15 results on '"Niemann, Heiner"'
Search Results
2. Transgenic Pigs Expressing Plant Genes
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Niemann, Heiner
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- 2004
3. Assessment of Fetal Cell Chimerism in Transgenic Pig Lines Generated by Sleeping Beauty Transposition.
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Garrels, Wiebke, Holler, Stephanie, Taylor, Ulrike, Herrmann, Doris, Niemann, Heiner, Ivics, Zoltan, and Kues, Wilfried A.
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CHIMERISM ,CELL culture ,CELL lines ,TRANSGENIC animals ,LABORATORY swine ,SEMEN - Abstract
Human cells migrate between mother and fetus during pregnancy and persist in the respective host for long-term after birth. Fetal microchimerism occurs also in twins sharing a common placenta or chorion. Whether microchimerism occurs in multiparous mammals such as the domestic pig, where fetuses have separate placentas and chorions, is not well understood. Here, we assessed cell chimerism in litters of wild-type sows inseminated with semen of transposon transgenic boars. Segregation of three independent monomeric transposons ensured an excess of transgenic over non-transgenic offspring in every litter. Transgenic siblings (n = 35) showed robust ubiquitous expression of the reporter transposon encoding a fluorescent protein, and provided an unique resource to assess a potential cell trafficking to non-transgenic littermates (n = 7) or mothers (n = 4). Sensitive flow cytometry, fluorescence microscopy, and real-time PCR provided no evidence for microchimerism in porcine littermates, or piglets and their mothers in both blood and solid organs. These data indicate that the epitheliochorial structure of the porcine placenta effectively prevents cellular exchange during gestation. [ABSTRACT FROM AUTHOR]
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- 2014
- Full Text
- View/download PDF
4. Long-term effects of PERV-specific RNA interference in transgenic pigs.
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Semaan, Marwan, Kaulitz, Danny, Petersen, Björn, Niemann, Heiner, and Denner, Joachim
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RNA interference ,XENOTRANSPLANTATION ,TRANSGENIC animals ,SWINE ,FLUORESCENCE microscopy ,FIBROBLASTS ,WESTERN immunoblotting - Abstract
Semaan M, Kaulitz D, Petersen B, Niemann H, Denner J. Long-term effects of PERV-specific RNA interference in transgenic pigs. Xenotransplantation 2012; 19: 112-121. © 2012 John Wiley & Sons A/S. Abstract: Background: Porcine endogenous retroviruses (PERVs) represent a risk of xenotransplantation using porcine cells, tissues, or organs, as they are integrated in the porcine genome and have been shown to be able to infect human cells in vitro. To increase viral safety by RNA interference, transgenic pigs expressing a PERV-specific small hairpin (sh)RNA targeted to a highly conserved sequence in the pol gene (pol2) were generated in which expression of PERVs was reduced (Xenotransplantation, 15, 2008, 38). However, it remains to be shown how long expression of the shRNA and the RNA interference is effective in reducing PERV expression. Methods: To analyze the long-term duration of RNA interference, expression of the PERV-specific pol2 shRNA and inhibition of PERV expression was studied repeatedly in fibroblasts and peripheral blood mononuclear cells (PBMCs) of transgenic pigs over a period of 3 yr, when animals were sacrificed and expression was studied in different organs. Expression of the PERV-specific shRNA was measured using a newly developed real-time PCR, and expression of PERV was measured using a PERV-specific real-time PCR. Results: Over a period of 3 yr, PERV-specific shRNA and green fluorescent protein (GFP) as reporter of the vector system were consistently expressed in transgenic animals. PERV expression was significantly reduced during the entire period. Levels of PERV and shRNA expression were different in the various organs. PERV expression was highest in the spleen and the lungs and lowest in liver and heart. However, in all organs of the transgenic pigs, PERV expression was inhibited compared with the vector control animals. Conclusions: Transgenic pigs expressing PERV-specific shRNA maintained their specific RNA interference long term, suggesting that PERV expression in the xenotransplants will be suppressed over extended periods of time. [ABSTRACT FROM AUTHOR]
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- 2012
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5. Advances in farm animal transgenesis
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Kues, Wilfried A. and Niemann, Heiner
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DOMESTIC animals , *TRANSGENIC animals , *GENE silencing , *EPIGENESIS , *GENOMES , *MICROINJECTIONS , *DNA - Abstract
Abstract: The first transgenic livestock were produced in 1985 by microinjection of foreign DNA into zygotic pronuclei. This was the method of choice for more than 20 years, but more efficient protocols are now available, including somatic cell nuclear transfer and lentiviral transgenesis. Typical applications include carcass composition, lactational performance and wool production, as well as enhanced disease resistance and reduced environmental impact. Transgenic farm animal production for biomedical applications has found broad acceptance. In 2006 the European Medicines Agency (EMA) approved commercialization of the first recombinant pharmaceutical protein, antithrombin, produced in the mammary gland of transgenic goats. As the genome sequencing projects for various farm animal species are completed, it has become feasible to perform precise genetic modifications employing the emerging tools of lentiviral vectors, small interfering ribonucleic acids, meganucleases, zinc finger nucleases and transposons. We anticipate that genetic modification of farm animals will be instrumental in meeting global challenges in agricultural production and will open new horizons in biomedicine. [Copyright &y& Elsevier]
- Published
- 2011
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6. Germline Transgenic Pigs by Sleeping Beauty Transposition in Porcine Zygotes and Targeted Integration in the Pig Genome.
