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5. Quantitative PCR: the determination of template copy numbers by temperature gradient gel electrophoresis (TGGE)

Author

M. Heibey and K. Henco

Subjects
Electrophoresis, Gel electrophoresis, Base Composition, Chromatography, Base Sequence, Temperature, RNA, DNA, Templates, Genetic, Biology, Polymerase Chain Reaction, Molecular biology, law.invention, chemistry.chemical_compound, Real-time polymerase chain reaction, chemistry, law, Genetics, Humans, Quantitative analysis (chemistry), Polymerase chain reaction, Temperature gradient gel electrophoresis
Published
1990
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6. Isolation and Characterization of High-Molecular Mass DNA from Hair Shafts

Author

K Henco, L S Meyer-Stork, D Riesner, P Loss, J. Kalbé, Heinz Berndt, S L Sauter, Rolf Kuropka, and Hartwig Höcker

Subjects
Sheep, High molecular mass, integumentary system, Wool, DNA–DNA hybridization, Hair analysis, Nucleic Acid Hybridization, DNA, YAK, Isolation (microbiology), Biochemistry, Molecular Weight, Nucleic acid thermodynamics, chemistry.chemical_compound, Liver, Species Specificity, chemistry, otorhinolaryngologic diseases, Animals, Humans, Mohair, sense organs, Hair
Abstract

Experiments to identify species by DNA analysis of their hair failed so far because no DNA could be isolated from hair shafts. In this work the preparation of DNA from human--as well as from animal hair shafts (alpaca, angora-rabbit, cashmere, cashgora, mohair, merino and yak) is described for the first time. In general the isolated DNA shows a length of more than 20 kbp. The species of the hair shaft samples could be exactly identified by DNA hybridization experiments. The isolated DNA from hair shafts allow new possibilities to identify species and individuals employing techniques from molecular biology.

Published
1988
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7. Molecular cloning of two west African human immunodeficiency virus type 2 isolates that replicate well in macrophages: a Gambian isolate, from a patient with neurologic acquired immunodeficiency syndrome, and a highly divergent Ghanian isolate

Author

Herbert Kühnel, A. Immelmann, D. Mix, K. Henco, L. Biesert, Michalina Adamski, Renate Kreutz, H. Von Briesen, Ursula Dietrich, and C. Meichsner

Subjects
Genes, Viral, Restriction Mapping, Molecular cloning, Biology, Virus Replication, medicine.disease_cause, medicine, Humans, Lymphocytes, Cloning, Molecular, Cells, Cultured, Acquired Immunodeficiency Syndrome, Syncytium, Multidisciplinary, Macrophages, Nucleic acid sequence, virus diseases, RNA-Directed DNA Polymerase, Simian immunodeficiency virus, biology.organism_classification, Virology, Reverse transcriptase, Rhesus macaque, Viral replication, Cell culture, DNA, Viral, HIV-2, Gambia, Nervous System Diseases, Research Article
Abstract

Human immunodeficiency virus type 2 (HIV-2)-related viruses were isolated from a Gambian dying of exclusively neurological disease (HIV-2D194) and from an asymptomatic Ghanian (HIV-2D205). Both strains exhibited properties of HIV-1 biological subtype c: they grew slowly and induced few or no syncytia but eventually produced high levels of particle-associated reverse transcriptase in cultures of fresh peripheral blood lymphocytes, and they established stable infection of T-lymphoma (HUT-78) and monocytic (U937) cell lines. Each produced even higher levels of reverse transcriptase when fresh human monocytes/macrophages were used as target cells. The viruses were molecularly cloned after a single passage in culture, in order to minimize in vitro selection of subtypes present in vivo. Restriction-site analysis showed heterogeneity within each isolate. Nucleotide sequence analysis of a portion of the HIV-2D194 genome revealed that it is a member of the prototypic HIV-2 family, displaying 13% divergence versus HIV-2ROD and HIV-2NIHZ, as compared to 9% divergence between HIV-2ROD and HIV-2NIHZ. In contrast, HIV-2D205 is the most highly divergent HIV-2 strain yet described: it is equidistant in relation between the known HIV-2 strains and the simian immunodeficiency virus isolates from rhesus macaque monkeys (23-25% divergence).

Published
1989
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8. Structural relationship of human interferon alpha genes and pseudogenes

Author

K. Todokoro, Shigekazu Nagata, J. I. Fujisawa, A. Fujisawa, K. Henco, J. Hochstadt, M. Wälchli, Jürgen Brosius, J. Haynes, A. Schamböck, M. Pasek, Charles Weissmann, T. Kovacic, and J. Schmid

Subjects
clone (Java method), Transcription, Genetic, Genetic Linkage, Pseudogene, Reading frame, Alpha interferon, Protein Sorting Signals, Biology, chemistry.chemical_compound, Structural Biology, Genetic linkage, Sequence Homology, Nucleic Acid, Humans, Amino Acid Sequence, Molecular Biology, Gene, Genetics, Base Sequence, Chromosome Mapping, DNA, Cosmids, Genes, chemistry, Interferon Type I, Cosmid
Abstract

We have isolated and characterized DNA segments containing IFN-alpha-related sequences from human lambda and cosmid clone banks. We describe six linkage groups comprising 18 distinct IFN-alpha-related loci, and report the nucleotide sequences of nine chromosomal IFN-alpha-genes with intact reading frames, as well as of five pseudogenes. Taking into account as yet unsequenced genes as well as clones described by others, there are now seven linkage groups and 23 loci, of which 15 correspond to potentially functional genes and six to non-functional genes; two loci remain unsequenced. Eighteen additional sequences are likely to be allelic to the above. The finding that at least two IFN-alpha genes appear to be natural hybrids of other IFN-alpha genes, and that two distinct IFN-alpha loci have completely identical coding sequences, although their flanking regions are different, is evidence for information exchange between the individual genes.

