ALBERT — All Library Books, journals and Electronic Records Telegrafenberg

1

Electronic Resource

Incorporation of phosphorothioate groups into fd and φX174 DNA (1977)

Vosberg, Hans Peter ; Eckstein, Fritz

s.l. : American Chemical Society

Biochemistry 16 (1977), S. 3633-3640

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ISSN: 1520-4995

Source: ACS Legacy Archives

Topics: Biology , Chemistry and Pharmacology

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1021/bi00635a020

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2

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Cardiac myosin binding protein–C gene splice acceptor site mutation is associated with familial hypertrophic cardiomyopathy (1995)

Bonne, Gisèle ; Carrier, Lucie ; Bercovici, Josiane ; [et al.]

[s.l.] : Nature Publishing Group

Nature genetics 11 (1995), S. 438-440

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ISSN: 1546-1718

Source: Nature Archives 1869 - 2009

Topics: Biology , Medicine

Notes: [Auszug] To refine the limits of CMH4, we conducted a detailed genetic analysis on the first family linked to this locus, Family 714. Analysis of forty microsatellite markers indicated four recombinant individuals, III-l, III-11, IV-4 and IV-9, which when analysed reduced the locus from 17 cM5 to 5 cM (Fig. ...

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1038/ng1295-438

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3

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Molecular cloning of DNA (1977)

Vosberg, Hans-Peter

Springer

Human genetics 〈Berlin〉 40 (1977), S. 1-72

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ISSN: 1432-1203

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Summary Biochemical, biophysical and genetic studies of DNA segments of complex genomes are greatly facilitated by a variety of techniques, called molecular cloning of DNA, which permit propagation of single DNA segments of virtually any origin in bacterial cells. Molecular cloning requires in vitro recombination of DNA fragments with a prokaryotic genetic element (a plasmid or a bacteriophage DNA) which serves as replication vehicle (also called vector) in the bacterial host. The experimental conditions allow the production of bacterial clones each harboring a single fragment of exogeneous DNA out of an initially highly heterogeneous mixture of fragments. The following steps are involved: foreign DNA is first dissected into small pieces of up to some 17 000 basepairs in length. The fragments are then joined in vitro to the vector molecules by means of well characterized DNA enzymes. The resulting recombinant molecules are introduced into the host cells by a transformation or transfection step. Among the progeny of transformed or transfected cells those clones are selected which carry a fragment of interest. Selection is in most cases accomplished by a combination of genetic and physical methods and is based on properties of the vectors as well as on attributes of the cloned foreign DNA. It is anticipated that bacterial host cells are not only suitable for amplifying DNA but also for the expression of useful functions which originate from other, preferably higher organisms. Two questions cannot be answered conclusively at present: first, is functional expression of genes generally possible in a heterologous cellular environment, and second, if it is possible, is it always harmless or does it create, at least occasionally, a biological hazard. Besides a detailed description of the techniques developed for molecular cloning, problems connected with functional expression and biohazards are discussed. In addition, results are presented which were obtained in the recent past by applying DNA cloning procedures.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00280831

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4

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Intracellular distribution of DNA topoisomerase I in fibroblasts from patients with Fanconi's anaemia (1982)

Auer, Benhard ; Vosberg, Hans-Peter ; Buhre, Ursula ; [et al.]

Springer

Human genetics 〈Berlin〉 61 (1982), S. 369-371

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ISSN: 1432-1203

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Summary The activity of DNA topoisomerase I (DNA nicking-closing enzyme) was analysed in cytoplasmic and nuclear extracts of six independently derived Fanconi and four normal fibroblast cell lines. In all experiments the total cellular activity was predominantly found in the nuclear extracts (88–100%). In addition, a minor proportion of the enzyme (up to 12%) was randomly present in some of the cytoplasmic fractions of both Fanconi and normal fibroblasts. These results indicate that Fanconi's anaemia is probably not due to or accompanied by a maldistribution of topoisomerase I between nuclei and cytoplasm.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00276603

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5

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Genomic structure and fine mapping of the two human filamin gene paralogues FLNB and FLNC and comparative analysis of the filamin gene family (2000)

Chakarova, Christina ; Wehnert, Manfred ; Uhl, Kerstin ; [et al.]