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Garrels, Wiebke, Mátés, Lajos, Holler, Stephanie, Dalda, Anna, Taylor, Ulrike, Petersen, Björn, Niemann, Heiner, Izsvák, Zsuzsanna, Ivics, Zoltán, and Kues, Wilfried A.
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GERM cells ,TRANSGENIC animals ,CHROMOSOMAL translocation ,GENE targeting ,LABORATORY swine ,TRANSGENE expression ,TRANSPLANTATION of cell nuclei - Abstract
Genetic engineering can expand the utility of pigs for modeling human diseases, and for developing advanced therapeutic approaches. However, the inefficient production of transgenic pigs represents a technological bottleneck. Here, we assessed the hyperactive Sleeping Beauty (SB100X) transposon system for enzyme-catalyzed transgene integration into the embryonic porcine genome. The components of the transposon vector system were microinjected as circular plasmids into the cytoplasm of porcine zygotes, resulting in high frequencies of transgenic fetuses and piglets. The transgenic animals showed normal development and persistent reporter gene expression for>12 months. Molecular hallmarks of transposition were confirmed by analysis of 25 genomic insertion sites. We demonstrate germ-line transmission, segregation of individual transposons, and continued, copy number-dependent transgene expression in F1-offspring. In addition, we demonstrate target-selected gene insertion into transposon-tagged genomic loci by Cre-loxP-based cassette exchange in somatic cells followed by nuclear transfer. Transposase-catalyzed transgenesis in a large mammalian species expands the arsenal of transgenic technologies for use in domestic animals and will facilitate the development of large animal models for human diseases. [ABSTRACT FROM AUTHOR]
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- 2011
- Full Text
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7. Distribution and expression of porcine endogenous retroviruses in multi-transgenic pigs generated for xenotransplantation.
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Dieckhoff, Britta, Kessler, Barbara, Jobst, Danny, Kues, Wilfried, Petersen, Björn, Pfeifer, Alexander, Kurth, Reinhard, Niemann, Heiner, Wolf, Eckhard, and Denner, Joachim
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RETROVIRUSES ,TRANSPLANTATION of organs, tissues, etc. ,POLYMERASE chain reaction ,ANIMAL models in research ,TRANSGENIC animals ,MEDICAL research - Abstract
Background: Multi-transgenic pigs produced for use in xenotransplantation have to be screened for the presence and expression of porcine endogenous retroviruses (PERV) to select animals with low PERV load. The production of transgenic pigs may also be associated with the integration of the transgene adjacent to or into the locus of a PERV provirus, potentially leading to an enhanced virus expression. Methods: Non-transgenic animals, single-transgenic, and multi-transgenic pigs were screened for the presence of PERV-A, -B, and -C and recombinant PERV-A/C using polymerase chain reaction (PCR). PERV expression was determined by real time reverse transcriptase-PCR. An assay based on the activation of PERV in peripheral blood mononuclear cells by mitogens was used to discriminate between low and high PERV producer animals. Results: All animals carried PERV-A and -B. A total of 176 from 181 (97.2%) animals carried PERV-C in the germ line and 18 from 64 animals carried PERV-A/C in the genome of lymphoid cells but not in the germ line. The expression of PERV was very low in all animals and not different between transgenic pigs and non-transgenic animals. PERV expression differed between various pig lines. The highest expression was found in mini-pigs and crossing other pig lines with mini-pigs resulted in increased PERV expression in the progeny. However, expression of viral proteins and particle release were not observed in all transgenic animals. Conclusions: No evidence for elevated PERV expression in (multi-) transgenic pigs was observed. Differences in PERV expression correlated with the genetic background of the animals, not with the specific transgene. Mini-pigs consistently had the highest level of PERV expression and animals with a mini-pig background had a higher level of expression compared with animals without mini-pig background. [ABSTRACT FROM AUTHOR]
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- 2009
- Full Text
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8. Knockdown of porcine endogenous retrovirus (PERV) expression by PERV-specific shRNA in transgenic pigs.