Published
1985
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10. STRUCTURE AND EXPRESSION OF HUMAN ALPHA-INTERFERON GENES

Author

C. Weissmann, S. Nagata, W. Boll, M. Fountoulakis, A. Fujisawa, J.-I. Fujisawa, J. Haynes, K. Henco, N. Mantei, H. Ragg, C. Schein, J. Schmid, G. Shaw, M. Streuli, H. Taira, K. Todokoro, and U. Weidle

Subjects
Cloning, chemistry.chemical_classification, chemistry, Complementary DNA, Protein biosynthesis, RNA, Alpha interferon, Biology, Gene, Molecular biology, Peptide sequence, Amino acid
Abstract

cDNA was prepared from induced leukocyte poly(A) RNA and cloned in Escherichia coli. Interferon (IFN)-alpha cDNA clones were isolated by subculture cloning using a translation hybridization assay. Definitive identification of the clones was based on the production of an interferon-like protein by the transformed bacteria. Different IFN-alpha cDNAs, with characteristic target cell specificities, were identified. The cloned cDNAs typically encode a mature polypeptide of 166 (or, in the case of IFN-alpha 2, 165) amino acids and a signal sequence of 23 amino acids.

Published
1982
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11. Partial mapping of ten genes of the human interferon- alpha family

Author

C. Brack, K. Henco, S. Nagata, A. Schamböck, and Charles Weissmann

Subjects
Genetics, Base Sequence, Sequence analysis, Genetic Linkage, Immunology, Intron, DNA, Recombinant, Nucleic Acid Hybridization, DNA Restriction Enzymes, Biology, law.invention, Nucleic acid thermodynamics, Genes, Genetic linkage, law, Virology, Interferon α, Recombinant DNA, Humans, Interferons, Allele, Gene, Alleles
Abstract

HuIFN-α genes form a family of not less than 9–10 distinct members, at least three of which are arranged in tandem. In one case, two variants, believed to be alleles of the same gene, could be identified by sequence analysis. The three genes sequenced so far are devoid of introns.

Published
1981

12. Structure and expression of human IFN-alpha genes

Author

K. Todokoro, K. Henco, Michael Fountoulakis, J. Haynes, Catherine H. Schein, Hermann Ragg, Werner Boll, Shigekazu Nagata, Ned Mantei, Michel Streuli, Ulrich Weidle, Hideharu Taira, J. Schmid, J. I. Fujisawa, G. Shaw, Charles Weissmann, and A. Fujisawa

Subjects
Pseudogene, DNA, Recombinant, Receptors, Cell Surface, Biology, Plasmid, Complementary DNA, Escherichia coli, Gene family, Humans, RNA, Messenger, Cloning, Molecular, Gene, Receptors, Interferon, Cloning, Genetics, Base Sequence, Intron, Gene Amplification, Promoter, General Medicine, DNA, Molecular biology, Biological Evolution, Gene Expression Regulation, Genes, Interferon Type I
Abstract

Copy DNA (cDNA) was prepared from induced leucocyte poly (A) RNA and cloned inEscherichia coli. IFN-α cDNA clones were isolated by subculture cloning with the use of a translation hybridization assay. Definitive identification of the clones was based on the production of an interferon-like protein by the transformed bacteria. Different IFN-α cDNAs, with characteristic target cell specificities, were identified. The cloned cDNAs typically encode a mature polypeptide of 166 (or, for IFN-α2, 165) amino acids and a signal sequence of 23 amino acids. A human chromosomal library was screened with IFN cDNA and 17 distinct IFN-α-related sequences were isolated and identified, of which 7 proved to be nonallelic authentic genes and 4 pseudogenes; 6 sequences remain to be elucidated. Taking into account the work of Goeddel and his colleagues, 13 non-allelic authentic genes and 6 pseudogenes can be distinguished. In addition, 9 genes believed to be allelic to the 13 authentic genes have been sequenced. The IFN-α genes may be classified into two major subfamilies, which diverged at least 33 Ma ago, but perhaps much earlier, if sequence rectification occurred. At least one IFN-α gene appears to have resulted by a recombinational event between members of the subfamily I and II. IFN-β is distantly related to IFN-α’s and may have diverged from a common ancestor at least 500 Ma ago. Both IFN-α and IFN-β genes differ from most other genes of higher organisms by being devoid of introns. The mouse was found to possess an IFN-α gene family of a size similar to that of man; the murine genes also do not have introns. IFN-α genes devoid of their signal sequence were joined to prokaryotic promoters to produce the mature interferons inE. coliin high yield. IFN-α2, purified to homogeneity, has been crystallized by T. Unge and B. Strandberg (Uppsala). Hybrid genes consisting of IFN-α1 and IFN-α2 segments were constructed and expressed inE. coli; the target cell specificities of such hybrids were dependent on the arrangement of the segments and were different from those of either parent. The chromosomal gene for HuIFN-α1 was introduced into mouse L cells to study the mechanism of its expression. Correct transcription was only detected after induction (with Newcastle disease virus); expression was transient, with the same kinetics as those of the endogenous mouse IFN mRNA. Natural murine IFNs and human IFN-β and IFN-γ are glycosylated. BecauseE. colicells transformed with the genes of eukaryotic glycoproteins are not expected to yield correctly glycosylated polypeptides, we prepared lines of hamster cells permanently transformed with hybrid plasmids, which contained an IFN gene linked to the SV40 early promoter, as well as dihydrofolate reductase as a selective marker. After intracellular amplification of the introduced genes, cell lines were obtained which constitutively produced IFN at about 40 000 units ml-1and could be propagated for at least several months.

