Your search keyword '"P M Kooiman"' showing total 8 results

1. [Untitled]

Author

Monique Rijnkels, Jan H. Nuijens, P M Kooiman, de Boer Ha, van Dixhoorn M, Frank Pieper, and Gerard Platenburg

Subjects

Genetically modified mouse, Ratón, Transgene, Biology, Molecular biology, law.invention, law, Casein, Gene expression, Genetics, Recombinant DNA, Cosmid, Animal Science and Zoology, Agronomy and Crop Science, Gene, Biotechnology

Abstract

The bovine αs1-casein gene, isolated from a cosmid library, was introduced into the murine germline. Transgene expression occurred in all transgenic mice, and was confined to the lactating mammary gland. Half of the mouse lines (five out of ten) expressed at relatively high expression levels (>1 mg ml−1). The highest levels of expression were obtained with a transgene containing 14.2 kb of 5′ flanking sequence, in two cases expression levels comparable to (10 mg ml−1) or well above (20 mg ml−1) αs1-casein levels in bovine milk were obtained. Transcription initiation occurred at the same site in the bovine αs1-casein gene in transgenic mouse as in the cow. A marked induction of expression occurred at parturition rather than at mid-pregnancy, and thus resembled the bovine rather than the murine developmental expression pattern. Bovine αs1-casein specific immunoblotting and RIA were developed for characterization and quantificatio n of the recombinant protein. Using these assays, the properties of the recombinant protein could not be distinguished from those of the natural bovine protein. In spite of the high-level tissue-specific and correctly regulated developmental expression of the transgene, expression levels were integration-site dependent. This may indicate that not all cis-acting regulatory elements involved in bovine αs1-casein expression were included in the transgene

Published

1997

2. Expression analysis of the individual bovine β-,αs2- and κ-casein genes in transgenic mice

Author

P M Kooiman, F R Pieper, Monique Rijnkels, Paul J.A. Krimpenfort, and H. A. De Boer

Subjects

Genetically modified mouse, Casein, Transgene, Clone (cell biology), Cosmid, RNA, Cell Biology, Transfection, Biology, Molecular Biology, Biochemistry, Gene, Molecular biology

Abstract

To identify cis-acting regulatory elements involved in the regulation of expression of the casein genes, the bovine beta-, alpha s2- and kappa-casein genes were isolated from cosmid libraries and introduced into the murine germline. Bovine casein expression was analysed at the RNA and protein level. The bovine beta-casein gene, including 16 kb of 5′- and 8 kb of 3′-flanking region, appeared to be expressed in all 12 transgenic mouse lines analysed. In 50% of these lines expression levels in milk exceeded 1 mg/ml. Three lines displayed expression levels comparable with or well above (20 mg/ml) the beta-casein levels in bovine milk. Transgene expression was restricted to the mammary gland. Strong induction of expression occurred at parturition and thus resembled the bovine rather than the murine pattern. In spite of this high-level tissue-specific and developmentally regulated expression, beta-casein expression levels were integration-site-dependent, suggesting that not all elements involved in regulation of expression were included in this beta-casein clone. Neither the bovine alpha s2- nor the kappa-casein gene, including 8 kb and 5 kb of 5′- and 1.5 kb and 19 kb of 3′-flanking sequences respectively, were properly expressed in transgenic mice. However, they were transcribed in stably transfected mouse mammary epithelial cells. This indicates that regulatory elements required for high-level, mammary gland-specific expression are not present in the alpha s2- and kappa-casein clones used in this study and are probably located elsewhere in the casein gene locus.

Published

1995

3. Efficient generation of functional transgenes by homologous recombination in murine zygotes

Author

Arjan C.J. Pronk, Rein Strijker, Frank Pieper, Jan H. Nuyens, Herman A. de Boer, De Wit Ineke, P M Kooiman, and Paul J.A. Krimpenfort

Subjects

Zygote, Transgene, Blotting, Western, Molecular Sequence Data, DNA, Recombinant, Radioimmunoassay, Gene Expression, Mice, Transgenic, Biology, Polymerase Chain Reaction, law.invention, Mice, chemistry.chemical_compound, law, Gene expression, Genetics, Animals, Humans, Gene, Serum Albumin, Recombination, Genetic, Base Sequence, DNA, Blotting, Northern, Molecular biology, body regions, Blot, Blotting, Southern, genomic DNA, Genetic Techniques, chemistry, embryonic structures, Recombinant DNA, Homologous recombination

Abstract

To assess the feasibility of generating functional transgenes directly via homologous recombination between microinjected DNA fragments, three overlapping genomic DNA fragments, together constituting the human serum albumin (hSA) gene, were coinjected into murine zygotes. The resulting transgenic mice were analyzed for structure and expression of the transgene. All transgenic mice carried recombined hSA DNA fragments and 74% contained a reconstituted hSA gene. HSA expression could be detected in liver and serum in most (72%) of these animals. Only correctly sized hSA transcripts were observed. Transgenic hSA could not be distinguished from the human serum-derived protein by radioimmunoassay or Western blotting. The high frequency and accuracy of homologous recombination in murine zygotes reported here allows the efficient generation of relatively large transgenes.

