Your search keyword '"M. Leipoldt"' showing total 51 results

1. Two novel translocation breakpoints upstream of SOX9 define borders of the proximal and distal breakpoint cluster region in campomelic dysplasia

Author

James R. Lupski, M Theurl, Gabriel A. Bien-Willner, Pawel Stankiewicz, AL Shanske, AH Lane, Svetlana A. Yatsenko, M Leipoldt, M Erdel, Marta Smyk, and Gerd Scherer

Subjects

Male, Molecular Sequence Data, Chromosomal translocation, SOX9, Biology, Translocation, Genetic, Genetics, medicine, Humans, Abnormalities, Multiple, In Situ Hybridization, Fluorescence, Genetics (clinical), Bone Diseases, Developmental, Base Sequence, medicine.diagnostic_test, Breakpoint, High Mobility Group Proteins, Infant, Newborn, breakpoint cluster region, Infant, SOX9 Transcription Factor, Karyotype, Sequence Analysis, DNA, Sex reversal, medicine.disease, Radiography, Campomelic dysplasia, Female, Chromosomes, Human, Pair 17, Transcription Factors, Fluorescence in situ hybridization

Abstract

The semilethal skeletal malformation syndrome campomelic dysplasia (CD) with or without XY sex reversal is caused by mutations within the SOX9 gene on 17q24.3 or by chromosomal aberrations (translocations, inversions or deletions) with breakpoints outside the SOX9 coding region. The previously published CD translocation breakpoints upstream of SOX9 fall into two clusters: a proximal cluster with breakpoints between 50-300 kb and a distal cluster with breakpoints between 899-932 kb. Here, we present clinical, cytogenetic and molecular data from two novel CD translocation cases. Case 1 with karyotype 46,XY,t(1;17)(q42.1;q24.3) has characteristic symptoms of CD, including mild tibial bowing, cryptorchidism and hypospadias. By standard fluorescence in situ hybridization (FISH) and by high-resolution fiber FISH, the 17q breakpoint was mapped 375 kb from SOX9, defining the centromeric border of the proximal breakpoint cluster region. Case 2 with karyotype 46,X,t(Y;17)(q11.2;q24.3) has the acampomelic form of CD and complete XY sex reversal. By FISH and somatic cell hybrid analysis, the 17q breakpoint was mapped 789 kb from SOX9, defining the telomeric border of the distal breakpoint cluster region. We discuss the structure of the 1 Mb cis-control region upstream of SOX9 and the correlation between the position of the 14 mapped translocation breakpoints with respect to disease severity and XY sex reversal.

Published

2006

2. Extended Pedigree with Multiple Cases of XX Sex Reversal in the Absence of SRY and of a Mutation at the SOX9 Locus

Author

W.J. Jin, Halil Saglam, Nizamettin Kılıç, M. Leipoldt, Tuna Gulten, Gerd Scherer, E. Bausch, Tahsin Yakut, and Sehime Gulsun Temel

Subjects

Genetics, endocrine system, Embryology, Gonad, urogenital system, Endocrinology, Diabetes and Metabolism, Locus (genetics), social sciences, SOX9, Biology, Sex reversal, Embryonic stem cell, medicine.anatomical_structure, Testis determining factor, parasitic diseases, medicine, Gene, geographic locations, Developmental Biology

Abstract

It is well established that testicular differentiation of the human embryonic gonad depends on the action of the Y-chromosomal gene SRY. However, exceptional cases such as SRY-negative cases of 46,XX testicular disorder of sexual development (DSD), and of 46,XX ovotesticular DSD document that testicular tissue can develop in the absence of the SRY gene. These SRY-negative XX sex reversal cases are very rare and usually sporadic, but a few familial cases have been reported. We present a large, consanguineous family with nine affected individuals with phenotypes ranging from 46,XX testicular DSD to 46,XX ovotesticular DSD, with predominance of male characteristics. Absence of SRY in peripheral blood was documented by fluorescence in situ hybridization (FISH) and PCR analysis in all nine affected individuals, and by FISH analysis on gonadal sections with testicular tissue in four affected individuals. By quantitative PCR, a duplication of the SOX9 gene was excluded. In addition, as linkage analysis showed that the nine affected members of the family do not share a common SOX9 haplotype, any mutation at the SOX9 locus could be ruled out. Together, these findings implicate a mutation at a sex-determining locus other than SRY and SOX9 as the cause for the XX sex reversal trait in this family.

Published

2006

3. Abstracts of Other Papers Delivered

Author

Y. Rumpler, S. Atsalis, Helga Schulze, Joanna Fietz, Michelle Bayes, Michael Günther, Matthew J. Anderson, Robin H. Crompton, L.T. Nash, E. Zimmermann, Marie-Luise Kopp, H. Neveu, Christopher R. Birkinshaw, Lesley Ambrose, Robert W. Sussman, P.M. Kappeler, W. Scheffrahn, N. Rakotoarison, Ian C. Colquhoun, M. Leipoldt, B. Ludes, Russell Savage, W.I. Sellers, J. Schmid, Andreas Christian, Patrice Antilahimena, J.K. Hodges, Holger Preuschoft, R.L. Ange, Iain R. Spears, Kimberley Nekaris, E. Jean Wickings, Marc Godinot, S.S. Waters, L. Bachmann, K.A. Weisenseel, B. Meier, P Poorman-Allen, Jörg U. Ganzhorn, Ruth Dorcas Warren, J.C. Masters, C.D. Buesching, Bernhard Meier, I. Wilden, Josephine R. Andrews, Elke Zimmermann, J.S. Varley, Michelle L. Sauther, Radoslaw Ratajszczak, Elwyn L. Simons, Josephine Andrews, Alexandra Nietsch, Simon K. Bearder, C. Rabarivola, J. Tomiuk, Dang Huy Huynh, M. Heistermann, Achim Johann, C. Langer, Alison Jolly, F. Bayart, T. Hafen, Carl J. Erickson, Roland Wirth, Ian Tattersall, E.J. Sterling, D. Tab Rasmussen, J.U. Ganzhorn, Wolfgang Scheffrahn, Sharon Gursky, M.K. Izard, Gerald Doyle, Jürgen Tomiuk, and Leanne T. Nash

Subjects

Geography, Animal Science and Zoology, Ecology, Evolution, Behavior and Systematics

Published

1998

4. Contents Vol. 93, 2001

Author

T. Brueckmann, W. Brenner, M. Steinemann, W. Vogel, S. Schlaubitz, C. Zühlke, M. Lombard, F. Boán, K. Benirschke, S. Naumann, S.W. Bremer, C. Steinlein, S. Steinemann, F. Richard, P.D. Thomsen, M. Yerle, K.D. Zang, Z. Docherty, C. Amid, K. Mrasek, I. Schubert, M. Mende, I. Nanda, T. Paiss, C. Genêt, L.J. Peelman, I. Chudoba, M. Hughes, R.-D. Wegner, U. Claussen, L. Sánchez, B. Seipel, F. Grützner, F.J. García-Cozar, D. Prawitt, B.U. Zabel, J.L. Wright, A. Van Zeveren, K. Stout, V. Kalscheuer, M. Stumm, R.V. Rambau, N. Reissmann, D.S. Gallagher, B. Zabel, A. Ishikawa, C. Messaoudi, A.T. Kumamoto, E.C. Akeson, A. Mujica, A. Dalski, P. Kaiser, T. Liehr, J.G. Scammell, S. Bremer, C. Pfeifer, S. Munsche, M.M. Valdivia, M. Van Poucke, M. Schmid, C.M. Tuck-Muller, H. Starke, F. Domínguez, Y. Matsuda, S. Störkel, C.G. Mathew, F.F.B. Elder, S. Narayanswami, H. Scherthan, J. Decker, E. Schwinger, A. Niveleau, V. Trifonov, H. Mayrhofer, J. Gómez-Márquez, J.P. Lambert, S.-E. Bikar, E. Zend-Ajusch, L.J. Bechtel, T. Haaf, Y.A. Wang, A. Viñas, C. Iglesias, C. Mackie Ogilvie, A. Bahr, T. Nagase, A. Dufke, H.H.Q. Heng, A. Winterpacht, W. Lu, T.J. Robinson, C. Maier, K. Matsubara, A. Heller, A. Kuroiwa, M. Rocchi, B. Dutrillaux, C.J. Ye, N. Nomura, N. Rubtsov, E.R. Schmidt, T. Namikawa, M.T. Davisson, C. Tuggle, K. Gardiner, H. Enders, G. Liu, M. Buceta, H. Hanson, H. Hauser, N. Sampson, H. Neitzel, P.D. Waters, T. Hankeln, H. Tönnies, C. Pendón, J. Bolívar, M.L. Houck, D. Reutzel, M. Leipoldt, A. Cichutek, P. Moens, J.A.M. Graves, P.J. Kirby, B. Maurer, A. Astola, S.A. Krawetz, and F. Piumi

Subjects

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

Published

2001

5. Unusual chromosomal mosaicism as a cause of mental retardation and congenital malformations in a familial reciprocal translocation carrier, t(17;22)(q24.2;q11.23)

Author

Herbert Enders, Andreas Dufke, M Leipoldt, P. Kaiser, and H Mayrhofer

Subjects

Male, Adolescent, Derivative chromosome, Chromosomes, Human, Pair 22, Chromosomal translocation, Biology, Translocation, Genetic, Intellectual Disability, Genetics, Homologous chromosome, medicine, Humans, Abnormalities, Multiple, Crossing Over, Genetic, Molecular Biology, In Situ Hybridization, Fluorescence, Genetics (clinical), Mosaicism, Meiosis II, Infant, Newborn, Infant, Chromosome, Karyotype, medicine.disease, Uniparental disomy, Chromosome Banding, Nondisjunction, Child, Preschool, Karyotyping, Chromosomes, Human, Pair 17

Abstract

Familial reciprocal translocations are generally without phenotypic effect, although there is some evidence for a small excess of mental retardation and congenital malformations (MR/CM) in children carrying familial reciprocal translocations. Possible mechanisms whereby such translocations could have a phenotypic effect include cryptic unbalanced rearrangements, uniparental disomy, and disruption of putative genes at the breakpoints, unmasking recessive alleles on the normal homologs. Mosaicism for a supernumerary derivative chromosome in a carrier of a familial reciprocal translocation has not yet been described. We report a boy presenting with MR/CM and a familial reciprocal translocation, t(17;22)(q24.2;q11.23), inherited from the mother. Cytogenetic analysis of peripheral blood lymphocytes showed a balanced karyotype in all 32 analyzed metaphase spreads. Molecular genetic analysis was consistent with biparental origin of the normal homologs. In metaphase spreads from skin fibroblasts a supernumerary chromosome was found in all 24 cells analyzed and could be identified as der(22)t(17;22)(q24.2;q11.23). Several possible segregation modes at meiosis I followed by meiosis II or postzygotic nondisjunction of the der(22) might have led to this unusual chromosomal mosaicism. We propose hidden mosaicism as a possible cause for MR/CM in patients who apparently carry a balanced familial reciprocal translocation.

