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Featured researches published by Thomas Cremer.


Human Genetics | 1988

Delineation of individual human chromosomes in metaphase and interphase cells by in situ suppression hybridization using recombinant DNA libraries

Peter Lichter; Thomas Cremer; J. Borden; Laura Manuelidis; David C. Ward

SummaryA method of in situ hybridization for visualizing individual human chromosomes from pter to qter, both in metaphase spreads and interphase nuclei, is reported. DNA inserts from a single chromosomal library are labeled with biotin and partially preannealed with a titrated amount of total human genomic DNA prior to hybridization with cellular or chromosomal preparations. The cross-hybridization of repetitive sequences to nontargeted chromosomes can be markedly suppressed under appropriate preannealing conditions. The remaining single-stranded DNA is hybridized to specimens of interest and detected with fluorescent or enzymelabeled avidin conjugates following post-hybridization washes. DNA inserts from recombinant libraries for chromosomes 1, 4, 7, 8, 13, 14, 18, 20, 21, 22, and X were assessed for their ability to decorate specifically their cognate chromosome; most libraries proved to be highly specific. Quantitative densitometric analyses indicated that the ratio of specific to nonspecific hybridization signal under optimal preannealing conditions was at least 8:1. Interphase nuclei showed a cohesive territorial organization of chromosomal domains, and laserscanning confocal fluorescence microscopy was used to aid the 3-D visualization of these domains. This method should be useful for both karyotypic studies and for the analysis of chromosome topography in interphase cells.


Human Genetics | 1988

Detection of chromosome aberrations in metaphase and interphase tumor cells by in situ hybridization using chromosome-specific library probes

Thomas Cremer; Peter Lichter; J. Borden; David C. Ward; Laura Manuelidis

SummaryChromosome aberrations in two glioma cell lines were analyzed using biotinylated DNA library probes that specifically decorate chromosomes 1, 4, 7, 18 and 22 from pter to qter. Numerical changes, deletions and rearrangements of these chromosomes were radily visualized in metaphase spreads, as well as in early prophase and interphase nuclei. Complete chromosomes, deleted chromosomes and segments of translocated chromosomes were rapidly delineated in very complex karyotypes. Simultaneous hybridizations with additional subregional probes were used to further define aberrant chromosomes. Digital image analysis was used to quantitate the total complement of specific chromosomal DNAs in individual metaphase and interphase cells of each cell line. In spite of the fact that both glioma lines have been passaged in vitro for many years, an under-representation of chromosome 22 and an over-representation of chromosome 7 (specifically 7p) were observed. These observations agree with previous studies on gliomas. In addition, sequences of chromosome 4 were also found to be under-represented, especially in TC 593. These analyses indicate the power of these methods for pinpointing chromosome segments that are altered in specific types of tumors.


Genetic Analysis: Biomolecular Engineering | 1991

Analysis of genes and chromosomes by nonisotopic in situ hybridization

Peter Lichter; Ann L. Boyle; Thomas Cremer; David C. Ward

Nonisotopic in situ hybridization is a powerful tool to analyze the organization of complex genomes. Current approaches utilizing this technique for the analysis of linear and spatial genome organizations are presented. Clinical applications of these approaches, which open new avenues for diagnosis of disease-related chromosomal changes, are also discussed.


Experimental Cell Research | 1988

Rapid interphase and metaphase assessment of specific chromosomal changes in neuroectodermal tumor cells by in situ hybridization with chemically modified DNA probes

Thomas Cremer; D. Tesin; Anton H.N. Hopman; Laura Manuelidis

Repeated DNAs from the constitutive heterochromatin of human chromosomes 1 and 18 were used as probes in nonradioactive in situ hybridization experiments to define specific numerical and structural chromosome aberrations in three human glioma cell lines and one neuroblastoma cell line. The number of spots detected in interphase nuclei of these tumor cell lines and in normal diploid nuclei correlated well with metaphase counts of chromosomes specifically labeled by in situ hybridization. Rapid and reliable assessments of aneuploid chromosome numbers in tumor lines in double hybridization experiments were achieved, and rare cells with bizarre phenotype and chromosome constitution could be evaluated in a given tumor cell population. Even with suboptimal or rare chromosome spreads specific chromosome aberrations were delineated. As more extensive probe sets become available this approach will become increasingly powerful for uncovering various genetic alterations and their progression in tumor cells.


Archive | 1992

Chromosome analysis by non-isotopic in situ hybridization.

Peter Lichter; Thomas Cremer


Archive | 1996

Arrangement of nucleic acid sequences for comparative genomic hybridization

Thomas Cremer; Thomas Ried; Michael R. Speicher; Anna Jauch; Peter Lichter


Archive | 1989

In situ suppression hybridization and uses therefor

David C. Ward; Peter Lichter; Thomas Cremer; Laura Manuelidis


American Journal of Hematology | 1990

Detection of monosomy 7 in interphase cells of patients with myeloid disorders

Rukmini V. Kolluri; Laura Manuelidis; Sheila N.J. Sait; Thomas Cremer; Sefer Gezer; Azra Raza


Archive | 1996

Ultrahigh resolution comparative nucleic acid hybridization to combed dna fibers

Aaron Bensimon; Thomas Cremer; Juergen Kraus; Peter Lichter


Archive | 1994

Delineation of individual human chromosomes in metaphase and interphase cells by in situ suppression hybridization

David C. Ward; Peter Lichter; Thomas Cremer; Laura Manuelidis; Thomas Ried; Antonio Baldini

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Thomas Ried

National Institutes of Health

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