Published
1982

13. Structure and expression of human alpha-interferon genes

Author

C, Weismann, S, Nagata, S, Boll, M, Fountoulakis, A, Fujisawa, J, Fujisawa, J, Haynes, K, Henco, N, Mantei, and H, Ragg

Subjects
Base Sequence, Nucleic Acid Hybridization, DNA, Genes, Protein Biosynthesis, Interferon Type I, Escherichia coli, Leukocytes, Humans, RNA, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Poly A
Abstract

cDNA was prepared from induced leukocyte poly(A) RNA and cloned in Escherichia coli. Interferon (IFN)-alpha cDNA clones were isolated by subculture cloning using a translation hybridization assay. Definitive identification of the clones was based on the production of an interferon-like protein by the transformed bacteria. Different IFN-alpha cDNAs, with characteristic target cell specificities, were identified. The cloned cDNAs typically encode a mature polypeptide of 166 (or, in the case of IFN-alpha 2, 165) amino acids and a signal sequence of 23 amino acids.

Published
1982

14. Isolation of variants of lymphocytopathic retroviruses from the peripheral blood and cerebrospinal fluid of patients with ARC or AIDS

Author

E. B. Helm, H. Rübsamen-Waigmann, R. Brodt, K. Henco, H. D. Brede, W. B. Becker, and H. Fischer

Subjects
viruses, Fluorescent Antibody Technique, Biology, Deltaretrovirus, Virus, Western blot, Cytopathogenic Effect, Viral, Virology, Antigenic variation, medicine, Humans, Lymphocytes, Cytopathic effect, Southern blot, Acquired Immunodeficiency Syndrome, medicine.diagnostic_test, Nucleic Acid Hybridization, RNA-Directed DNA Polymerase, Reverse transcriptase, Microscopy, Electron, Infectious Diseases, Peripheral blood lymphocyte, DNA, Viral, Tissue tropism, Immunologic Techniques, Retroviridae Infections
Abstract

LAV/HTLV-III/AAV viruses were isolated from 20 German patients with ARC/ AIDS in order to investigate strain variation. Virus was isolated from the peripheral blood and/or cerebrospinal fluid (CSF) in umbilical cord peripheral blood lymphocyte (PBL) cultures. Isolates were identified by their cytopathic effect (CPE), by reverse transcriptase assays on cell-free infected culture supernatant fluid (SNF), and one or more of the following: immunofluorescence assays on infected cells for viral antigen using HTLV-I11 reference sera, Western blot analysis of cell-free infected culture SNF, electron microscopy of infected cells, and Southern blot restriction analysis and specific HTLV-I11 probing of DNA extracted from infected cultured PBL. The isolates could be classified into three groups according to differences in growth rate and cytopathic effect: Most showed what was regarded as the typical CPE, while some either grew rapidly and induced a striking CPE and others grew slowly with minimal CPE. In one patient, virus producing typical CPE was isolated from the peripheral blood while the isolate from his filtered cell-free CSF produced atypical slow CPE, suggesting that antigenic variation may occur with persistent infection or that superinfection may occur. Southern blot DNA restriction analysis of the DNA of three selected isolates showed that two of the isolates were similar but that the restriction pattern of all three differed from patterns previously published. Our results supplement the accumulating evidence of genetic variation among LAV/HTLV-I11 strains. The extent of this variation needs to be evaluated for any effect on the sensitivity of diagnostic tests, on the strategy of vaccine development, on tissue tropism by altering the viral surface receptor-binding sites, and possibly on the development of specific chemotherapy.

Published
1986

16. STRUCTURE AND EXPRESSION OF HUMAN IFN-α GENES

Author

Catherine H. Schein, Hideharu Taira, M. Mishina, Shigekazu Nagata, Ulrich Weidle, Michel Streuli, Werner Boll, Charles Weissmann, Ned Mantei, Alan Hall, K. Henco, and Josef Ecsödi

Subjects
Expression (architecture), Biology, Biochemistry, Gene, Molecular biology
Published
1981
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17. Discretization of Gene Expression Data Unmasks Molecular Subgroups Recurring in Different Human Cancer Types.