Published

2001

6. Identification of subtelomere rearrangements in patients with idiopathic mental retardation

Author

R Korinthenberg, Heymut Omran, Andrea Superti-Furga, B Zabel, M Leipoldt, S Unger, and K Storm van's Gravesande

Subjects

business.industry, Pediatrics, Perinatology and Child Health, Medicine, Identification (biology), In patient, Neurology (clinical), General Medicine, Subtelomere, Bioinformatics, business

Published

2008

7. Extended pedigree with multiple cases of XX sex reversal in the absence of SRY and of a mutation at the SOX9 locus

Author

S G, Temel, T, Gulten, T, Yakut, H, Saglam, N, Kilic, E, Bausch, W J, Jin, M, Leipoldt, and G, Scherer

Subjects

Adult, Doublecortin Domain Proteins, Male, Adolescent, Reverse Transcriptase Polymerase Chain Reaction, Neuropeptides, Disorders of Sex Development, High Mobility Group Proteins, SOX9 Transcription Factor, Hormones, Sex-Determining Region Y Protein, Pedigree, Gene Expression Regulation, Haplotypes, Child, Preschool, Cytogenetic Analysis, Mutation, Testis, Humans, Female, Child, Microtubule-Associated Proteins, Transcription Factors

Abstract

It is well established that testicular differentiation of the human embryonic gonad depends on the action of the Y-chromosomal gene SRY. However, exceptional cases such as SRY-negative cases of 46,XX testicular disorder of sexual development (DSD), and of 46,XX ovotesticular DSD document that testicular tissue can develop in the absence of the SRY gene. These SRY-negative XX sex reversal cases are very rare and usually sporadic, but a few familial cases have been reported. We present a large, consanguineous family with nine affected individuals with phenotypes ranging from 46,XX testicular DSD to 46,XX ovotesticular DSD, with predominance of male characteristics. Absence of SRY in peripheral blood was documented by fluorescence in situ hybridization (FISH) and PCR analysis in all nine affected individuals, and by FISH analysis on gonadal sections with testicular tissue in four affected individuals. By quantitative PCR, a duplication of the SOX9 gene was excluded. In addition, as linkage analysis showed that the nine affected members of the family do not share a common SOX9 haplotype, any mutation at the SOX9 locus could be ruled out. Together, these findings implicate a mutation at a sex-determining locus other than SRY and SOX9 as the cause for the XX sex reversal trait in this family.

Published

2006

8. Loss of chromosomes in clear cell renal cell carcinoma and in corresponding renal parenchyma

Author

G, Feil, M, Leipoldt, H J, Nelde, A, Wunderer, H W, Wechsel, P, Kaiser, and K H, Bichler

Subjects

Male, Chromosome Mapping, Loss of Heterozygosity, Middle Aged, Kidney, Kidney Neoplasms, Karyotyping, Y Chromosome, Humans, Female, Chromosome Deletion, Carcinoma, Renal Cell, Adenocarcinoma, Clear Cell, Aged

Abstract

Chromosome studies were done on six renal cell carcinomas (RCC) and on the corresponding renal parenchymas of the tumor bearing kidneys. Histopathologically, all tumors belonged to the clear cell subtype. All examined parenchymas were pathologically benign. None of the tumor cells showed the typical chromosomal aberrations described for (nonpapillary) RCC, i.e. deletions in the short arm of chromosome #3, or gains in the long arm of chromosome #5. In our series both the tumor and the benign kidney tissues were characterized by loss of chromosomes, especially of the chromosomes #6, #9, #16, #20, and of the Y chromosome. Trisomy of chromosome #7 was found frequently in benign parenchyma cells. The identical chromosomal changes in the tumor and in the parenchyma tissues might reflect rather in vivo mosaics rather than primary chromosomal aberrations in the oncogenetic process of clear cell RCC.

Published

1999

9. The evaluation of gonosomal mosaics: lymphocyte interphase nuclei analyzed by FISH

Author

Peter Kaiser, M. Schliephacke, Jürgen Tomiuk, C. I. M. Maier, M. Leipoldt, and G. Majlinger

Subjects

In situ, Adult, Male, Adolescent, Satellite DNA, Lymphocyte, Biology, Risk Factors, Genetics, medicine, Humans, Lymphocytes, Interphase, Genetics (clinical), In Situ Hybridization, Fluorescence, Cell Nucleus, medicine.diagnostic_test, Mosaicism, Hybridization probe, Molecular biology, medicine.anatomical_structure, %22">Fish , Female, Gonadoblastoma, Molecular probe, Fluorescence in situ hybridization

Abstract

The reliable evaluation of chromosomal mosaics is still considered to be difficult in clinical diagnosis if aberrant metaphases are only present at low frequencies. Classical cytogenetic findings cannot significantly exclude low mosaic levels, obviously, because of the relatively low number of analyzed metaphases. To study this problem, the number of gonosomes in lymphocyte interphase nuclei was determined by FISH (fluorescence in situ hybridization) application of two satellite DNA probes, DXZ1 and DYZ1. The results obtained with this method from lymphocytes of clinically and cytogenetically inconspicuous persons showed a high degree of reliability. The DNA probe yielded correct signals in more than 95% of the analyzed nuclei. Additionally, patients were examined who showed cytogenetically confirmed numerical gonosome aberrations. These results were compared with those obtained from the control group of inconspicuous patients and discussed with respect to the evaluation of gonosomal mosaics.

Published

1996

10. Immunohistochemical and cytogenetic findings in malignant rhabdoid tumor

Author

E, Kaiserling, P, Ruck, R, Handgretinger, M, Leipoldt, and R, Hipfel

Subjects

Male, Cytogenetics, Humans, Infant, Female, Soft Tissue Neoplasms, Immunohistochemistry, Kidney Neoplasms, Rhabdoid Tumor

Abstract

The histogenesis of malignant rhabdoid tumor (RT) remains a matter of controversy. From published reports it appears that some extrarenal RT (ERRT) exhibit neural or neuroectodermal features. Systematic investigation of renal RT (RRT) for neural differentiation has not yet been published. In this study, two RRT and two ERRT were investigated by light and electron microscopy, immunocytochemistry, and cytogenetic analysis.All four cases exhibited similar morphology and a largely consistent immunohistochemical staining profile. Both tumor types showed immunoreactivity for various cytokeratins, epithelial membrane antigen (EMA), vimentin, neurofilaments, S100 protein, neuron specific enolase, Leu7, CD34, p53, MB2, MIC2, VS38c, laminin and fibronectin. Reactivity was usually confined to a small proportion of the tumor cells, especially in the case of antibodies against neurofilaments, NSE, S100 proteins Leu7, CD34 and p53. Only a few of the antibodies (anti-vimentin, MB2, MIC2, anti-EMA, and VS38c) stained the majority of the tumor cells. Chromosome analysis revealed a discrete aberration in 11p (most probably a paracentric inversion in 11p15) in the one RRT investigated. One ERRT had a normal karyotype, but the other one exhibited various structural abnormalities on chromosomes 18 and 22.The immunohistochemical investigations revealed many similarities between RRT and ERRT, and all four tumors investigated exhibited neuroectodermal differentiation. As far as histogenetic classification is concerned, our findings point in the direction of the group of tumors that includes Ewing's sarcoma and primitive neuroectodermal tumors.

Published

1996

11. Genetic intervention in human beings

Author

M. Leipoldt

Subjects

Sociology of scientific knowledge, Human biology, Intervention (counseling), Eugenics, Psychological intervention, Context (language use), Engineering ethics, Human genome, Genetic discrimination, Psychology

Abstract

Various aspects of human biology and medicine will be influenced by the information provided by the Human Genome Project regarding the entire human DNA sequence. In addition to scientific knowledge, the primary benefit for the community will lie in improvements in the diagnosis and therapy of monogenic as well as multifactorially inherited genetic disorders including many forms of cancer. An overview of the first five years is presented here and the achievements regarding DNA-based diagnosis, screening and therapy are discussed. The consequences for medical practice are outlined and placed in the context of individual, familial and social concerns. It is emphasized, however, that practicable interventions in human genomes leading to broad and long-term consequences are at present not a realistic possibility due to insufficient albeit rapidly improving technology. Negative developments could arise in the form of various kinds of genetic discrimination pending the revival of old and persisting eugenic concepts.