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Dieckhoff, Britta, Petersen, Björn, Kues, Wilfried A., Kurth, Reinhard, Niemann, Heiner, and Denner, Joachim
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RETROVIRUSES ,SMALL interfering RNA ,TRANSGENIC animals ,TRANSPLANTATION of organs, tissues, etc. ,FIBROBLASTS ,NUCLEIC acid hybridization ,REVERSE transcriptase ,POLYMERASE chain reaction - Abstract
Background: Xenotransplantation using porcine cells, tissues or organs may be associated with the transmission of porcine endogenous retroviruses (PERVs). More than 50 viral copies have been identified in the pig genome and three different subtypes of PERV were released from pig cells, two of them were able to infect human cells in vitro. RNA interference is a promising option to inhibit PERV transmission. Methods: We recently selected an efficient si (small interfering) RNA corresponding to a highly conserved region in the PERV DNA, which is able to inhibit expression of all PERV subtypes in PERV-infected human cells as well as in primary pig cells. Pig fibroblasts were transfected using a lentiviral vector expressing a corresponding sh (short hairpin) RNA and transgenic pigs were produced by somatic nuclear transfer cloning. Integration of the vector was proven by PCR, expression of shRNA and PERV was studied by in-solution hybridization analysis and real-time RT PCR, respectively. Results: All seven born piglets had integrated the transgene. Expression of the shRNA was found in all tissues investigated and PERV expression was significantly inhibited when compared with wild-type control animals. Conclusion: This strategy may lead to animals compatible with PERV safe xenotransplantation. [ABSTRACT FROM AUTHOR]
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- 2008
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9. International Symposium on Xenotransplantation.
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Denner, Joachim, Niemann, Heiner, Reichart, Bruno, Schmoeckel, Michael, Schwinzer, Reinhard, and Tönjes, Ralf
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TRANSPLANTATION of organs, tissues, etc. , *CONFERENCES & conventions , *TRANSGENIC animals , *IMMUNOLOGY , *VIROLOGY ,ABSTRACTS - Abstract
The article presents the program and abstracts featured at the 9th Minisymposium on Xenotransplantation of the German working Group on Xenotransplantation held at Robert Kock Institute in Berlin, Germany on June 8-9, 2006. They include generation and characteristics of multi-transgenic pigs, immunologic aspects, virological aspects, islet cell and hepatocyte xenotransplantation and stem cell research.
- Published
- 2006
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10. Health status of transgenic pigs expressing the human complement regulatory protein CD59.