Author

Beleut M, Soeldner R, Egorov M, Guenther R, Dehler S, Morys-Wortmann C, Moch H, Henco K, and Schraml P

Subjects
Algorithms, Carcinoma, Renal Cell classification, Carcinoma, Renal Cell genetics, Carcinoma, Renal Cell metabolism, Gene Expression Profiling, Genes, Neoplasm genetics, Genome-Wide Association Study, Humans, Kidney Neoplasms classification, Kidney Neoplasms genetics, Kidney Neoplasms metabolism, Models, Theoretical, Neoplasms classification, Neoplasms metabolism, Oligonucleotide Array Sequence Analysis, Gene Expression Regulation, Neoplastic genetics, Neoplasms genetics
Abstract

Despite the individually different molecular alterations in tumors, the malignancy associated biological traits are strikingly similar. Results of a previous study using renal cell carcinoma (RCC) as a model pointed towards cancer-related features, which could be visualized as three groups by microarray based gene expression analysis. In this study, we used a mathematic model to verify the presence of these groups in RCC as well as in other cancer types. We developed an algorithm for gene-expression deviation profiling for analyzing gene expression data of a total of 8397 patients with 13 different cancer types and normal tissues. We revealed three common Cancer Transcriptomic Profiles (CTPs) which recurred in all investigated tumors. Additionally, CTPs remained robust regardless of the functions or numbers of genes analyzed. CTPs may represent common genetic fingerprints, which potentially reflect the closely related biological traits of human cancers.

Published
2016
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18. NanoStore: a concept for logistical improvements of compound handling in high-throughput screening.

Author

Benson N, Boyd HF, Everett JR, Fries J, Gribbon P, Haque N, Henco K, Jessen T, Martin WH, Mathewson TJ, Sharp RE, Spencer RW, Stuhmeier F, Wallace MS, and Winkler D

Subjects
Automation, Chromatography, Liquid, Combinatorial Chemistry Techniques, Drug Stability, Drug Storage methods, Inhibitory Concentration 50, Mass Spectrometry, Models, Chemical, Molecular Weight, Nanotechnology, Pharmaceutical Preparations, Solubility, Specimen Handling, Temperature, Time Factors, Chemistry, Pharmaceutical methods, Drug Evaluation, Preclinical methods
Abstract

Small molecule screening, the systematic encounter of biology space with chemical space, has provoked the emergence of a whole industry that recreates itself by constant iterative improvements to this process. The authors describe an approach to tackle the problem for one of the most time-consuming steps in the execution of a screening campaign, namely, the reformatting of high-throughput screening test compounds from master plates to daughter assay plates used in the execution of the screen. Through an engineered storage procedure, they prepare plates ahead of the screening process with the respective compounds in a ready-to-use format. They show the biological inertness of the method and how it facilitates efficient recovery of compound activity. This uncoupling of normally interconnected processes provides time and compound savings, avoids repeated freeze-thaw cycles of compound solutions, and removes the problems associated with the DMSO sensitivity of certain assays types.

Published
2005
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20. Fluorescence correlation spectroscopy (FCS)--a highly sensitive method to analyze drug/target interactions.

Author

Sterrer S and Henco K

Subjects
Animals, Binding, Competitive, Biological Assay methods, DNA metabolism, Humans, Ligands, Models, Molecular, Nucleic Acids metabolism, Proteins metabolism, Receptors, Cell Surface, Spectrometry, Fluorescence methods
Abstract

Fluorescence Correlation Spectroscopy (FCS) a new analytical technology, allows binding properties to be determined very accurately in biological assays at the level of single molecules. At concentrations of > or = 10(-12) M, binding constants, on/off-rates, and even reaction/enzyme kinetics can be determined in real-time, and in sample volumes as low as 10(-9) microliters. The FCS technology can be applied to study molecular and cellular interactions in homogeneous assays. Assay times in the range of seconds in combination with nanoliter sample volumes allow FCS to be used for high throughput screening to identify new pharmaceutical lead structures or new pharmacological targets. FCS is fully compatible with standard microtiter plate formats. However, for high throughput screening, specially designed sample carriers containing many thousand sub-microliter sample wells may be used in combination with a nanopipetting and sample retrieval system.

Published
1997
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22. 6xHis-Ni-NTA chromatography as a superior technique in recombinant protein expression/purification.

Author

Crowe J, Döbeli H, Gentz R, Hochuli E, Stüber D, and Henco K

Subjects
Chelating Agents, Escherichia coli genetics, Genetic Vectors, Nickel metabolism, Nitrilotriacetic Acid, Operator Regions, Genetic, Promoter Regions, Genetic, Recombinant Fusion Proteins biosynthesis, Chromatography, Affinity methods, Histidine, Recombinant Fusion Proteins isolation & purification
Published
1994
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24. Quantitative determination of human cytomegalovirus target sequences in peripheral blood leukocytes by nested polymerase chain reaction and temperature gradient gel electrophoresis.