Springer

Human genetics 〈Berlin〉 107 (2000), S. 597-611

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ISSN: 1432-1203

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Abstract. The genomic structure of the filamin gene paralogues FLNB and FLNC was determined and related to FLNA. FLNB consists of 45 exons and 44 introns and spans ~80 kb of genomic DNA. FLNC is divided into 48 exons and 47 introns and covers ~29.5 kb of genomic DNA. A previously unknown intron was found in FLNA. The comparison of all three filamin gene paralogues revealed a highly conserved exon-intron structure with significant differences in the exons 32 of all paralogues encoding the hinge I region, as well as the insertion of a novel exon 40A in FLNC only. Gene organization does not correlate with the domain structures of the respective proteins. To improve candidate gene cloning approaches, FLNB was precisely mapped at 3p14 in an interval of 0.81 cM between WI3771 and WI6691 and FLNC at 7q32 in an interval of 2.07 cM between D7S530 and D7S649.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/s004390000414

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6

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The polymerase chain reaction: an improved method for the analysis of nucleic acids (1989)

Vosberg, Hans-Peter

Springer

Human genetics 〈Berlin〉 83 (1989), S. 1-15

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ISSN: 1432-1203

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Summary The polymerase chain reaction (PCR) is a method for the selective amplification of DNA or RNA segments of up to 2 kilobasepairs (kb) or more in length. Synthetic oligonucleotides flanking sequences of interest are used in repeated cycles of enzymatic primer extension in opposite and overlapping directions. The essential steps in each cycle are thermal denaturation of double-stranded target molecules, primer annealing to both strands and enzymatic synthesis of DNA. The use of the heat-stable DNA polymerase from the archebacterium Thermus aquaticus (Taq polymerase) makes the reaction amenable to automation. Since both strands of a given DNA segment are used as templates, the number of target sequences increases exponentially. The reaction is simple, fast and extremely sensitive. The DNA or RNA content of a single cell is sufficient to detect a specific sequence. This method greatly facilitates the diagnosis of mutations or sequence polymorhisms of various types in human genetics, and the detection of pathogenic components and conditions in the context of clinical research and diagnostics; it is also useful in simplifying complex analytical or synthetic protocols in basic molecular biology. This article describes the principles of the reaction and discusses the applications in different areas of biomedical research.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00274139

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7

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Isolation and characterization of the complete human β-myosin heavy chain gene (1989)

Diederich, Klaus W. ; Eisele, Ingrid ; Ried, Thomas ; [et al.]

Springer

Human genetics 〈Berlin〉 81 (1989), S. 214-220

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ISSN: 1432-1203

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Summary The entire gene coding for the human β-myosin heavy chain has been isolated from genomic EMBL3A phage libraries by chromosomal walking starting from clone gMHC-1, reported earlier (Appelhans and Vosberg 1983). gMHC-1 has been shown to carry coding information for the C-terminal two-thirds of β-myosin heavy chain, which is expressed in cardiac muscle and in slow skeletal muscle fibers (Lichter et al. 1986). Three DNA clones were identified as overlapping with gMHC-1 by restriction mapping and DNA sequencing. They span a 30-kb region in the genome. About 22 kb extend from the initiation codon ATG to the poly(A) addition site. The clones include about 4 kb of 5′ flanking sequences upstream of the promoter. Comparisons of β- and α-myosin heavy chain sequences indicate that gene duplication of the cardiac myosin heavy chain isogenes preceded the mammalian species differentiation.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00278991

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8

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Scl 70 autoantibodies from scleroderma patients recognize a 95 kDa protein identified as DNA topoisomerase I (1986)

Guldner, Hans-Herbert ; Szostecki, Carin ; Vosberg, Hans-Peter ; [et al.]