Published

1996

12. Subject Index Vol. 93, 2001

Author

N. Sampson, W. Lu, H. Neitzel, P.D. Waters, T. Brueckmann, W. Brenner, C. Mackie Ogilvie, A. Heller, H. Tönnies, B. Dutrillaux, M. Steinemann, C. Pendón, J. Bolívar, R.-D. Wegner, M. Lombard, C.J. Ye, A. Ishikawa, E. Zend-Ajusch, T. Nagase, Y.A. Wang, F. Richard, A. Kuroiwa, N. Rubtsov, E.R. Schmidt, C. Tuggle, C. Genêt, K. Gardiner, H. Enders, B. Zabel, A. Van Zeveren, M. Rocchi, H. Scherthan, A. Dalski, R.V. Rambau, J.P. Lambert, K. Stout, A. Dufke, B. Seipel, F.F.B. Elder, J.L. Wright, T. Namikawa, H. Hauser, E. Schwinger, M. Buceta, C. Pfeifer, S. Narayanswami, A.T. Kumamoto, H. Starke, V. Kalscheuer, J.G. Scammell, M. Stumm, K. Matsubara, V. Trifonov, C. Amid, K. Mrasek, G. Liu, A. Bahr, T. Haaf, A. Viñas, C. Iglesias, Z. Docherty, H. Mayrhofer, P. Kaiser, S.-E. Bikar, I. Chudoba, C.M. Tuck-Muller, J. Decker, L.J. Bechtel, H.H.Q. Heng, A. Winterpacht, M.M. Valdivia, C. Messaoudi, D. Reutzel, M. Van Poucke, C. Steinlein, S. Störkel, U. Claussen, T.J. Robinson, J.A.M. Graves, A. Niveleau, F. Grützner, A. Mujica, N. Nomura, W. Vogel, S. Naumann, M. Hughes, E.C. Akeson, S. Steinemann, I. Nanda, S. Bremer, S. Munsche, S.W. Bremer, P.D. Thomsen, F.J. García-Cozar, D. Prawitt, B.U. Zabel, B. Maurer, A. Astola, T. Liehr, F. Domínguez, M.T. Davisson, H. Hanson, T. Hankeln, L.J. Peelman, M.L. Houck, N. Reissmann, Y. Matsuda, J. Gómez-Márquez, M. Leipoldt, A. Cichutek, K.D. Zang, P. Moens, T. Paiss, D.S. Gallagher, M. Schmid, C.G. Mathew, S.A. Krawetz, F. Piumi, S. Schlaubitz, C. Zühlke, F. Boán, K. Benirschke, M. Yerle, I. Schubert, M. Mende, P.J. Kirby, L. Sánchez, and C. Maier

Subjects

Genetics, Index (economics), Subject (documents), Social science, Biology, Molecular Biology, Genetics (clinical)

Published

2001

13. Schnelle Karyotyp-Analyse aus Nabelschnurblut

Author

M. Leipoldt, C. Rotsch, and P. Müller

Abstract

Chromosomenaberrationen treten bei Neugeborenen mit einer Inzidenz von etwa 6 auf 1000 auf. Mehr als ein Drittel dieser Falle zeigt schwerwiegende phanotypische Effekte als Folge von autosomalen Trisomien und unbalancierten Strukturveranderungen. Die zytogenetische Diagnose erfolgt in der Regel aus peripheren Lymphozyten nach konventioneller 72 h-Kultur, in Fallen von pranatal durch Sonographie festgestellten Fehlbildungen auch aus kultivierten Zellen nach Amniozentese oder Plazentabiopsie sowie aus fetalem Nabelschnurblut. Verbesserte sonographische Diagnostik fuhrt in zunehmendem Mase dazu, das Chromo-somenstorungen als Ursache kindlicher Fehlbildungen zum Zeitpunkt der Geburt als Ergebnis pranataldiagnostischer Masnahmen bereits nachgewiesen sind. Dennoch ergibt sich immer wieder die Konstellation bei Geburt eines komplex fehlgebildeten Kindes unmittelbar notwendiger Masnahmen bei nicht abgeklartem zytogenetischen Befund. Hier ist eine im Vergleich mit der 72 h-Blutkultur beschleunigte Karyotypisierung ebenso hilfreich wie eine schnelle zytogenetische Diagnosestellung unter Umgehung von Langzeitkulturen in der Schwangerschaftsspatphase im Hinblick auf das Geburtsmanagement. Die Erfahrungen zur schnellen Karyotypisierung Neugeborener haben entweder bei Verwendung von Knochenmarksaspirat (Francke et al. 1979) keinen Eingang in die Routinediagnostik gefunden oder sie basieren bei Verwendung von Nabelschnurblut (Garn-ham u. Sutherland 1987) auf einer geringen Anzahl untersuchter Falle.

Published

1991

14. Prenatal diagnosis and postnatal follow-up of a child with two de novo unrelated balanced reciprocal translocations

Author

B. Zoll, M. Pruggmayer, M. Leipoldt, and Ulrike Thies

Subjects

Proband, Adult, Pathology, medicine.medical_specialty, Physiology, Chromosomal translocation, Prenatal diagnosis, Biology, Translocation, Genetic, 03 medical and health sciences, Pregnancy, medicine, Humans, Genetics (clinical), 030304 developmental biology, 0303 health sciences, Chromosomes, Human, Pair 15, medicine.diagnostic_test, Chromosomes, Human, Pair 10, 030305 genetics & heredity, Cytogenetics, Obstetrics and Gynecology, Chromosome, Karyotype, Gene rearrangement, Karyotyping, Amniocentesis, Female, Chromosomes, Human, Pair 3, Chromosomes, Human, Pair 17

Abstract

Two unrelated, apparently balanced, reciprocal translocations involving chromosomes 3 and 17, and 10 and 15 were found in cultured amniotic fluid cells from a 41-year-old 10-gravida. Chromosome analysis of peripheral blood lymphocytes of both parents revealed normal katryotypes. Post-partum examination of lymphocyte cultures from the proband confirmed the chromosome rearrangements. The child showed normal development during follow-up examinations up to the age of 4 years.

Published

1990

15. Ribosomal RNA structure in the diploid and phylogenetically polyploid amphibian species Hyla and Odontophrynus

Author

M. Kellner and M. Leipoldt

Subjects

Physiology, Zoology, Biology, Kidney, Hyla chrysoscelis, Biochemistry, Amphibians, Odontophrynus, Species Specificity, Polyploid, parasitic diseases, Animals, Ceratophrys ornata, Molecular Biology, Phylogeny, Genetics, Ovary, fungi, food and beverages, General Medicine, Ribosomal RNA, biology.organism_classification, Hyla, Diploidy, Liver, Organ Specificity, RNA, Ribosomal, Female, Ploidy, Odontophrynus americanus

Abstract

1. 1. Ribosomal RNA of the diploid amphibian species Hyla chrysoscelis and Odontophrynus americanus is structurally modified by hidden breaks. 2. 2. Phylogenetically polyploid related species like the tetraploid Hyla versicolor, the tetraploid Odontophrynus americanus and the octoploid Ceratophrys ornata do not show hidden breaks in ribosomal RNA. 3. 3. Structural modifications of rRNA molecules in diploid amphibians has no detectable effect on the ribosomal activity in vitro.

Published

1984

16. Satellited Y chromosomes: Structure, origin, and clinical significance

Author

Werner Schempp, Michael Schmid, Thomas Haaf, Eva Solleder, M. Leipoldt, and H. Heilbronner

Subjects

Male, Adolescent, Euchromatin, Heterochromatin, DNA, Satellite, Biology, Translocation, Genetic, 03 medical and health sciences, Y Chromosome, Centromere, Nucleolus Organizer Region, Genetics, Humans, Sex Chromosome Aberrations, Genetics (clinical), 030304 developmental biology, 0303 health sciences, Autosome, 030305 genetics & heredity, Chromosome, Karyotype, Chromosome Banding, Pedigree, Karyotyping, Nucleolus organizer region, Satellite chromosome

Abstract

Three cases of inherited satellited Y chromosomes (Yqs) were analysed using several cytogenetic techniques. The cytogenetic data of the 14 cases of Yqs chromosomes described to date were reviewed. All Yqs chromosomes carry an active nucleolus organizer region (NOR) in their long arm and must have developed from translocations involving the short arms of the acrocentric autosomes. The structure of the heterochromatic satellite region in the Yqs chromosomes shows conspicuous inter-familial differences; this permits the reconstruction of the translocations from which the various Yqs were derived. Some causal factors leading to the development of Yqs chromosomes are considered: the specific localization of the four satellite DNAs and highly methylated DNA sequences in the karyotype, and some new experimental data on the spatial arrangement of heterochromatic regions in interphase nuclei. These provide distinct evidence for a preferential involvement of the autosomes 15 and 22 in the translocations with the Y heterochromatin. All clinical reports documenting Yqs males born with malformations were reviewed. It appears that the presence of an extra NOR and NOR-associated heterochromatin in the Yqs chromosomes does not cause any phenotypic abnormalities (as long as the Y euchromatin is intact). The possibility that a Yqs chromosome predisposes to non-disjunction and/or to translocations of other chromosomes is discussed.