Author

Schäfer P, Braun RW, Möhring K, Henco K, Kang J, Wendland T, and Kühn JE

Subjects
Base Sequence, Blood Donors, Cytomegalovirus genetics, Cytomegalovirus Infections genetics, Genome, Viral, Globins genetics, Humans, Kidney Transplantation adverse effects, Molecular Sequence Data, Transplantation, Homologous adverse effects, Cytomegalovirus isolation & purification, Cytomegalovirus Infections diagnosis, DNA, Viral blood, Electrophoresis, Polyacrylamide Gel methods, Leukocytes microbiology, Polymerase Chain Reaction methods
Abstract

A competitive nested PCR-temperature gradient gel electrophoresis protocol (nPCR/TGGE) has been established for the quantification of human cytomegalovirus (HCMV) target sequences. The measurement was achieved by co-amplification of a defined copy number of an internal standard (st) and separation of st and wild-type (wt) amplimers by temperature gradient gel electrophoresis (TGGE). The number of HCMV target sequences could be precisely determined within wt/st ratios of 0.1 to 10. With 50 copies of the st sequence the detection limit of nPCR/TGGE was found to be five to 10 copies of the target sequence. Effects of sample preparation on quantitative HCMV PCR were minimized by the additional quantification of beta-globin target sequences and calculation of the ratio of HCMV copies/beta-globin copies. Serial peripheral blood leukocyte specimens of 17 renal allograft recipients positive in a qualitative nested HCMV PCR were tested using nPCR/TGGE. Thirty healthy blood donors served as negative controls. Positive results were obtained by nPCR/TGGE in nine renal allograft recipients but in none of the healthy blood donors. Five of five patients with an HCMV pp65 antigenaemia and positive for HCMV IgM were positive in nPCR/TGGE. The highest HCMV/beta-globin ratios (10,000 to 8000 copies HCMV/10(6) copies beta-globin) were found in transplant recipients experiencing acute clinically symptomatic HCMV infection. HCMV DNA levels in asymptomatic patients ranged from 900 to 200 copies HCMV/10(6) beta-globin.

Published
1993
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25. Temperature-gradient gel electrophoresis for the detection of polymorphic DNA and for quantitative polymerase chain reaction.

Author

Riesner D, Steger G, Wiese U, Wulfert M, Heibey M, and Henco K

Subjects
DNA Mutational Analysis, Humans, Nerve Tissue Proteins genetics, Polymorphism, Genetic, PrPSc Proteins, Prion Diseases genetics, Prions genetics, Temperature, DNA genetics, DNA isolation & purification, Electrophoresis, Polyacrylamide Gel methods, Polymerase Chain Reaction methods
Abstract

In order to detect mutations in a gene, either known mutations from human diseases or artificial ones in transgenic animals, or to screen for not yet identified mutations in patients, a method is required which guarantees detection of mutations which might occur in every single position of the whole open reading frame (ORF). It will be shown that a combination of polymerase chain reaction (PCR) and temperature gradient gel electrophoresis (TOGE) fulfills these requirements. By thermodynamic calculations the shift in the gel electrophoresis due to a mutation can be calculated in dependence on the position of the mutation. The theoretical results were tested with the mutations known so far. The quantitative determination of the copy number of a specific DNA or RNA sequence in a biological specimen (quantitative PCR) can be performed precisely and easily by combining PCR and TGGE. The system uses a quantification strategy of a new type of internal standardization. TGGE is applied to separate homo- and heteroduplexes which correspond respectively to standard and template sequences. The accuracy of this quantification strategy is very high, with a variability of < 15%. In addition to quantification, PCR/TGGE detects PCR artifacts and template mutants.

Published
1992
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26. Direct sequencing of variable HLA gene segments after in vitro amplification and allele separation by temperature-gradient gel electrophoresis.

Author

Meyer CG, Tannich E, Harders J, Henco K, and Horstmann RD

Subjects
Amino Acid Sequence, Base Sequence, Electrophoresis, Agar Gel, Humans, Molecular Sequence Data, Oligonucleotide Probes genetics, Polymerase Chain Reaction, Polymorphism, Genetic, Sequence Homology, Nucleic Acid, HLA Antigens genetics, Immunophenotyping methods
Abstract

Previously unrecognized variants of human leukocyte antigens (HLA) are currently being analyzed by in vitro amplification and sequencing of the variable gene segments. In heterozygous individuals, molecular cloning is required to separate the two concomitantly amplified haplotypic gene segments. A method is presented which facilitates the procedure of separating the two haplotypic gene segments by using a temperature-gradient gel electrophoresis (TGGE). The procedure comprises PCR amplification of the variable HLA gene segments, allele separation by TGGE, re-amplification of each of the separated allelic segments, and direct DNA sequencing using the PCR primers.

Published
1991
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27. Temperature-gradient gel electrophoresis of nucleic acids: analysis of conformational transitions, sequence variations, and protein-nucleic acid interactions.

Author

Riesner D, Steger G, Zimmat R, Owens RA, Wagenhöfer M, Hillen W, Vollbach S, and Henco K

Subjects
Base Sequence, DNA analysis, Electrophoresis, Polyacrylamide Gel instrumentation, Molecular Sequence Data, Molecular Structure, Mosaic Viruses analysis, Nucleic Acid Denaturation, Nucleic Acid Renaturation, Plasmids, RNA analysis, Staining and Labeling, Temperature, Viroids analysis, DNA-Binding Proteins analysis, Electrophoresis, Polyacrylamide Gel methods, Nucleic Acid Conformation, Nucleic Acids analysis
Abstract

