactive and nonradioactive in situ hybridization

Author

Christiane Löffler, V.V.N. Gopal Rao, John M. Wozney, and Ingo Hansmann

Subjects

Genetics, 0303 health sciences, Decapentaplegic, Bone morphogenetic protein 8A, Bone morphogenetic protein 10, Autosomal dominant trait, Locus (genetics), Biology, Bone morphogenetic protein, BMPR1B, Cell biology, 03 medical and health sciences, Bone morphogenetic protein 6, 0302 clinical medicine, 030217 neurology & neurosurgery, Genetics (clinical), 030304 developmental biology

Abstract

Bone morphogenetic protein 2A (BMP2A), a member of the decapentaplegic-Vg-related family, belongs to the transforming growth factor beta superfamily and has a striking sequence similarity to the decapentaplegic locus in Drosophila melanogaster, a major determinant of pattern specification during embryogenesis. BMP2A is thought to be involved in cartilage and bone formation during embryogenesis, but may have additional functions in morphogenesis as implied by its expression in various organs and embryonic tissues of mice. Human BMP2A, assigned to chromosome 20 by the use of human-Chinese hamster ovary cell hybrids, is considered to be a reasonable candidate gene for the autosomal dominant disease of fibrodysplasia (myositis) ossificans progressiva. We have confirmed the localization of BMP2A to chromosome 20 and regionally assigned the locus to 20p12 by radioactive and nonradioactive in situ hybridization.

Published

1992

33. The human gene for oxytocin-neurophysin I (OXT) is physically mapped to chromosome 20p13 by in situ hybridization

Author

J. Battey, Christiane Löffler, V.V.N. Gopal Rao, and Ingo Hansmann

Subjects

medicine.medical_specialty, Neurophysin I, Chromosomes, Human, Pair 20, In situ hybridization, Biology, Oxytocin, 03 medical and health sciences, 0302 clinical medicine, Neurophysin II, Posterior pituitary, Internal medicine, Lactation, Genetics, medicine, Humans, Molecular Biology, Genetics (clinical), In Situ Hybridization, In Situ Hybridization, Fluorescence, Metaphase, 030304 developmental biology, Neurophysins, 0303 health sciences, Autosomal dominant trait, Chromosome Mapping, Molecular biology, Arginine Vasopressin, Endocrinology, medicine.anatomical_structure, Chromosome 20, hormones, hormone substitutes, and hormone antagonists, 030217 neurology & neurosurgery, medicine.drug

Abstract

Two posterior pituitary hormones oxytocin and arginine-vasopressin control the important activities of water excretion, parturition and lactation. Both these hormones are synthesized as inactive precursors in the hypothalamus along with their carrier proteins neurophysin I and neurophysin II respectively and are activated upon transport to posterior pituitary. Human genes for both oxytocin-neurophysin I (OXT) and arginine-vasopressin-neurophysin II (ARVP) are cloned and found to be linked on chromosome 20 separated by approximately 12 kb of intergenic sequences. Though OXT is not yet associated with any disease, ARVP is linked to the autosomal dominant disease neurohypophyseal diabetes insipidus (AD-NDI). We have mapped regionally the OXT locus to chromosome 20p13 by both radioactive (ISH) and fluorescence in situ hybridization (FISH).

Published

1992

34. Characterization and regional mapping of new anonymous chromosome 20-specific DNA markers isolated from a flow-sorted DNA library

Author

Susanne Schnittger, Hans-Peter Pfau, Ingo Hansmann, Frank-Michael Stolz, Gernot Reipen, and Karl-Heinz Grzeschik

Subjects

Genetic Markers, Male, Chromosomes, Human, Pair 20, Biology, Hybrid Cells, 03 medical and health sciences, chemistry.chemical_compound, Gene mapping, Genetics, Humans, Genomic library, Bacteriophages, Cloning, Molecular, 030304 developmental biology, Gene Library, 0303 health sciences, 030305 genetics & heredity, Chromosome, Chromosome Mapping, Flow Cytometry, Molecular biology, Chromosome Banding, Pedigree, Blotting, Southern, chemistry, Genetic marker, Female, Chromosome 20, Restriction fragment length polymorphism, Chromosome 22, DNA, Polymorphism, Restriction Fragment Length

Abstract

Employing the flow-sorted chromosome 20-specific DNA library LL20NS01, we isolated seven novel unique poly- and monomorphic DNA markers specific to human chromosome 20. Initially, 201 phage clones were analyzed regarding insert size and repetitivity. By testing 14 single- and low-copy number clones for their ability to detect RFLPs, three polymorphisms were revealed by two probes, pFMS22-1.4 [D20S22] and pFMS76 [D20S23]. Seven of twenty probes (35%) were assigned to chromosome 20 using a somatic cell hybrid DNA panel. Five of them were regionally mapped by in situ hybridization. Three DNA markers, pFMS51 [D20S29], pFMS76 [D20S23], and pFMS106 [D20S30], were assigned to 20p11.2-p12, and two markers, pFMS22-1.4 [D20S22] and pFMS135 [D20S31], to 20q12-q13.3. Our new chromosome 20-specific DNA markers should be useful for the molecular characterization of this rather underpopulated human chromosome.