Published

1984

17. Towards an understanding of the molecular mechanisms regulating gene expression during diploidization in phylogenetically polyploid lower vertebrates

Author

M. Leipoldt

Subjects

Transcription, Genetic, Cyprinidae, Genome, Amphibians, Birds, Polyploidy, 03 medical and health sciences, Polyploid, Phylogenetics, biology.animal, Gene duplication, Genetics, Animals, Humans, Gene, Phylogeny, Genetics (clinical), 030304 developmental biology, 0303 health sciences, Models, Genetic, biology, fungi, 030302 biochemistry & molecular biology, Fishes, Gene Amplification, food and beverages, Vertebrate, pathological conditions, signs and symptoms, Evolution of mammals, Gene Expression Regulation, RNA, Ribosomal, Evolutionary biology, Ploidy

Abstract

Polyploidization and regional gene duplication have occurred frequently during vertebrate evolution, providing the genetic material necessary for creating evolutionary novelties. Mammals, including man, can be regarded as diploid species with a polyploid history of evolution. Polyploidization steps during the phylogeny of mammals probably took place in the genomes of amphibian- or fish-like mammalian ancestors. The polyploid status has subsequently been shaped by the process of diploidization, leading to genomes that are polyploid with respect to the amount of genetic material and the number of gene copies, and diploid with respect to the level of gene expression and chromosomal characteristics. Phylogenetically tetraploid amphibian and teleost species together with their diploid close relatives can be used as a model system to study the effect of polyploidization and the mechanisms of diploidization of a parallel event during early mammalian evolution. Experimental evidence permits the assumption that the diploidization of gene expression in tetraploid cyprinid fish may be functionally correlated with structural modifications of the ribosomal components, RNA and protein. These findings are discussed in the light of reduced protein synthesis in diploidized tetraploid species and a mechanism to explain diploidization during mammalian evolution.

Published

1983

18. Wissenschaftlicher Teil

Author

P. Albert, C. Pake, K. Rotte, K. Reusch, K. -D. Schulz, H. H. Zippel, E. Doppelfeld, R. Kaiser, M. Albrecht, G. Trams, A. Kleinkauf-Houken, K. Thomsen, M. Kaufmann, P. Drings, W. Queißer, H. Lochbühler, F. Kubli, D. Fournier, H. Sievers, P. Wöllgens, R. Nedden, A. Nessler, P. J. Pfuhl, D. Thüre, H. Kuttig, S. Wysocki, J. Heep, R. Blobel, U. Abel, K. Brunnert, G. Lammers, D. Gammert, W. Audretsch, H. Erdmann, H. H. zippel, G. Crombach, E. Burrenkopf, P. Schmidt-Rhode, H. Nienhaus, W. Holzgreve, F. K. Beller, F. -K. Klöck, H. Rotthaus, J. Timmermann, M. Leipoldt, M. Ludovico, M. Bauer, K. zum Winkel, O. Späh, A. Müller, N. K. Schöndorf, St. Gräber, H. Eckel, M. Volk, J. Scheuffele, G. Rossbach, G. Bastert, H. Naujoks, W. Kühn, G. Leppien, H. H. Rummel, G. Dick, U. D. Koenig, S. Erdman, U. Koldovský, J. Hilkens, H. G. Bender, H. Matthiessen, J. Hilgers, M. Spielmann, H. -J. Kitschke, K. Tietje, W. Meier, H. Würz, A. Fuchs, H. Geyer, J. L. Wittliff, A. Pfleiderer, R. -T. Michel, H. P. Fortmeyer, M. Stegmüller, H. Schmidt-Matthiesen, C. Lapp, D. S. Alberts, R. Ceschan, R. Goebel, H. Caffier, W. Kleine, R. Jerabek, G. Daxenbichler, C. Marth, R. Callies, A. Röthig, G. X. Zeller, K. A. Walz, L. Heilmann, U. Kock, W. E. Simon, F. Hölzel, K. Maillot, J. Süssenbach, U. Ochs, L. Wolnik, R. Eulenburg, C. -P. Janisch, R. Friedland, P. -G. Knapstein, D. Heberling, K. Wurster, M. Grewe, J. Rieth, J. Zander, I. Pichlmayr, S. Pohl, U. Steude, H. A. Hirsch, H. O. Klein, A. Hettenbach, W. Wiest, K. Kupka, K. Böhme, H. U. Lohmann, H. Behrendt, W. Homann, E. H. Schmidt, C. Stening, L. Beck, D. Henschler, R. Kreienberg, F. Melchert, A. Feige, E. Rose, I. Haubitz, J. Gille, W. Burkert, J. Hilfrich, H. K. Weitzel, A. Majewski, G. Horner, H. Brandau, G. Sturm, A. Werner, L. Matzanke, B. Seegert, E. Schuster, H. Wellmann, D. Krebs, A. Bichler, D. Fuchs, A. Hausen, H. Hetzel, G. Reibnegger, H. Wachter, H. F. Nauth, R. E. Herzog, S. Stange, D. Dagy, H. -A. Ladner, H. G. Hillemanns, T. Bauknecht, H. G. Meerpohl, and T Bauknecht

Subjects

business.industry, Obstetrics and Gynecology, Medicine, General Medicine, business

Published

1983

19. Amount of repeated and non-repeated DNA in the genomes of closely related fish species with varying genome sizes

Author

W. Engel, J. Schmidtke, E. Schmitt, and M. Leipoldt

Subjects

Guanine, Physiology, Cyprinidae, Fish species, Bacterial genome size, In Vitro Techniques, Biology, Biochemistry, Genome, DNA sequencing, Cytosine, chemistry.chemical_compound, Species Specificity, Animals, Molecular Biology, Genome size, Genetics, Base Composition, fungi, DNA, General Medicine, Genes, chemistry, C-value, Ploidy

Abstract

1. 1. Within the teleostean family Cyprinidae , diploid species occur with wide variation in genome size. There also exist species which were anciently tetraploid. 2. 2. The quantitative changes of DNA content in the diploids are primarily due to differences in the amount of intermediately repeated DNA. DNA sequence composition of the ancient tetraploid genomes suggests that the species derived from diploid ancestors of small genome size. 3. 3. The average base composition and the base compositional heterogeneity are similar in all the species examined.

Published

1979

20. Kinetic analysis of nucleolar rna polymerase I in diploid and phylogenetically tetraploid fish species

Author

A. Ebrecht and M. Leipoldt

Subjects

chemistry.chemical_classification, Ostariophysi, biology, Physiology, Nucleolus, Fish species, General Medicine, biology.organism_classification, Biochemistry, Molecular biology, chemistry.chemical_compound, Enzyme, chemistry, Phylogenetics, RNA polymerase, RNA polymerase I, Ploidy, Molecular Biology

Abstract

1. 1. Using whole purified nucleoli the K m and V max values of RNA polymerase I in various species of Isospondyli and Ostariophysi were evaluated to be 17–33 μ M UTP and 29 800 pM UTP/min x mg, respectively. 2. 2. RNA polymerase 1 in fish species is not inhibited by low concentrations of α-amanitin. 3. 3. RNA polymerase I can be purified from isolated nucleoli by solubilization, (NH 4 ) 2 SO 2 -precipitation and Sephadex-chromatography 60–80-fold. 4. 4. The kinetic properties of partially pure RNA polymerase do not differ considerably from those obtained with whole nucleoli.

Published

1984

21. Comparative analysis of ribosomal RNA in various fish and other vertebrate species: Hidden breaks and ribosomal function in phylogenetically tetraploid species of Cyprinidae

Author

H.G. Kellner, S. Stark, and M. Leipoldt

Subjects

Genetics, biology, Physiology, Somatic cell, Vertebrate, General Medicine, Ribosomal RNA, biology.organism_classification, Biochemistry, Ribosome, 18S ribosomal RNA, Phylogenetics, biology.animal, Cyprinidae, Ploidy, Molecular Biology

Abstract

1. 1. Ribosomal RNA of tetraploid species of Cyprinidae is modified by hidden breaks. A fraction of about 90% of the large rRNA molecules and about 50% of the small rRNA molecules shows hidden breaks in somatic cells. 2. 2. Germ cell rRNA is not modified by hidden breaks in tetraploid cyprinid fish. 3. 3. Diploid species of Cyprinidae either do not show detectable amounts of labile rRNA or have a fraction of 20–30% of 28 S rRNA modified by hidden breaks. 4. 4. Hidden breaks could not be detected in the rRNA of various other fish species, including diploid and tetraploid members of the order Isospondyli and not in the rRNA of several representatives of different vertebrate classes. 5. 5. Ribosomes isolated from somatic cells of tetraploid cyprinid fish show a reduced translational activity in vitro.

Published

1984

22. Comparative DNA/DNA reassociation kinetics in three hamster species

Author

M. Schmid, R. Eckhardt, and M. Leipoldt

Subjects

Physiology, Hamster, Biochemistry, Genome, Homology (biology), Chinese hamster, chemistry.chemical_compound, Cricetulus, Species Specificity, Cot analysis, Cricetinae, Animals, Repeated sequence, Molecular Biology, Genetics, biology, Base Sequence, Mesocricetus, General Medicine, DNA, biology.organism_classification, Molecular biology, chemistry, Liver, Nucleic Acid Renaturation, Nucleic Acid Conformation

Abstract

1. 1. Three major DNA repetition classes can be distinguished in the genomes of three hamster species Mesocricetus auratus, Cricetulus griseus , and Phodopus sungorus sungorus : A very fast reassociating fraction of about 13% of the DNA, a fast reassociating fraction comprising 10-23% of the DNA, and a slowly reassociating fraction containing single-copy sequences of 63-78% of hamster DNA. 2. 2. In the DNA of the Syrian and Djungarian hamster 43%-53%, and in the DNA of the Chinese hamster 80% of the single-copy sequences are interspersed with repetitive sequences. 3. 3. The lengths of repetitive DNA sequences, vary between more than 3 kb and 0.3 kb, with the majority of sequences having a length of 0.3 kb to 0.5 kb kb. 4. 4. The findings suggest that the genomes of the hamster species studied are organized in a short period interspersion pattern. 5. 5. Unlike other vertebrate and invertebrate genomes, moderately repetitive sequences exhibit a high degree of intraspecific homology in the hamster genome.