Temperature-gradient gel electrophoresis (TGGE) is applied to analyze conformational transitions and sequence variations of nucleic acids and protein-nucleic acid interactions. A linear and highly reproducible temperature-gradient is established perpendicular or parallel to the direction of the electrophoresis. The instrument consists of an electrically insulated metal plate, which is heated at one edge and cooled at the other edge by two thermostating baths and is used as an ancillary device for commercial horizontal gel electrophoresis instruments. Biopolymers are separated in TGGE according to size, shape and thermal stability of their conformational transitions. If the temperature-gradient is established perpendicular to the electrophoresis, monomolecular conformational transitions of nucleic acids show up as continuous transition curves; strand-separation leads to discontinuous transitions. In the studies on viroid RNA it was shown that natural circular viroid RNA undergoes one highly cooperative transition detected by TGGE as a drastic retardation in mobility. Oligomeric replication intermediates of viroids exhibit coexisting structures which could not be detected by any other technique. Double-stranded satellite RNA from cucumber mosaic virus is a mixture of sequence variants, all of which have the identical length of 335 nucleotides. In TGGE six different strains were resolved. Sequence variants of viroids were analyzed by hybridizing viroid RNA to (-)strand viroid RNA transcripts from viroid cDNA clones. Sequence variations lead to mismatches in the double strands and thereby to a shift of the transition curve to lower temperature. Mutations in plasmids, particularly in cloned inserts, were detected by mixing plasmids of two different clones, linearizing, denaturing, renaturing, and searching for shifts in the transition curves, which are generated by mismatch-formation during the renaturation of (+)- and (-)strands from different clones. Examples are given for different viroid clones and HIV-clones from one and the same patient. In another example, clones with point mutations from site-directed mutagenesis are analyzed and selected by TGGE. TGGE is also applied to study the effect of amino acid exchanges in the Tet repressor from E. coli on the thermal stability of the repressor and on the mode of binding of the repressor to the operator DNA. The results are discussed under the aspect that TGGE may be applied as routine analytical laboratory procedure.

Published
1989
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29. Structure and expression of human IFN-alpha genes.

Author

Weissmann C, Nagata S, Boll W, Fountoulakis M, Fujisawa A, Fujisawa JI, Haynes J, Henco K, Mantei N, Ragg H, Schein C, Schmid J, Shaw G, Streuli M, Taira H, Todokoro K, and Weidle U

Subjects
Base Sequence, Biological Evolution, Cloning, Molecular, DNA genetics, DNA, Recombinant, Escherichia coli genetics, Gene Amplification, Gene Expression Regulation, Genes, Humans, Interferon Type I classification, RNA, Messenger genetics, Receptors, Cell Surface physiology, Receptors, Interferon, Interferon Type I genetics
Abstract

Copy DNA (cDNA) was prepared from induced leucocyte poly(A) RNA and cloned in Escherichia coli. IFN-alpha cDNA clones were isolated by subculture cloning with the use of a translation hybridization assay. Definitive identification of the clones was based on the production of an interferon-like protein by the transformed bacteria. Different IFN-alpha cDNAs, with characteristic target cell specificities, were identified. The cloned cDNAs typically encode a mature polypeptide of 166 (or, for IFN-alpha 2, 165) amino acids and a signal sequence of 23 amino acids. A human chromosomal library was screened with IFN cDNA and 17 distinct IFN-alpha-related sequences were isolated and identified, of which 7 proved to be nonallelic authentic genes and 4 pseudogenes; 6 sequences remain to be elucidated. Taking into account the work of Goeddel and his colleagues, 13 non-allelic authentic genes and 6 pseudogenes can be distinguished. In addition, 9 genes believed to be allelic to the 13 authentic genes have been sequenced. The IFN-alpha genes may be classified into two major subfamilies, which diverged at least 33 Ma ago, but perhaps much earlier, if sequence rectification occurred. At least one IFN-alpha gene appears to have resulted by a recombinational event between members of the subfamily I and II. IFN-beta is distantly related to IFN-alpha's and may have diverged from a common ancestor at least 500 Ma ago. Both IFN-alpha and IFN-beta genes differ from most other genes of higher organisms by being devoid of introns. The mouse was found to possess an IFN-alpha gene family of a size similar to that of man; the murine genes also do not have introns. IFN-alpha genes devoid of their signal sequence were joined to prokaryotic promoters to produce the mature interferons in E. coli in high yield. IFN-alpha 2, purified to homogeneity, has been crystallized by T. Unge and B. Strandberg (Uppsala). Hybrid genes consisting of IFN-alpha 1 and IFN-alpha 2 segments were constructed and expressed in E. coli; the target cell specificities of such hybrids were dependent on the arrangement of the segments and were different from those of either parent. The chromosomal gene for HuIFN-alpha 1 was introduced into mouse L cells to study the mechanism of its expression. Correct transcription was only detected after induction (with Newcastle disease virus); expression was transient, with the same kinetics as those of the endogenous mouse IFN mRNA. Natural murine IFNs and human IFN-beta and IFN-gamma are glycosylated. Because E. coli cells transformed with the genes of eukaryotic glycoproteins are not expected to yield correctly glycosylated polypeptides, we prepared lines of hamster cells permanently transformed with hybrid plasmids, which contained an IFN gene linked to the SV40 early promoter, as well as dihydrofolate reductase as a selective marker. After intracellular amplification of the introduced genes, cell lines were obtained which constitutively produced IFN at about 40 000 units ml-1 and could be propagated for at least several months.

Published
1982
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30. Isolation of variants of lymphocytopathic retroviruses from the peripheral blood and cerebrospinal fluid of patients with ARC or AIDS.