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Deppenmeier, Stefanie, Bock, Oliver, Mengel, Michael, Niemann, Heiner, Kues, Wilfried, Lemme, Erika, Wirth, Dagmar, Wonigeit, Kurt, and Kreipe, Hans
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LABORATORY swine ,TRANSGENIC animals ,PHENOTYPES ,DNA ,ANIMAL genetic engineering ,IMMUNOHISTOCHEMISTRY ,EDUCATION - Abstract
Background: Microinjection of foreign DNA into pronuclei of zygotes has been the method of choice for the production of transgenic domestic animals. Following microinjection the transgene is randomly integrated into the host genome which can be associated with insertional mutagenesis and unwanted pathological side effects. Methods: Here, we evaluated the health status of pigs transgenic for the human regulator of complement activation (RCA) CD59 and conducted a complete pathomorphological examination on 19 RCA transgenic pigs at 1 to 32 months of age from nine transgenic lines. Nine wild-type animals served as controls. Expression levels of human complement regulator CD59 (hCD59) mRNA were measured by RT-PCR and distribution of hCD59 protein was determined by immunohistochemistry. Results: Albeit variable transgene expression levels, no specific pathomorphologic phenotype associated with the presence of the transgene in all analyzed pig lines could be detected. Conclusions: Transgenic expression of this human RCA gene construct is not correlated with a specific pathological phenotype in pigs. This is crucial for the application of the technology and the use of transgenic pigs for biomedical and agricultural applications. [ABSTRACT FROM AUTHOR]
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- 2006
- Full Text
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11. Epigenetic silencing and tissue independent expression of a novel tetracycline inducible system in double-transgenic pigs.
- Author
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Kues, Wilfried A., Schwinzer, Reinhard, Wirth, Dagmar, Verhoeyen, Els, Lemme, Erika, Herrmann, Doris, Barg-Kues, Brigitte, Hauser, Hansjörg, Wonigeit, Kurt, and Niemann, Heiner
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TRANSGENIC animals ,CELL lines ,TETRACYCLINES ,GENE expression ,MEDICAL research - Abstract
Discusses research which aimed to demonstrate that single-construct tetracycline-responsive bicistronic expression cassettes can be successfully expressed in animals and to improve xenotransplantation by producing tet-off regulated human complement regulator transgenic animals. Functionality of autoregulatory regulator of complement activation-nitrilotriacetate (RCA-NTA) regulator expression cassettes in cell lines; Characteristic expression pattern in RCA-NTA transgenic pigs; Enhanced tissue-independent expression of CD59 in crossbred animals carrying two NTA-RCA cassettes.
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- 2006
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12. Recent progress in the production of transgenic pigs.
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Niemann, Heiner, Petersen, Björn, Kues, Wilfried, and Carnwath, Joseph W.
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TRANSGENIC animals , *SWINE ,ABSTRACTS - Abstract
An abstract of the article "Recent progress in the production of transgenic pigs," by Heiner Niemann and colleagues is presented.
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- 2012
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13. Transgenic pigs with reduced PERV expression by RNA interference.
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Semaan, Marwan, Kaulitz, Danny, Petersen, Björn, Kues, Wilfried A., Niemann, Heiner, and Denner, Joachim
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ABSTRACTS ,RNA interference ,TRANSGENIC animals - Abstract
An abstract of the article "Transgenic pigs with reduced PERV expression by RNA Interference," by Marwan Semaan and colleagues is presented.
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- 2012
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14. The perspectives for porcine-to-human xenografts
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Petersen, Bjoern, Carnwath, Joseph W., and Niemann, Heiner
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XENOGRAFTS , *TRANSPLANTATION of organs, tissues, etc. , *SWINE , *ANIMAL genetics , *TRANSGENIC animals , *GENOMES , *SOMATIC cells , *TRANSPLANTATION of cell nuclei - Abstract
Abstract: The shortage of donated human organs for transplantation continues to be a life threatening problem for patients suffering from complete organ failure. Although this gap is increasing due to the demographic changes in aging Western populations, it is generally accepted that international trading in human organ is not an ethical solution. Alternatives to the use of human organs for transplantation must be developed and these alternatives include stem cell therapy, artificial organs and organs from other species, i.e. xenografts. For practical reasons but most importantly because of its physiological similarity with humans, the pig is generally accepted as the species of choice for xenotransplantation. Nevertheless, before porcine organs can be used in human xenotransplantation, it is necessary to make a series of precise genetic modifications to the porcine genome, including the addition of genes for factors which suppress the rejection of transplanted porcine tissues and the inactivation or removal of undesirable genes which can only be accomplished at this time by targeted recombination and somatic nuclear transfer. This review will give an insight into the advances in transgenic manipulation and cloning in pigs—in the context of porcine-to-human xenotransplantation. [Copyright &y& Elsevier]
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- 2009
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15. DNA Nucleases and their Use in Livestock Production
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Petersen, Bjoern, Niemann, Heiner, editor, and Wrenzycki, Christine, editor
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- 2018
- Full Text
- View/download PDF
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