Published

1982

23. Pontine Tegmental Cap Dysplasia in an Extremely Preterm Infant and Review of the Literature.

Author

Picker-Minh S, Hartenstein S, Proquitté H, Fröhler S, Raile V, Kraemer N, Apeshiotis S, Leipoldt M, Kalache KD, Morris-Rosendahl D, Boltshauser E, Chen W, and Kaindl AM

Subjects

Cerebellum diagnostic imaging, Developmental Disabilities diagnostic imaging, Female, Humans, Infant, Extremely Premature, Infant, Newborn, Magnetic Resonance Imaging, Pontine Tegmentum diagnostic imaging, Cerebellum abnormalities, Muscle Hypotonia diagnostic imaging, Nervous System Malformations diagnostic imaging, Pontine Tegmentum abnormalities

Abstract

Pontine tegmental cap dysplasia is a rare hindbrain malformation syndrome with a hypoplastic pons, a tissue protrusion into the fourth ventricle, and cranial nerve dysfunction. We here report clinical, imaging, and genetic findings of the first extremely low-birth-weight preterm infant with pontine tegmental cap dysplasia born at 25 weeks of gestation and provide an overview of 29 sporadic cases. A prenatally diagnosed hypoplastic and rostrally shifted cerebellum was indicative of a hindbrain defect and later identified as an early sign of pontine tegmental cap dysplasia in our patient. The neonate exhibited severe muscle hypotonia, persistent thermolability, and clinical signs of an involvement of facial, cochlear, and hypoglossal nerves. Furthermore, paroxysmal episodes of agonizing pain with facial tics, tonic and clonic muscle contractions, blepharospasm, and singultus are highlighted as new phenotypic features of pontine tegmental cap dysplasia. With our report, we present a severe case of pontine tegmental cap dysplasia and provide a brief overview of current knowledge on this rare disease.

Published

2017

24. Clinical and Genetic Heterogeneity of the 15q13.3 Microdeletion Syndrome.

Author

Hassfurther A, Komini E, Fischer J, and Leipoldt M

Abstract

The 15q13.3 microdeletion is a recurrent CNV, presumably mediated by NAHR between segmental duplications in chromosome 15. The 15q13.3 deletion and duplication are associated with a wide range of clinical manifestations, such as intellectual deficits, seizures, autism, language and developmental delay, neuropsychiatric impairments, and behavioral problems illustrating incomplete penetrance and expressivity. This study comprises an evaluation of 106 symptomatic patients carrying the heterozygous deletion, as well as of 21 patients carrying the duplication, who have been described in previous studies. The analysis shows considerable heterogeneity for the manifestation of different key symptoms and familiar occurrence. Furthermore, 8 new patients are introduced. Convoluted familiar connections give new insights into the complexity of symptomatic manifestation. In previous studies, different opinions have been expressed as to the nature and precise location of the deletion breakpoints. Here, we show that not CHRNA7 and CHRFAM7A, but rather FAM7A or GOLGA8, serve as breakpoint regions concerning our patients. The deletion is described as heterogeneous in size. However, we assume that not only different breakpoints but also the imprecision of aCGH analysis on chromosome 15 due to segmental duplications accounts for the variability in size.

Published

2016

25. Mutations in CERS3 cause autosomal recessive congenital ichthyosis in humans.

Author

Radner FP, Marrakchi S, Kirchmeier P, Kim GJ, Ribierre F, Kamoun B, Abid L, Leipoldt M, Turki H, Schempp W, Heilig R, Lathrop M, and Fischer J

Subjects

ADAMTS Proteins, Animals, Genes, Recessive, Homozygote, Humans, Mutation, Organ Specificity, Polymorphism, Single Nucleotide, RNA Splice Sites genetics, RNA, Long Noncoding genetics, Sphingolipids metabolism, Sphingosine N-Acyltransferase metabolism, Tunisia, ADAM Proteins genetics, Genome-Wide Association Study, Ichthyosiform Erythroderma, Congenital genetics, Sphingosine N-Acyltransferase genetics

Abstract

Autosomal recessive congenital ichthyosis (ARCI) is a rare genetic disorder of the skin characterized by abnormal desquamation over the whole body. In this study we report four patients from three consanguineous Tunisian families with skin, eye, heart, and skeletal anomalies, who harbor a homozygous contiguous gene deletion syndrome on chromosome 15q26.3. Genome-wide SNP-genotyping revealed a homozygous region in all affected individuals, including the same microdeletion that partially affects two coding genes (ADAMTS17, CERS3) and abolishes a sequence for a long non-coding RNA (FLJ42289). Whereas mutations in ADAMTS17 have recently been identified in autosomal recessive Weill-Marchesani-like syndrome in humans and dogs presenting with ophthalmologic, cardiac, and skeletal abnormalities, no disease associations have been described for CERS3 (ceramide synthase 3) and FLJ42289 so far. However, analysis of additional patients with non-syndromic ARCI revealed a splice site mutation in CERS3 indicating that a defect in ceramide synthesis is causative for the present skin phenotype of our patients. Functional analysis of patient skin and in vitro differentiated keratinocytes demonstrated that mutations in CERS3 lead to a disturbed sphingolipid profile with reduced levels of epidermis-specific very long-chain ceramides that interferes with epidermal differentiation. Taken together, these data present a novel pathway involved in ARCI development and, moreover, provide the first evidence that CERS3 plays an essential role in human sphingolipid metabolism for the maintenance of epidermal lipid homeostasis., Competing Interests: The authors have declared that no competing interests exist.

Published

2013

26. Multigene deletions on chromosome 20q13.13-q13.2 including SALL4 result in an expanded phenotype of Okihiro syndrome plus developmental delay.

Author

Borozdin W, Graham JM Jr, Böhm D, Bamshad MJ, Spranger S, Burke L, Leipoldt M, and Kohlhase J

Subjects

Child, Preschool, Duane Retraction Syndrome pathology, Female, Humans, Infant, Infant, Newborn, Male, Nucleic Acid Hybridization, Phenotype, Chromosomes, Human, Pair 20 genetics, Developmental Disabilities complications, Developmental Disabilities genetics, Duane Retraction Syndrome complications, Duane Retraction Syndrome genetics, Gene Deletion, Transcription Factors genetics

Abstract

Okihiro syndrome results from truncating mutations in the SALL4 locus on the chromosome 20q13.13-q13.2. Deletions of the whole SALL4 coding region as well as single exon deletions are also a common cause of Okihiro syndrome and indicate haploinsufficiency as the disease causing mechanism. The phenotypes caused by SALL4 deletions are not different from those caused by point mutations. No multigene deletion including SALL4 has been documented to date. Here we report the detection and molecular characterization of four novel, overlapping microdeletions, all spanning SALL4 and flanking genes, in four unrelated cases with features of Okihiro syndrome and variable degrees of psychomotor delay. All deletions were first identified and mapped by quantitative Real Time PCR. Subsequently, three of four deletions were mapped in further detail by high-resolution array CGH (244k oligo-arrays). All cases had larger deletions of varying size (1.76-1.78 Mb, 2.01-2.05 Mb, 2.16-2.17 Mb, and 1.3-2.8 Mb, respectively), which included SALL4 plus 3 to 7 additional functional genes. While three cases with largely overlapping deletions are mildly developmentally delayed, the only patient with a more centromeric deletion is clearly mentally retarded. In this patient, four genes (MOCS3, DPM1, ADNP, BCAS4) are deleted, which were not affected in the other three cases, suggesting that the deletion of one or more of these genes contributes to the mental retardation. Since two of the four cases presented with choanal atresia, large deletions including SALL4 should be considered in the differential diagnosis of children with suspected CHARGE syndrome but without detectable CHD7 mutations.

Published

2007

27. Extended pedigree with multiple cases of XX sex reversal in the absence of SRY and of a mutation at the SOX9 locus.

Author

Temel SG, Gulten T, Yakut T, Saglam H, Kilic N, Bausch E, Jin WJ, Leipoldt M, and Scherer G

Subjects

Adolescent, Adult, Child, Child, Preschool, Cytogenetic Analysis, Doublecortin Domain Proteins, Female, Gene Expression Regulation, Haplotypes, High Mobility Group Proteins metabolism, Hormones blood, Humans, Male, Microtubule-Associated Proteins genetics, Microtubule-Associated Proteins metabolism, Neuropeptides genetics, Neuropeptides metabolism, Reverse Transcriptase Polymerase Chain Reaction, SOX9 Transcription Factor, Sex-Determining Region Y Protein genetics, Sex-Determining Region Y Protein metabolism, Testis pathology, Transcription Factors metabolism, Disorders of Sex Development, High Mobility Group Proteins genetics, Mutation genetics, Pedigree, Sex-Determining Region Y Protein deficiency, Transcription Factors genetics

Abstract

It is well established that testicular differentiation of the human embryonic gonad depends on the action of the Y-chromosomal gene SRY. However, exceptional cases such as SRY-negative cases of 46,XX testicular disorder of sexual development (DSD), and of 46,XX ovotesticular DSD document that testicular tissue can develop in the absence of the SRY gene. These SRY-negative XX sex reversal cases are very rare and usually sporadic, but a few familial cases have been reported. We present a large, consanguineous family with nine affected individuals with phenotypes ranging from 46,XX testicular DSD to 46,XX ovotesticular DSD, with predominance of male characteristics. Absence of SRY in peripheral blood was documented by fluorescence in situ hybridization (FISH) and PCR analysis in all nine affected individuals, and by FISH analysis on gonadal sections with testicular tissue in four affected individuals. By quantitative PCR, a duplication of the SOX9 gene was excluded. In addition, as linkage analysis showed that the nine affected members of the family do not share a common SOX9 haplotype, any mutation at the SOX9 locus could be ruled out. Together, these findings implicate a mutation at a sex-determining locus other than SRY and SOX9 as the cause for the XX sex reversal trait in this family., ((c) 2007 S. Karger AG, Basel)

Published

2007

28. Two novel translocation breakpoints upstream of SOX9 define borders of the proximal and distal breakpoint cluster region in campomelic dysplasia.