Springer

Chromosoma 94 (1986), S. 132-138

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ISSN: 1432-0886

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Abstract Sera of patients suffering from the autoimmune disease progressive systemic sclerosis (PSS) are known to contain autoantibodies which have been reported to recognize a 70 kDa antigenic protein, designated the Scl 70 antigen. By immunoblotting of nuclear extracts from HeLa cells with sera from scleroderma patients we observed that the size of the antigen present in such cells depends on the conditions of antigen isolation. When protease inhibitors were included in the extraction buffer, a 95 kDa protein was identified instead of a 70 kDa protein. When protease inhibitors were omitted, a number of polypeptides in the size range 66 to 95 kDa was found. Furthermore, antibodies which had been affinity purified on the 95 kDa antigen, crossreacted with the 66 to 95 kDa polypeptides. These results suggest that the smaller proteins were degradation products of the 95 kDa antigen. Immunofluorescence studies on PtK-2 cells with the antibody specific for the 95 kDa protein gave staining of nuclei, nucleoli and of chromosomes and the nucleolar organizer region in mitotic cells. Since this distribution of antigens within the nucleus was reminiscent of the intranuclear distribution of DNA topoisomerase I found by others we probed purified DNA topoisomerase I from calf thymus directly with the autoantibodies from PSS patients, and also the 95 kDa antigens of HeLa cell nuclei with antibodies raised against the bovine DNA topoisomerase I. From the crossreaction pattern observed with the different antigens and antibodies we conclude that DNA topoisomerase I is one of the antigenic components against which autoantibodies are formed in scleroderma patients.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00286991

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9

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Expression of human β-myosin heavy chain fragments inEscherichia coli; localization of actin interfaces on cardiac myosin (1990)

Eldin, Patrick ; Cunff, Martine ; Diederich, Klaus W. ; [et al.]

Springer

Journal of muscle research and cell motility 11 (1990), S. 378-391

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ISSN: 1573-2657

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Summary A cDNA clone coding for an internal fragment of slow-cardiacβ-myosin heavy chain was isolated from aλgt10 human skeletal muscle library. Six overlapping cDNA subclones, which span myosin heavy chain subregions and presumably interact with actin, were derived from this clone, fused to aβ-galactosidase vector and expressed inEscherichia coli. Three of the subclones were obtained by PCR (polymerase chain reaction) which enables gene or cDNA fragments to be amplified independently of preexisting restriction sites. Initially, various experiments were carried out using a long MHC (myosin heavy chain) fusion protein containing the 50 kDa-20 kDa connecting region, the whole 20 kDa region and the short subfragment 2 region. This MHC fusion protein was chemically or proteolytically cleaved in the same conditions as the native myosin molecule. Whole and truncated forms of the MHC fusion protein were separated on polyacrylamide gels, electroblotted on nitrocellulose sheets and renatured. They were then assayed in overlay experiments with F-actin and/or myosin light chains in solution. Specific antibodies were used to detect interactions between heavy chain fragments and F-actin or light chains. We thus observed that one long heavy chain fragment synthesized byE. coli behaved like proteolytic or chemical MHC preparations made from native myosin molecules. Two chymotryptic fragments of the MHC fusion protein, which are soluble at low ionic strength, cosedimented with F-actin in solution. Our results demonstrate that, in actin overlay experiments with whole fusion proteins, interactions seem to be due to the heavy chain fragment, not to the bacterial component. All interactions were non ATP-sensitive. We further investigated the possible participation of the six recombinant MHC fragments in contributing to the actomyosin interfaces on the 50 kDa-20 kDa regions of the human cardiacβ-MHC. The present procedure, which enables the synthesis of any MHC fragment independent of any protease site, is a powerful new tool for studying structure-function relationships within the myosin molecule family.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01739759

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