Author

Rübsamen-Waigmann H, Becker WB, Helm EB, Brodt R, Fischer H, Henco K, and Brede HD

Subjects
Acquired Immunodeficiency Syndrome blood, Acquired Immunodeficiency Syndrome cerebrospinal fluid, Cytopathogenic Effect, Viral, DNA, Viral analysis, Fluorescent Antibody Technique, Humans, Immunologic Techniques, Lymphocytes, Microscopy, Electron, Nucleic Acid Hybridization, RNA-Directed DNA Polymerase analysis, Retroviridae Infections blood, Retroviridae Infections cerebrospinal fluid, Acquired Immunodeficiency Syndrome microbiology, Deltaretrovirus isolation & purification, Retroviridae Infections microbiology
Abstract

LAV/HTLV-III/AAV viruses were isolated from 20 German patients with ARC/AIDS in order to investigate strain variation. Virus was isolated from the peripheral blood and/or cerebrospinal fluid (CSF) in umbilical cord peripheral blood lymphocyte (PBL) cultures. Isolates were identified by their cytopathic effect (CPE), by reverse transcriptase assays on cell-free infected culture supernatant fluid (SNF), and one or more of the following: immunofluorescence assays on infected cells for viral antigen using HTLV-III reference sera, Western blot analysis of cell-free infected culture SNF, electron microscopy of infected cells, and Southern blot restriction analysis and specific HTLV-III probing of DNA extracted from infected cultured PBL. The isolates could be classified into three groups according to differences in growth rate and cytopathic effect: Most showed what was regarded as the typical CPE, while some either grew rapidly and induced a striking CPE and others grew slowly with minimal CPE. In one patient, virus producing typical CPE was isolated from the peripheral blood while the isolate from his filtered cell-free CSF produced atypical slow CPE, suggesting that antigenic variation may occur with persistent infection or that superinfection may occur. Southern blot DNA restriction analysis of the DNA of three selected isolates showed that two of the isolates were similar but that the restriction pattern of all three differed from patterns previously published. Our results supplement the accumulating evidence of genetic variation among LAV/HTLV-III strains. The extent of this variation needs to be evaluated for any effect on the sensitivity of diagnostic tests, on the strategy of vaccine development, on tissue tropism by altering the viral surface receptor-binding sites, and possibly on the development of specific chemotherapy.

Published
1986
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31. Structure and expression of human alpha-interferon genes.

Author

Weismann C, Nagata S, Boll S, Fountoulakis M, Fujisawa A, Fujisawa J, Haynes J, Henco K, Mantei N, and Ragg H

Subjects
Amino Acid Sequence, Base Sequence, Escherichia coli genetics, Humans, Leukocytes immunology, Nucleic Acid Hybridization, Poly A genetics, Protein Biosynthesis, RNA genetics, RNA, Messenger, Cloning, Molecular, DNA metabolism, Genes, Interferon Type I genetics
Abstract

cDNA was prepared from induced leukocyte poly(A) RNA and cloned in Escherichia coli. Interferon (IFN)-alpha cDNA clones were isolated by subculture cloning using a translation hybridization assay. Definitive identification of the clones was based on the production of an interferon-like protein by the transformed bacteria. Different IFN-alpha cDNAs, with characteristic target cell specificities, were identified. The cloned cDNAs typically encode a mature polypeptide of 166 (or, in the case of IFN-alpha 2, 165) amino acids and a signal sequence of 23 amino acids.

Published
1982

32. Common structural features of different viroids: serial arrangement of double helical sections and internal loops.

Author

Langowski J, Henco K, Riesner D, and Sänger HL

Subjects
Mathematics, Nucleic Acid Conformation, Nucleic Acid Denaturation, Thermodynamics, Plant Viruses ultrastructure, RNA, Viral
Abstract

The thermodynamic parameters of five different highly purified viroid "species" were determined by applying UV-absorption melting analysis and temperature jump methods. Their thermal denaturation proved to be a highly cooperative process with midpoint-temperatures (Tm) between 48.5 and 51 degrees C in 0.01 M sodium cacodylate, 1 mM EDTA, pH 6.8. The values of the apparent reaction enthalpies of the different viroid species range between 3,140 and 3,770 kJ/mol. Although the cooperativity is as high as found in homogeneous RNA double helices the Tm-value of viroid melting is more than 30 degrees C lower than in the homogeneous RNA. In order to explain this deviation, melting curves were simulated for different models of the secondary structure of viroids using literature values of the thermodynamic parameters of nucleic acids. Our calculations show that the following refinement of our earlier model is in complete accordance with the experimental data: In their native conformation viroids exist as an extended rodlike structure characterized by a series of double helical sections and internal loops. In the different viroid species 250-300 nucleotides out of total 350 nucleotides are needed to interprete the thermodynamic behaviour.

Published
1978
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33. Partial mapping of ten genes of the human interferon- alpha family.

Author

Nagata S, Brack C, Henco K, Schamböck A, and Weissmann C

Subjects
Alleles, Base Sequence, DNA Restriction Enzymes, DNA, Recombinant, Genes, Genetic Linkage, Humans, Nucleic Acid Hybridization, Interferons genetics
Abstract

HulFN-alpha genes form a family of not less than 9-10 distinct members, at least three of which are arranged in tandem. In one case, two variants, believed to be alleles of the same gene, could be identified by sequence analysis. The three gene sequenced so far are devoid in introns.

Published
1981
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34. Fine structure melting of viroids as studied by kinetic methods.