Published

1991

35. The gene for the novel vasoactive peptide endothelin 3 (EDN3) is localized to human chromosome 20q13.2-qter

Author

Christiane Löffler, V.V.N. Gopal Rao, and Ingo Hansmann

Subjects

Chromosomes, Human, Pair 20, Neuropeptide, Biology, Hybrid Cells, 03 medical and health sciences, Mice, Gene mapping, Genetics, Gene family, Animals, Humans, education, Gene, 030304 developmental biology, 0303 health sciences, education.field_of_study, Endothelins, 030305 genetics & heredity, Chromosome Mapping, Molecular biology, Endothelin 1, Endothelin 3, Genes, Multigene Family, Chromosome 20, Endothelin receptor

Abstract

Endothelin 3 is a novel vasoactive peptide of unique structure and belongs to the endothelin gene family. Though it mainly functions as a vasoconstrictor/pressor, it plays a major role in a wide variety of other biological functions, possibly as a novel neuropeptide. Studies with human-mouse somatic cell hybrids have suggested that the gene EDN3 is localized on human chromosome 20. We confirmed this localization and regionally mapped the gene to the region 20q13.2–q13.3.

Published

1991

36. A sterile male with 45,X0 and a Y;22 translocation

Author

Ingo Hansmann, Joachim Arnemann, Georg Klaus Hinkel, Jörg Schmidtke, Susanne Schnittger, and Erika Tolkendorf

Subjects

Adult, Male, medicine.medical_specialty, Chromosomes, Human, Pair 22, Aneuploidy, Chromosomal translocation, Biology, Y chromosome, Polymerase Chain Reaction, Translocation, Genetic, 03 medical and health sciences, Y Chromosome, Genetics, medicine, Humans, Genetics (clinical), Infertility, Male, 030304 developmental biology, Southern blot, 0303 health sciences, Hybridization probe, 030305 genetics & heredity, Cytogenetics, Karyotype, medicine.disease, Molecular biology, Blotting, Southern, DNA Probes, Chromosome 22

Abstract

Cytogenetic analysis of a 20-year-old sterile male revealed a 45,X0 karyotype with no evidence for Y-chromosomal material on any of the chromosomes analysed by Q-, G- and C-banding. DNA analysis with 17 different Y chromosome-derived probes revealed the presence of Yp DNA sequences in the patient's genome. In situ hybridization with the Yp-derived probe pJA36B disclosed a translocation of Y-chromosomal material onto the short arm of a chromosome 22.

Published

1991

37. Mapping of the ribophorin II (RPN II) gene to human chromosome 20q12-q13.1 by in-situ hybridization

Author

Christiane Löffler, V.V.N. Gopal Rao, and Ingo Hansmann

Subjects

0303 health sciences, 030305 genetics & heredity, Chromosomes, Human, Pair 20, Chromosome, Chromosome Mapping, Membrane Proteins, Nucleic Acid Hybridization, Chromosomal translocation, In situ hybridization, Biology, Molecular biology, 03 medical and health sciences, Gene mapping, Complementary DNA, Genetics, Humans, Chromosome 20, Gene, Genetics (clinical), 030304 developmental biology, Synteny

Abstract

Ribophorin I and II (RPN I and RPN II), two specific glycoproteins, span the rough regions of the endoplasmic reticulum (RER) and are thought to play an important role either in translocation or in the maintenance of RER. Studies with human-mouse somatic cell hybrids have localized the gene for RPN I on human chromosome 3q, while RPN II is on chromosome 20. Using a radioactive labelled cDNA probe, we have regionally mapped the RPN II gene to human chromosome 20q12-q13.1 by in situ hybridization. This assignment predicts a location of the murine homologue, Rpn-2, to the syntenic segment on mouse chromosome 2 in close proximity to Ada, Src and Gnas.