Author

Leipoldt M, Erdel M, Bien-Willner GA, Smyk M, Theurl M, Yatsenko SA, Lupski JR, Lane AH, Shanske AL, Stankiewicz P, and Scherer G

Subjects

Abnormalities, Multiple diagnostic imaging, Base Sequence, Female, Humans, In Situ Hybridization, Fluorescence, Infant, Infant, Newborn, Male, Molecular Sequence Data, Radiography, SOX9 Transcription Factor, Sequence Analysis, DNA, Abnormalities, Multiple genetics, Bone Diseases, Developmental genetics, Chromosomes, Human, Pair 17 genetics, High Mobility Group Proteins genetics, Transcription Factors genetics, Translocation, Genetic genetics

Abstract

The semilethal skeletal malformation syndrome campomelic dysplasia (CD) with or without XY sex reversal is caused by mutations within the SOX9 gene on 17q24.3 or by chromosomal aberrations (translocations, inversions or deletions) with breakpoints outside the SOX9 coding region. The previously published CD translocation breakpoints upstream of SOX9 fall into two clusters: a proximal cluster with breakpoints between 50-300 kb and a distal cluster with breakpoints between 899-932 kb. Here, we present clinical, cytogenetic and molecular data from two novel CD translocation cases. Case 1 with karyotype 46,XY,t(1;17)(q42.1;q24.3) has characteristic symptoms of CD, including mild tibial bowing, cryptorchidism and hypospadias. By standard fluorescence in situ hybridization (FISH) and by high-resolution fiber FISH, the 17q breakpoint was mapped 375 kb from SOX9, defining the centromeric border of the proximal breakpoint cluster region. Case 2 with karyotype 46,X,t(Y;17)(q11.2;q24.3) has the acampomelic form of CD and complete XY sex reversal. By FISH and somatic cell hybrid analysis, the 17q breakpoint was mapped 789 kb from SOX9, defining the telomeric border of the distal breakpoint cluster region. We discuss the structure of the 1 Mb cis-control region upstream of SOX9 and the correlation between the position of the 14 mapped translocation breakpoints with respect to disease severity and XY sex reversal.

Published

2007

29. Contiguous hemizygous deletion of TBX5, TBX3, and RBM19 resulting in a combined phenotype of Holt-Oram and ulnar-mammary syndromes.

Author

Borozdin W, Bravo-Ferrer Acosta AM, Seemanova E, Leipoldt M, Bamshad MJ, Unger S, and Kohlhase J

Subjects

Abnormalities, Multiple diagnosis, Child, Female, Gene Deletion, Heart Defects, Congenital diagnosis, Heart Defects, Congenital genetics, Humans, Male, Pedigree, Phenotype, Radiography, Syndrome, Upper Extremity Deformities, Congenital diagnosis, Upper Extremity Deformities, Congenital diagnostic imaging, Abnormalities, Multiple genetics, Nuclear Proteins genetics, RNA-Binding Proteins genetics, T-Box Domain Proteins genetics, Upper Extremity Deformities, Congenital genetics

Published

2006

30. Detection of heterozygous SALL1 deletions by quantitative real time PCR proves the contribution of a SALL1 dosage effect in the pathogenesis of Townes-Brocks syndrome.

Author

Borozdin W, Steinmann K, Albrecht B, Bottani A, Devriendt K, Leipoldt M, and Kohlhase J

Subjects

Codon, Facies, Female, Genes, Dominant, Homozygote, Humans, Male, Mutation, Phenotype, Point Mutation, Syndrome, Abnormalities, Multiple genetics, DNA Mutational Analysis methods, Gene Dosage, Heterozygote, Reverse Transcriptase Polymerase Chain Reaction methods, Transcription Factors genetics

Abstract

Townes-Brocks syndrome (TBS) is an autosomal dominantly inherited disorder characterized by ear, anal, limb, and renal malformations, and results from mutations in the gene SALL1. All SALL1 mutations previously found in TBS patients create preterminal termination codons. In accordance with the findings of pericentric inversions or balanced translocations, TBS was initially assumed to be caused by SALL1 haploinsufficiency. This assumption was strongly contradicted by a Sall1 mouse knock-out, because neither hetero- nor homozygous knock-out mutants displayed a TBS-like phenotype. A different mouse mutant mimicking the human SALL1 mutations, however, showed a TBS-like phenotype in the heterozygous situation, suggesting a dominant-negative action of the mutations causing TBS. We applied quantitative real time PCR to detect and map SALL1 deletions in 240 patients with the clinical diagnosis of TBS, who were negative for SALL1 mutations. Deletions were found in three families. In the first family, a 75 kb deletion including all SALL1 exons had been inherited by two siblings from their father. A second, sporadic patient carried a de novo 1.9-2.6 Mb deletion including the whole SALL1 gene, and yet another sporadic case was found to carry an intragenic deletion of 3384 bp. In all affected persons, the TBS phenotype is rather mild as compared to the phenotype resulting from point mutations. These results confirm that SALL1 haploinsufficiency is sufficient to cause a mild TBS phenotype but suggest that it is not sufficient to cause the severe, classical form. It therefore seems that there is a different contribution of SALL1 gene function to mouse and human embryonic development., (2006 Wiley-Liss, Inc.)

Published

2006

31. SALL4 deletions are a common cause of Okihiro and acro-renal-ocular syndromes and confirm haploinsufficiency as the pathogenic mechanism.

Author

Borozdin W, Boehm D, Leipoldt M, Wilhelm C, Reardon W, Clayton-Smith J, Becker K, Mühlendyck H, Winter R, Giray O, Silan F, and Kohlhase J

Subjects

Base Sequence, Chromosome Breakage genetics, Female, Humans, In Situ Hybridization, Fluorescence, Male, Pedigree, Phenotype, Polymerase Chain Reaction, Syndrome, Abnormalities, Multiple genetics, Duane Retraction Syndrome genetics, Sequence Deletion genetics, Transcription Factors genetics

Published

2004

32. Chromosomal mosaicism in familial reciprocal translocation carriers: necessity of karyotyping different tissues.

Author

Dufke A, Leipoldt M, and Enders H

Subjects

Abnormalities, Multiple pathology, Humans, Karyotyping, Abnormalities, Multiple genetics, Chromosome Segregation, Chromosomes, Human, Pair 11 genetics, Chromosomes, Human, Pair 22 genetics, Mosaicism, Translocation, Genetic

Published

2003

33. Establishing an algorithm for molecular genetic diagnostics in 127 families with juvenile nephronophthisis.

Author

Hildebrandt F, Rensing C, Betz R, Sommer U, Birnbaum S, Imm A, Omran H, Leipoldt M, and Otto E

Subjects

Adaptor Proteins, Signal Transducing, Base Sequence genetics, Cytoskeletal Proteins, Gene Deletion, Genetic Testing, Haplotypes, Heterozygote, Homozygote, Humans, Membrane Proteins, Molecular Sequence Data, Point Mutation, Proteins genetics, Algorithms, Kidney Diseases, Cystic diagnosis, Kidney Diseases, Cystic genetics, Molecular Biology methods

Abstract

Background: Juvenile nephronophthisis (NPH1), an autosomal recessive cystic disease of the kidney, represents the most common genetic cause of end-stage renal disease in the first two decades of life. On the basis of identification of the gene (NPHP1) defective in NPH1 and the presence of homozygous deletions of NPHP1 in the majority of NPH1 patients, molecular genetic diagnosis for NPH1 is now possible. Molecular genetic testing offers the only method for definite diagnosis of NPH1 and avoids invasive diagnostic measures like renal biopsy., Methods: We examined 127 families (204 patients) with the presumed diagnosis of NPH using molecular genetic diagnostic techniques. In 68 families, renal biopsy was performed and was consistent with NPH, and in 61 families, there was more than one affected child ("multiplex families")., Results: In 74 families (115 patients), there was proof of the diagnosis of NPH1 by detection of a homozygous deletion of the NPHP1 gene, and in 5 families a heterozygous deletion in combination with a point mutation in NPHP1 was demonstrated. Furthermore, for 16 families, NPH1 was excluded with high likelihood by linkage analysis, and for 20 families by detection of heterozygosity for two newly identified polymorphic markers within the deletion region. In 5 of the remaining 12 families, which were noninformative for these markers, fluorescence in situ hybridization did not detect any further heterozygous deletions., Conclusions: The diagnosis of NPH1 was proven by molecular genetic techniques in 62% of families with one or more children with the presumed diagnosis of NPH. We present evidence that there is a fourth locus for NPH, since only 6 of the 26 multiplex families in whom the diagnosis of NPH1 was excluded were compatible with linkage to other loci for NPH. On the basis of the presented data, we propose an algorithm for molecular genetic diagnostics in NPH.

Published

2001

34. Unusual chromosomal mosaicism as a cause of mental retardation and congenital malformations in a familial reciprocal translocation carrier, t(17;22)(q24.2;q11.23).