Author

Henco K, Sänger HL, and Riesner D

Subjects
Base Sequence, Kinetics, Nucleic Acid Conformation, Nucleic Acid Denaturation, Temperature, Plant Viruses analysis, RNA, Viral
Abstract

The conformational transitions of five viroid species were studied by melting analysis and by fast and slow temperature jump techniques. Experiments with the fast temperature jump technique had to be carried out in 10 mM Na-cacodylate, 0.1 M NaCl, 4 M urea, 1 mM EDTA, pH 6.8. In addition to the highly cooperative main transition (Tm between 46.5 and 49 degrees C for different viroid species [1]) all viroids show at higher temperatures an intermediate transition (Tm approximately equal to 57 degrees C) and a high temperature transition (Tm approximately equal to 68 degrees C). The maximum amplitudes of these transitions amount only to about 1% of that of the main transition. The main transition represents a net dissociation of 78 to 94 base pairs depending on the viroid species. The intermediate transition corresponds to the dissociation of two hairpins with 5-10 base pairs each, and 10-20 nucleotides in the loops. The high temperature transition corresponds to a hairpin of 9 G:C pairs and 1 A:U pair and more than 40 bases in the loop. It is shown that these stable hairpins are not part of the native structure but are newly formed during the main transition. Their formation is responsible for the extraordinary cooperativity observed in the main transition. Hairpins can be correlated to defined sequences of PSTV. Based on these studies, on the sequence of PSTV [2], and on a theoretical treatment [3] a detailed description of the whole mechanism of PSTV denaturation is given.

Published
1979
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35. Structure and structure formation of viroids.

Author

Riesner D, Henco K, Rokohl U, Klotz G, Kleinschmidt AK, Domdey H, Jank P, Gross HJ, and Sänger HL

Subjects
Aniline Compounds, Benzimidazoles, Coloring Agents, Ethidium, Microscopy, Electron, RNA, Viral, Temperature, Thermodynamics, Plant Viruses isolation & purification, Virion isolation & purification, Virion ultrastructure
Published
1979
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36. Modulation of the nucleosome structure by histone acetylation.

Author

Bode J, Henco K, and Wingender E

Subjects
Acetylation, Animals, Butyrates, Cell Cycle, Chickens, Cricetinae, Cricetulus, Erythrocytes, Female, Hot Temperature, Macromolecular Substances, Molecular Conformation, Ovary cytology, Protamines pharmacology, Histones, Nucleosomes drug effects
Abstract

A rapid procedure for the isolation of core particles from Chinese hamster ovary cells is described which permits measurements, usually at the day of their preparation. Particles of 145 +/- 5 base pairs, derived from interphase cells, will be compared with the analogue specimens from butyrate-treated cells, metaphase cells and a standard preparation from chicken erythrocytes. Butyrate cause an increase in the acetylation of histones H3 and H4, which induces alterations of the interhistone and histone-DNA interactions. Changes in the interhistone contacts, correlated to an extension of alpha-helical segments, lead to an altered accessibility of the H3 cysteine side-chains and to a different histone displacement by protamines. On the other hand, histone-DNA contacts are loosened in parts and this is particularly evident from the changes in the premelting region of a thermal-denaturation profile.

Published
1980
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37. Isolation frequency and growth properties of HIV-variants: multiple simultaneous variants in a patient demonstrated by molecular cloning.

Author

von Briesen H, Becker WB, Henco K, Helm EB, Gelderblom HR, Brede HD, and Rübsamen-Waigmann H

Subjects
Blood microbiology, Cells, Cultured, Cerebrospinal Fluid microbiology, Cloning, Molecular, Cytopathogenic Effect, Viral, DNA Restriction Enzymes, DNA, Viral genetics, Genes, Viral, HIV genetics, HIV growth & development, HIV physiology, Humans, Lymphocytes microbiology, Polymorphism, Restriction Fragment Length, Virus Replication, AIDS-Related Complex microbiology, Acquired Immunodeficiency Syndrome microbiology, HIV isolation & purification
Abstract

The biological properties and efficiency of isolation of different HIV (LAV/HTLV III, ARV, and AAV) subtypes were evaluated by recovering and growing HIV on fresh peripheral human lymphocytes. Cultures for virus isolation were performed from more than 180 German AIDS, ARC, LAS, and virus-exposed asymptomatic patients. The virus isolation rate depended on the state of health of the patients being close to 80% in AIDS patients, 30-40% in ARC/LAS patients, and lower in asymptomatic HIV seropositive patients. The cytopathic effects of the HIV isolates obtained on lymphocyte-cell cultures ranged from no effect to marked syncytia formation and cytopathogenicity. Marked differences were also observed in the replication rate of the various isolates. These properties were stable in all in vitro passages of the viruses performed so far and allowed to tentatively define four subtypes of HIV. In the majority of AIDS cases with neurological symptoms well-growing strains were obtained from peripheral blood, while all but two isolates from the cerebrospinal fluid of the same patients grew remarkably slowly and to only low titres on lymphocytes, suggesting that selection of variants for growth at specific sites of the body occurs. For one of the most cytopathogenic strains the influence of several variables of culture conditions (cell type, corticosteroids, IL-2, and polybrene) on virus replication was studied. Apart from polybrene, all parameters strongly influenced replication.

Published
1987
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