Published

1991

38. The gene for human growth hormone-releasing factor (GHRF) maps to or near chromosome 20p12

Author

C. Löffler, Ingo Hansmann, S. Schnittger, and V.V.N.G. Rao

Subjects

Chromosomes, Human, Pair 20, Biology, Growth Hormone-Releasing Hormone, 03 medical and health sciences, Nucleic acid thermodynamics, Gene mapping, Complementary DNA, Genetics, Humans, 0501 psychology and cognitive sciences, 050102 behavioral science & comparative psychology, Molecular Biology, Gene, Genetics (clinical), 030304 developmental biology, 0303 health sciences, 05 social sciences, Chromosome, Chromosome Mapping, Nucleic Acid Hybridization, Karyotype, DNA, Growth hormone–releasing hormone, Molecular biology, Chromosome Banding, Chromosome 20, DNA Probes

Abstract

Growth hormone-releasing factor (GHRF), a hypothalamic releasing factor also named somatocrinin, influences the secretion and synthesis of growth hormone. Human GHRF is encoded by a single gene which was assigned to chromosome 20 by dot-blot analysis of DNA from dual laser sorted chromosomes. Using a radioactive cDNA probe, we localized the GHRF gene to chromosome 20p12 or near band 20p12.

Published

1991

39. Trisomy 4 due to nondisjunction during maternal meiosis II

Author

Ingo Hansmann and Iris Bartels

Subjects

Genetics, 0303 health sciences, Fetus, Meiosis II, 030305 genetics & heredity, Aneuploidy, Trisomy, Biology, medicine.disease, Abortion, Spontaneous, 03 medical and health sciences, Nondisjunction, Genetic, Meiosis, Nondisjunction, Pregnancy, medicine, Humans, Female, Chromosomes, Human, Pair 4, Genetics (clinical), 030304 developmental biology

Published

2008

40. An MspI and PstI RFLP detected by probe pFMS22–1.4 [D20S22]

Author

Frank-Michael Stolz and Ingo Hansmann

Subjects

0106 biological sciences, 0303 health sciences, Chromosomes, Human, Pair 20, Biology, Bioinformatics, 01 natural sciences, Deoxyribonuclease HpaII, 03 medical and health sciences, Genetics, Humans, Restriction fragment length polymorphism, DNA Probes, Deoxyribonucleases, Type II Site-Specific, Polymorphism, Restriction Fragment Length, 030304 developmental biology, 010606 plant biology & botany, Genes, Dominant

Published

1990

41. Twelve novelJAG1gene mutations in polish Alagille syndrome patients

Author

Ewa Popowska, Dorota Jurkiewicz, Małgorzata Krajewska-Walasek, Ingo Hansmann, and Christiane Gläser

Subjects

Genetics, JAG1, Mutation, Point mutation, Biology, Gene mutation, medicine.disease_cause, medicine.disease, Frameshift mutation, Genotype, Alagille syndrome, medicine, Jagged-1 Protein, Genetics (clinical)

Abstract

Alagille syndrome (AGS) is an autosomal dominant disorder with developmental abnormalities of the liver, heart, eyes, vertebrae, and face. Mutations in the JAG1 (Jagged 1) gene, coding a ligand in the evolutionarily conserved Notch signaling pathway, are responsible for AGS. Here we present sixteen different JAG1 gene mutations, among them twelve novel, not described previously. Seven frameshift: c. 172_178del7 (p.Ala58fs), c.509delT (p.Leu170fs), c.1197delG (p.Val399fs), c.1485_1486delCT (p.Pro495fs), c.1809_1810insTGGG (p.Lys604fs), c.2122_2125delCAGT (p.Gln708fs), c.2753delT (p.Ile918fs); five nonsense: c.383G>A (p.Trp128X), c.496C>T (p.Glu166X), c.841C>T (p.Gln281X), c.1207C>T (p.Gln403X), c.1603C>T (p.Gln535X); two splice site: c.388-1G>C, c.3048+1_3048+2insG and two missense mutations: c.359T>A (p.Ile120Asn), c.560G>A (p.Cys187Tyr) were found. Forty percent of the changes were identified in exons 2 and 4, the remaining mutations are distributed along the entire coding sequence of the gene. Seventy-five percent of the mutations lead to creation of premature termination codons. Family studies revealed that the specific mutations were inherited in 3 out of 11 investigated cases. No correlation between genotype and phenotype was observed.