Author

Dufke A, Mayrhofer H, Enders H, Kaiser P, and Leipoldt M

Subjects

Abnormalities, Multiple physiopathology, Adolescent, Child, Preschool, Chromosome Banding, Crossing Over, Genetic genetics, Humans, In Situ Hybridization, Fluorescence, Infant, Infant, Newborn, Intellectual Disability physiopathology, Karyotyping, Male, Abnormalities, Multiple genetics, Chromosomes, Human, Pair 17 genetics, Chromosomes, Human, Pair 22 genetics, Intellectual Disability genetics, Mosaicism genetics, Translocation, Genetic genetics

Abstract

Familial reciprocal translocations are generally without phenotypic effect, although there is some evidence for a small excess of mental retardation and congenital malformations (MR/CM) in children carrying familial reciprocal translocations. Possible mechanisms whereby such translocations could have a phenotypic effect include cryptic unbalanced rearrangements, uniparental disomy, and disruption of putative genes at the breakpoints, unmasking recessive alleles on the normal homologs. Mosaicism for a supernumerary derivative chromosome in a carrier of a familial reciprocal translocation has not yet been described. We report a boy presenting with MR/CM and a familial reciprocal translocation, t(17;22)(q24.2;q11.23), inherited from the mother. Cytogenetic analysis of peripheral blood lymphocytes showed a balanced karyotype in all 32 analyzed metaphase spreads. Molecular genetic analysis was consistent with biparental origin of the normal homologs. In metaphase spreads from skin fibroblasts a supernumerary chromosome was found in all 24 cells analyzed and could be identified as der(22)t(17;22)(q24.2;q11.23). Several possible segregation modes at meiosis I followed by meiosis II or postzygotic nondisjunction of the der(22) might have led to this unusual chromosomal mosaicism. We propose hidden mosaicism as a possible cause for MR/CM in patients who apparently carry a balanced familial reciprocal translocation., (Copyright 2001 S. Karger AG, Basel)

Published

2001

35. Loss of chromosomes in clear cell renal cell carcinoma and in corresponding renal parenchyma.

Author

Feil G, Leipoldt M, Nelde HJ, Wunderer A, Wechsel HW, Kaiser P, and Bichler KH

Subjects

Adenocarcinoma, Clear Cell pathology, Adenocarcinoma, Clear Cell surgery, Aged, Carcinoma, Renal Cell pathology, Carcinoma, Renal Cell surgery, Chromosome Mapping, Female, Humans, Karyotyping, Kidney metabolism, Kidney Neoplasms pathology, Kidney Neoplasms surgery, Male, Middle Aged, Y Chromosome, Adenocarcinoma, Clear Cell genetics, Carcinoma, Renal Cell genetics, Chromosome Deletion, Kidney pathology, Kidney Neoplasms genetics, Loss of Heterozygosity

Abstract

Chromosome studies were done on six renal cell carcinomas (RCC) and on the corresponding renal parenchymas of the tumor bearing kidneys. Histopathologically, all tumors belonged to the clear cell subtype. All examined parenchymas were pathologically benign. None of the tumor cells showed the typical chromosomal aberrations described for (nonpapillary) RCC, i.e. deletions in the short arm of chromosome #3, or gains in the long arm of chromosome #5. In our series both the tumor and the benign kidney tissues were characterized by loss of chromosomes, especially of the chromosomes #6, #9, #16, #20, and of the Y chromosome. Trisomy of chromosome #7 was found frequently in benign parenchyma cells. The identical chromosomal changes in the tumor and in the parenchyma tissues might reflect rather in vivo mosaics rather than primary chromosomal aberrations in the oncogenetic process of clear cell RCC.

Published

1999

36. A cytogenetic study of Microcebus myoxinus.

Author

Rumpler Y, Ganzhorn JU, Tomiuk J, Leipoldt M, and Warter S

Subjects

Animals, Biopsy veterinary, Chromosome Banding veterinary, Female, Fibroblasts ultrastructure, Male, Skin cytology, Animals, Zoo genetics, Cheirogaleidae genetics, Chromosomes genetics

Published

1998

37. The impact of genetics on the conservation of Malagasy lemur species.

Author

Tomiuk J, Bachmann L, Leipoldt M, Atsalis S, Kappeler PM, Schmid J, and Ganzhorn JU

Subjects

Amino Acid Sequence, Animals, Madagascar, Molecular Sequence Data, Conservation of Natural Resources, Genetic Variation, Lemur genetics, Random Amplified Polymorphic DNA Technique

Published

1998

38. The evaluation of gonosomal mosaics: lymphocyte interphase nuclei analyzed by FISH.

Author

Schliephacke M, Maier CI, Majlinger G, Tomiuk J, Leipoldt M, and Kaiser P

Subjects

Adolescent, Adult, Cell Nucleus ultrastructure, Female, Gonadoblastoma epidemiology, Gonadoblastoma genetics, Humans, Interphase, Male, Risk Factors, In Situ Hybridization, Fluorescence, Lymphocytes ultrastructure, Mosaicism

Abstract

The reliable evaluation of chromosomal mosaics is still considered to be difficult in clinical diagnosis if aberrant metaphases are only present at low frequencies. Classical cytogenetic findings cannot significantly exclude low mosaic levels, obviously, because of the relatively low number of analyzed metaphases. To study this problem, the number of gonosomes in lymphocyte interphase nuclei was determined by FISH (fluorescence in situ hybridization) application of two satellite DNA probes. DXZI and DYZI. The results obtained with this method from lymphocytes of clinically and cytogenetically inconspicuous persons showed a high degree of reliability. The DNA probe yielded correct signals in more than 95% of the analyzed nuclei. Additionally, patients were examined who showed cytogenetically confirmed numerical gonosome aberrations. These results were compared with those obtained from the control group of inconspicuous patients and discussed with respect to the evaluation of gonosomal mosaics.

Published

1996

39. Immunohistochemical and cytogenetic findings in malignant rhabdoid tumor.

Author

Kaiserling E, Ruck P, Handgretinger R, Leipoldt M, and Hipfel R

Subjects

Cytogenetics, Female, Humans, Immunohistochemistry, Infant, Kidney Neoplasms genetics, Kidney Neoplasms immunology, Kidney Neoplasms pathology, Kidney Neoplasms ultrastructure, Male, Rhabdoid Tumor pathology, Rhabdoid Tumor ultrastructure, Soft Tissue Neoplasms genetics, Soft Tissue Neoplasms immunology, Soft Tissue Neoplasms pathology, Soft Tissue Neoplasms ultrastructure, Rhabdoid Tumor genetics, Rhabdoid Tumor immunology

Abstract

Background: The histogenesis of malignant rhabdoid tumor (RT) remains a matter of controversy. From published reports it appears that some extrarenal RT (ERRT) exhibit neural or neuroectodermal features. Systematic investigation of renal RT (RRT) for neural differentiation has not yet been published. In this study, two RRT and two ERRT were investigated by light and electron microscopy, immunocytochemistry, and cytogenetic analysis., Results: All four cases exhibited similar morphology and a largely consistent immunohistochemical staining profile. Both tumor types showed immunoreactivity for various cytokeratins, epithelial membrane antigen (EMA), vimentin, neurofilaments, S100 protein, neuron specific enolase, Leu7, CD34, p53, MB2, MIC2, VS38c, laminin and fibronectin. Reactivity was usually confined to a small proportion of the tumor cells, especially in the case of antibodies against neurofilaments, NSE, S100 proteins Leu7, CD34 and p53. Only a few of the antibodies (anti-vimentin, MB2, MIC2, anti-EMA, and VS38c) stained the majority of the tumor cells. Chromosome analysis revealed a discrete aberration in 11p (most probably a paracentric inversion in 11p15) in the one RRT investigated. One ERRT had a normal karyotype, but the other one exhibited various structural abnormalities on chromosomes 18 and 22., Conclusions: The immunohistochemical investigations revealed many similarities between RRT and ERRT, and all four tumors investigated exhibited neuroectodermal differentiation. As far as histogenetic classification is concerned, our findings point in the direction of the group of tumors that includes Ewing's sarcoma and primitive neuroectodermal tumors.

Published

1996

40. Pitfall: amniocentesis fails to detect mosaic trisomy 8 in a male newborn.

Author

Schneider M, Klein-Vogler U, Tomiuk J, Schliephacke M, Leipoldt M, and Enders H

Subjects

Adult, False Negative Reactions, Female, Humans, Male, Pregnancy, Amniocentesis, Chromosomes, Human, Pair 8, Mosaicism, Trisomy

Published

1994

41. Prenatal diagnosis and postnatal follow-up of a child with two de novo unrelated balanced reciprocal translocations.

Author

Pruggmayer M, Zoll B, Leipoldt M, and Thies U

Subjects

Adult, Chromosomes, Human, Pair 10, Chromosomes, Human, Pair 15, Chromosomes, Human, Pair 17, Chromosomes, Human, Pair 3, Female, Humans, Karyotyping, Pregnancy, Amniocentesis, Translocation, Genetic

Abstract

Two unrelated, apparently balanced, reciprocal translocations involving chromosomes 3 and 17, and 10 and 15 were found in cultured amniotic fluid cells from a 41-year-old 10-gravida. Chromosome analysis of peripheral blood lymphocytes of both parents revealed normal karyotypes. Post-partum examination of lymphocyte cultures from the proband confirmed the chromosome rearrangements. The child showed normal development during follow-up examinations up to the age of 4 years.

Published

1990

42. High incidence of minor chromosomal variants in teratozoospermic males.

Author

Eiben B, Leipoldt M, Rammelsberg O, Krause W, and Engel W

Subjects

Chromosomes, Human, Pair 9, Humans, Klinefelter Syndrome genetics, Male, Mosaicism, Semen analysis, Spermatozoa ultrastructure, Chromosome Aberrations, Infertility, Male genetics, Spermatozoa abnormalities

Abstract

Chromosomal analysis was performed on 109 males with teratozoospermia. Four cases of anomaly were found, including three cases of mosaic Klinefelter's syndrome and one balanced autosomal translocation. Among chromosomal heteromorphisms, 9qh+ was found in 25% of the patients. The fraction of malformed spermatozoa in the semen of the 9qh+ group is significantly higher than in the chromosomally normal group. It is speculated that heterochromatic variants like 9qh+ could be one of several unknown factors disturbing normal gametogenesis.