Published

2005

42. [Untitled]

Author

Bertram Müller-Myhsok, Nadine Lechtenböhmer, Ulf Wagner, Ingo Hansmann, Gernot Keyszer, G. Herborn, Sylvia Dörr, and Rolf Rau

Subjects

medicine.medical_specialty, MMP3, Linkage disequilibrium, MMP1, Haplotype, Biology, medicine.disease, Rheumatology, Internal medicine, Rheumatoid arthritis, Immunology, medicine, Interstitial collagenase, Allele

Abstract

The genetic background of rheumatoid arthritis (RA) is only partly understood, and several genes seem to be involved. The matrix metalloproteinases MMP1 (interstitial collagenase) and MMP3 (stromelysin 1) are thought to be important in destructive joint changes seen in RA. In the present study, functional relevant promoter polymorphisms of MMP1 and MMP3 were genotyped in 308 patients and in 110 controls, to test whether the polymorphisms contribute to the severity of the disease measured by radiographic progression of joint destruction. For comparison, the shared epitope of HLA DR4 and DR1 (SE) was determined by polymerase chain reaction. There was no association of MMP polymorphisms with susceptibility to RA. However, a strong linkage disequilibrium was observed between the 1G/2G (MMP1) and the 5A/6A (MMP3) polymorphisms (P << 10-6; linkage disequilibrium index D' = 0.46). In factorial regression, the degree of radiographic joint destruction correlated significantly with the 1G-5A haplotype (P = 0.0001) and the interaction term 'estimated number of 1G-5A haplotypes × duration of disease' (P = 0.0007). This association was phasic, indicating that possession of the 1G-5A haplotype has a protective effect over a period of about 15 years of RA, but might be associated with a more pronounced radiographic progression later on. Similar results were also found with the 1G allele of MMP1 alone (P = 0.015) and with the interaction term 'estimated number of 1G alleles × duration of disease' (P = 0.014). The correlation of SE with the Ratingen score was comparable (0.044). The regression model of MMP haplotypes explained 35% of the variance of the radiographic score, whereas the SE explained 29%. The 1G-5A haplotype across the closely linked MMP1 and MMP3 gene loci is a newly described genetic factor strongly associated with the progression of joint damage in RA. Our findings suggest that there are haplotypes in a MMP cluster region that modify the joint destruction in RA in a phasic manner.

Published

2004

43. Identification of 36 novel Jagged1 (JAG1) mutations in patients with Alagille syndrome

Author

Ingo Hansmann, Mechthild Gräber, Joannis Giannakudis, Albrecht Röpke, and Annegret Kujat

Subjects

Genetics, JAG1, Heart malformation, Notch signaling pathway, Biology, medicine.disease, Molecular biology, Exon, Alagille syndrome, medicine, Jagged-1 Protein, Missense mutation, Gene, Genetics (clinical)

Abstract

Alagille syndrome (AGS) is an autosomal dominant disorder characterized by five major symptoms: cholestasis, vertebral deformity, heart malformations, ocular defects and peculiar facial appearance. The previously described Jagged1 (JAG1) gene on chromosome 20p12 has been identified as being responsible for AGS. JAG1 encodes a transmembrane protein acting as ligand for the evolutionarily conserved Notch signaling pathway. Here we report 36 novel mutations in the JAG1 gene. We identified 12 novel deletions, 4 insertions, 8 missense, 7 nonsense and 5 splice site mutations. All mutations map to the sequence encoding the extracellular part of the Jagged1 protein. The mutations spread over the entire gene with slightly increased rates in exons 2 to 6 and exon 23 and 24. Eight novel missense mutations map to the Delta-Serrate-Lag2 (DSL) domain and adjacent sequences which are important for ligand-receptor interaction. Inheritance was determined in 27 families. Sixteen mutations (55%) were de novo and eleven mutations (45%) were transmitted. Altogether 226 different JAG1 mutations have been described in association with AGS, including our novel 36 mutations. AGS variants are spread over the entire gene with only a few mutations in exon 26. A relatively high number of mutations are clustered in exons 2 to 6. This sequence region shows high interspecies conservation and encodes the Notch receptor-binding region (DSL domain). © 2002 Wiley-Liss, Inc.

Published

2002

44. Erratum: Parental mosaicism of JAG1 mutations in families with Alagille syndrome

Author

Helen E. Hughes, Mike Schlicker, Agnes Bankier, Joannis Giannakudis, Małgorzata Krajewska-Walasek, Jean-Pierre Fryns, Annegret Kujat, Ingo Hansmann, David J. Amor, and Albrecht Röpke

Subjects

Genetics, JAG1, business.industry, media_common.quotation_subject, Alagille syndrome, medicine, medicine.disease, Legend, business, Genetics (clinical), media_common

Abstract

Figure 6 in the above paper was printed with an incorrect legend. The figure and legend are reproduced correctly below.