Published

1987

43. Amount of repeated and non-repeated DNA in the genomes of closely related fish species with varying genome sizes.

Author

Schmidtke J, Schmitt E, Leipoldt M, and Engel W

Subjects

Animals, Base Composition, Cytosine analysis, Genes, Guanine analysis, In Vitro Techniques, Species Specificity, Cyprinidae genetics, DNA analysis

Abstract

1. Within the teleostean family Cyprinidae, diploid species occur with wide variation in genome size. There also exist species which were anciently tetraploid. 2. The quantitative changes of DNA content in the diploids are primarily due to differences in the amount of intermediately repeated DNA. DNA sequence composition of the ancient tetraploid genomes suggests that the species derived from diploid ancestors of small genome size. 3. The average base composition and the base compositional heterogeneity are similar in all the species examined.

Published

1979

44. Comparative DNA/DNA reassociation kinetics in three hamster species.

Author

Leipoldt M, Eckhardt R, and Schmid M

Subjects

Animals, Base Sequence, Cricetulus metabolism, Liver analysis, Mesocricetus metabolism, Nucleic Acid Conformation, Species Specificity, Cricetinae metabolism, DNA analysis, Nucleic Acid Renaturation

Abstract

1. Three major DNA repetition classes can be distinguished in the genomes of three hamster species Mesocricetus auratus, Cricetulus griseus, and Phodopus sungorus sungorus: A very fast reassociating fraction of about 13% of the DNA, a fast reassociating fraction comprising 10-23% of the DNA, and a slowly reassociating fraction containing single-copy sequences of 63-78% of hamster DNA. 2. In the DNA of the Syrian and Djungarian hamster 43%-53%, and in the DNA of the Chinese hamster 80% of the single-copy sequences are interspersed with repetitive sequences. 3. The lengths of repetitive DNA sequences, vary between more than 3 kb and 0.3 kb, with the majority of sequences having a length of 0.3 kb to 0.5 kb. 4. The findings suggest that the genomes of the hamster species studied are organized in a short period interspersion pattern. 5. Unlike other vertebrate and invertebrate genomes, moderately repetitive sequences exhibit a high degree of intraspecific homology in the hamster genome.

Published

1982

45. Towards an understanding of the molecular mechanisms regulating gene expression during diploidization in phylogenetically polyploid lower vertebrates.

Author

Leipoldt M

Subjects

Animals, Birds genetics, Cyprinidae genetics, Gene Amplification, Humans, Models, Genetic, RNA, Ribosomal genetics, Transcription, Genetic, Amphibians genetics, Fishes genetics, Gene Expression Regulation, Phylogeny, Polyploidy

Abstract

Polyploidization and regional gene duplication have occurred frequently during vertebrate evolution, providing the genetic material necessary for creating evolutionary novelties. Mammals, including man, can be regarded as diploid species with a polyploid history of evolution. Polyploidization steps during the phylogeny of mammals probably took place in the genomes of amphibian- or fish-like mammalian ancestors. The polyploid status has subsequently been shaped by the process of diploidization, leading to genomes that are polyploid with respect to the amount of genetic material and the number of gene copies, and diploid with respect to the level of gene expression and chromosomal characteristics. Phylogenetically tetraploid amphibian and teleost species together with their diploid close relatives can be used as a model system to study the effect of polyploidization and the mechanisms of diploidization of a parallel event during early mammalian evolution. Experimental evidence permits the assumption that the diploidization of gene expression in tetraploid cyprinid fish may be functionally correlated with structural modifications of the ribosomal components, RNA and protein. These findings are discussed in the light of reduced protein synthesis in diploidized tetraploid species and a mechanism to explain diploidization during mammalian evolution.

Published

1983

46. Ribosomal RNA structure in the diploid and phylogenetically polyploid amphibian species Hyla and Odontophrynus.

Author

Leipoldt M and Kellner M

Subjects

Animals, Diploidy, Female, Kidney analysis, Liver analysis, Organ Specificity, Ovary analysis, RNA, Ribosomal isolation & purification, Species Specificity, Amphibians genetics, Phylogeny, RNA, Ribosomal genetics

Abstract

Ribosomal RNA of the diploid amphibian species Hyla chrysoscelis and Odontophrynus americanus is structurally modified by hidden breaks. Phylogenetically polyploid related species like the tetraploid Hyla versicolor, the tetraploid Odontophrynus americanus and the octoploid Ceratophrys ornata do not show hidden breaks in ribosomal RNA. Structural modifications of rRNA molecules in diploid amphibians has no detectable effect on the ribosomal activity in vitro.

Published

1984

47. Partial deletion of 4p in fetal cells not present in chorionic villi.

Author

Eiben B, Leipoldt M, Schübbe I, Ulbrich R, and Hansmann I

Subjects

Adult, Amniocentesis, Amnion pathology, Biopsy, Needle, False Negative Reactions, Female, Humans, Karyotyping, Pregnancy, Ultrasonography, Abnormalities, Multiple diagnosis, Chorionic Villi, Chromosome Deletion, Chromosomes, Human, Pair 4, Fetus pathology

Abstract

A case of a prenatal diagnosis at the second trimester is presented showing a normal karyotype in 12 metaphases from chorionic villi. In all cultured amniotic cells, however, and also in all fetal fibroblasts analyzed after abortion a structural anomaly (46,XY;del 4(pter----p15.2) was detected. Prenatal diagnosis was performed because of intrauterine growth retardation, cleft lip and esophagus atresia by ultrasound. The fetal stigmata are compatible with the Wolf Hirschhorn syndrome. We conclude that amniocentesis may be indicated notwithstanding a normal CV-diagnosis in those rare pregnancies with a characteristically abnormal ultrasound.

Published

1988

48. Hidden breaks in ribosomal RNA of phylogenetically tetraploid fish and their possible role in the diploidization process.

Author

Leipoldt M and Engel W

Subjects

Animals, Diploidy, Female, Male, Molecular Weight, Nucleic Acid Hybridization, Phylogeny, Protein Biosynthesis, Ribosomal Proteins genetics, Ribosomes metabolism, Cyprinidae genetics, Polyploidy, RNA, Ribosomal genetics

Abstract

Hidden breaks occur in the ribosomal RNA of tetraploid Cyprinid fish such that the large ribosomal RNA (28 S) yields upon denaturation two RNA fragments of 8.7 X 10(5) and 5.0 X 10(5) daltons, whereas the small rRNA (18 S) yields fragments of 3.2 X 10(5) to 5.0 X 10(4) daltons. In tetraploid Cyprinids hidden breaks occur only in the rRNA of somatic tissue and not in oocytes and sperm cells. Hidden breaks can be detected only slightly in diploid Cyprinid species. Ribosomes purified from somatic tissue of tetraploid Cyprinids show a reduced efficiency in protein synthesis in vitro. The ribosomal proteins from diploid and tetraploid Cyprinid fish show considerable electrophoretic differences. This is discussed in light of a possible functional role of hidden breaks in rRNA in the process of diploidization of gene expression in tetraploid Cyprinid species.

Published

1983

49. Satellited Y chromosomes: structure, origin, and clinical significance.

Author

Schmid M, Haaf T, Solleder E, Schempp W, Leipoldt M, and Heilbronner H

Subjects

Adolescent, Chromosome Banding, Heterochromatin ultrastructure, Humans, Karyotyping, Male, Nucleolus Organizer Region ultrastructure, Pedigree, DNA, Satellite genetics, Sex Chromosome Aberrations genetics, Translocation, Genetic, Y Chromosome ultrastructure

Abstract

Three cases of inherited satellited Y chromosomes (Yqs) were analysed using several cytogenetic techniques. The cytogenetic data of the 14 cases of Yqs chromosomes described to date were reviewed. All Yqs chromosomes carry an active nucleolus organizer region (NOR) in their long arm and must have developed from translocations involving the short arms of the acrocentric autosomes. The structure of the heterochromatic satellite region in the Yqs chromosomes shows conspicuous inter-familial differences; this permits the reconstruction of the translocations from which the various Yqs were derived. Some causal factors leading to the development of Yqs chromosomes are considered: the specific localization of the four satellite DNAs and highly methylated DNA sequences in the karyotype, and some new experimental data on the spatial arrangement of heterochromatic regions in interphase nuclei. These provide distinct evidence for a preferential involvement of the autosomes 15 and 22 in the translocations with the Y heterochromatin. All clinical reports documenting Yqs males born with malformations were reviewed. It appears that the presence of an extra NOR and NOR-associated heterochromatin in the Yqs chromosomes does not cause any phenotypic abnormalities (as long as the Y euchromatin is intact). The possibility that a Yqs chromosome predisposes to non-disjunction and/or to translocations of other chromosomes is discussed.

Published

1984

50. Nekrozoospermia in mosaic Klinefelter's syndrome.

Author

Leipoldt M, Eiben B, Krause W, and Engel W

Subjects

Adult, Humans, Infertility, Male etiology, Karyotyping, Klinefelter Syndrome complications, Male, Klinefelter Syndrome genetics, Mosaicism, Spermatozoa abnormalities

Abstract

A patient with nekrozoospermia is presented. His clinical, andrological and endocrinological data are described. Cytogenetically a complex chromosomal mosaic of 46,XX; 46,XY; 47,XXY and 48,XXXY was found.

Published

1987