Published

2001

45. The gene for receptor-linked protein-tyrosine-phosphatase (PTPA) is assigned to human chromosome 20p12-pter by in situ hybridization (ISH and FISH)

Author

Jan Sap, Ingo Hansmann, V.V.N. Gopal Rao, Joseph Schlessinger, and Christiane Lo¨ffler

Subjects

chemistry.chemical_classification, In situ, 0303 health sciences, 030305 genetics & heredity, Chromosomes, Human, Pair 20, Chromosome Mapping, Nucleic Acid Hybridization, Chromosome, In situ hybridization, Protein tyrosine phosphatase, Biology, Molecular biology, 03 medical and health sciences, Enzyme, Gene mapping, chemistry, Genetics, Humans, Protein Tyrosine Phosphatases, Receptor, Gene, 030304 developmental biology

Published

1992

46. The polymorphic DNA sequence D20S14 is assigned to human chromosome 20p12→p11.2 by in situ hybridization

Author

V.V.N.G. Rao, Ingo Hansmann, and C. Löffler

Subjects

Genetic Markers, Genetics, 0303 health sciences, Polymorphism, Genetic, Genetic Linkage, 030302 biochemistry & molecular biology, Chromosomes, Human, Pair 20, Chromosome Mapping, Nucleic Acid Hybridization, Locus (genetics), Biology, Molecular biology, Chromosome 17 (human), 03 medical and health sciences, Nucleic acid thermodynamics, Gene mapping, Genetic marker, Humans, Human genome, Chromosome 20, Molecular Biology, Chromosome 22, Genetics (clinical), 030304 developmental biology

Abstract

The polymorphic DNA marker D20S14 was previously mapped to human chromosome 20 and shown to be linked to two other DNA markers, D20S5 and D20S6, located at 20p12. This segment has been implicated in several human diseases. Because of its importance, we mapped the D20S14 locus to 20p12→p11.2 by radioactive in situ hybridization.

Published

1992

47. Excess of females in chromosomally normal spontaneous abortuses

Author

Bernd Eiben, Ingo Hansmann, and Iris Bartels

Subjects

0303 health sciences, Fetus, medicine.medical_specialty, Pregnancy, 030219 obstetrics & reproductive medicine, Obstetrics, Abortion, Biology, medicine.disease, Abortion, Spontaneous, 03 medical and health sciences, 0302 clinical medicine, Endocrinology, Internal medicine, medicine, Chromosomes, Human, Humans, Female, Sex Ratio, Genetics (clinical), Sex ratio, 030304 developmental biology

Published

1990

48. Errata

Author

Ingo Hansmann, Gopalrao V.N. Velagaleti, Susanne Schnittger, and Magnus Abrahamson

Subjects

Genetics, Candidate gene, Cystatin B, Cystatin C, biology, Cystatin A, biology.protein, Gene family, Genomics, Cystatin, Hereditary cystatin C amyloid angiopathy, Molecular biology

Published

1993

49. Subject Index Vol. 61, 1992

Author

Elizabeth Baker, D. Benova, Wendy Stock, Settara C. Chandrasekharappa, Raju Kucherlapati, David F. Callen, Alessandra M.V. Duncan, J. Battey, S. Natsuume-Sakai, L.L. Anderson, H. Winking, Carol A. Westbrook, M. Koleva, Howard P. Levy, Kenneth W. Harder, Hélène Hayes, Christiane Löffler, G.R. Sutherland, V.V.N. Gopal Rao, E. Petit, Ingo Hansmann, V.M. Chapman, T. Shiomi, Roy Layfield, Y.-N. Harada, W. L. Neuman, I.G. Melhado, M M Le Beau, John S. Mattick, U. Hirning-Folz, Yoichi Matsuda, Maimon M. Cohen, W.L. Neuman, Roger A. Schultz, Robert M. Gemmill, Peter F. Nixon, Ian W. Craig, Frank R. Jirik, Bernard H. Brownstein, N. Lemieux, Robert Williamson, N.M. Lapsys, Horst Hameister, M. Abedinia, Bernard Dutrillaux, and Kyeryoung Lee

Subjects

Index (economics), Statistics, Genetics, Subject (documents), Biology, Molecular Biology, Genetics (clinical)

Published

1992

50. Influence of antisense mos oligos on oocyte maturation in the mouse

Author

Bernd Grüning, Brigitte Pabst, and Ingo Hansmann

Subjects

medicine.anatomical_structure, Chemistry, Oligonucleotide, medicine, Cell Biology, Oocyte, Cell biology

Published

1990