Published

1992

4. High-level expression of bovine alpha s1-casein in milk of transgenic mice

Author

M, Rijnkels, P M, Kooiman, G J, Platenburg, M, van Dixhoorn, J H, Nuijens, H A, de Boer, and F R, Pieper

Subjects

Transcription, Genetic, Blotting, Western, Immunoblotting, Radioimmunoassay, Caseins, Gene Expression, Mice, Transgenic, Blotting, Northern, Cosmids, Blotting, Southern, Mice, Mammary Glands, Animal, Milk, Pregnancy, Animals, Cattle, Female, Transgenes

Abstract

The bovine alpha s1-casein gene, isolated from a cosmid library, was introduced into the murine germline. Transgene expression occurred in all transgenic mice, and was confined to the lactating mammary gland. Half of the mouse lines (five out of ten) expressed at relatively high expression levels (1 mg ml-1). The highest levels of expression were obtained with a transgene containing 14.2 kb of 5' flanking sequence, in two cases expression levels comparable to (10 mg ml-1) or well above (20 mg ml-1) alpha s1-casein levels in bovine milk were obtained. Transcription initiation occurred at the same site in the bovine alpha s1-casein gene in transgenic mouse as in the cow. A marked induction of expression occurred at parturition rather than at mid-pregnancy, and thus resembled the bovine rather than the murine developmental expression pattern. Bovine alpha s1-casein specific immunoblotting and RIA were developed for characterization and quantification of the recombinant protein. Using these assays, the properties of the recombinant protein could not be distinguished from those of the natural bovine protein. In spite of the high-level tissue-specific and correctly regulated developmental expression of the transgene, expression levels were integration-site dependent. This may indicate that not all cis-acting regulatory elements involved in bovine alpha s1-casein expression were included in the transgene.

Published

1998

5. Organization of the bovine casein gene locus

Author

Frank Pieper, Monique Rijnkels, P M Kooiman, and H. A. De Boer

Subjects

Genetics, Cell culture, Bovine casein, Animals, Caseins, Chromosome Mapping, Cattle, Biology, Human genetics, Cell Line, Electrophoresis, Gel, Pulsed-Field

Published

1997

6. Glycosylated and unglycosylated human lactoferrins both bind iron and show identical affinities towards human lysozyme and bacterial lipopolysaccharide, but differ in their susceptibilities towards tryptic proteolysis

Author

H. A. Van Veen, H. A. De Boer, Johannes Henricus Nuijens, Frank Pieper, P. H. C. Van Berkel, P M Kooiman, and Marlieke E.J Geerts

Subjects

Lipopolysaccharides, Glycosylation, Proteolysis, Iron, Molecular Sequence Data, Anti-Inflammatory Agents, Radioimmunoassay, Biology, Kidney, Biochemistry, law.invention, Cell Line, chemistry.chemical_compound, law, medicine, Humans, Trypsin, Amino Acid Sequence, Molecular Biology, medicine.diagnostic_test, Lactoferrin, Tunicamycin, Kidney metabolism, Cell Biology, Chromatography, Agarose, Recombinant Proteins, carbohydrates (lipids), chemistry, Recombinant DNA, biology.protein, Muramidase, Lysozyme, medicine.drug, Protein Binding, Research Article

Abstract

We studied the role of N-glycosylation of human lactoferrin (hLF) with respect to properties that are relevant to its antibacterial and anti-inflammatory activities. A human kidney-derived 293(S) cell line that constitutively expresses recombinant hLF (rhLF) was produced. The reactivity towards various antibodies of rhLF that had been expressed in the absence or presence of tunicamycin (which blocks N-linked glycosylation) did not differ from that of natural (human milk-derived) hLF. Cation-exchange chromatography and N-terminal protein sequencing showed identical cationic properties and an intact N-terminal sequence for rhLF and natural hLF. SDS/PAGE of rhLF expressed in the presence of tunicamycin revealed a protein with the same M(r) as that of enzymically deglycosylated natural hLF. Both glycosylated and unglycosylated rhLF appeared to be completely saturated with iron. The affinity of natural hLF, glycosylated and non-glycosylated rhLF for both human lysozyme (Kd 4.5 x 10(-8) M) and bacterial lipopolysaccharide did not differ. SDS/PAGE of hLF species subjected to trypsin indicated that unglycosylated rhLF was much more susceptible to degradation. Furthermore, this analysis suggests that N-glycosylation heterogeneity in natural hLF and rhLF resides in the C-lobe. Thus our results provide no argument for differential antibacterial and/or anti-inflammatory activity of natural and (glycosylated) rhLF and suggest that a major function of glycosylation in hLF is to protect it against proteolysis.

Published

1995

7. Expression analysis of the individual bovine beta-, alpha s2- and kappa-casein genes in transgenic mice

Author

M, Rijnkels, P M, Kooiman, P J, Krimpenfort, H A, de Boer, and F R, Pieper

Subjects

Male, Caseins, Gene Expression, Mice, Transgenic, Mice, Mammary Glands, Animal, Milk, Gene Expression Regulation, Genes, Regulator, Animals, Lactation, RNA, Cattle, Female, Research Article

Abstract

To identify cis-acting regulatory elements involved in the regulation of expression of the casein genes, the bovine beta-, alpha s2- and kappa-casein genes were isolated from cosmid libraries and introduced into the murine germline. Bovine casein expression was analysed at the RNA and protein level. The bovine beta-casein gene, including 16 kb of 5'- and 8 kb of 3'-flanking region, appeared to be expressed in all 12 transgenic mouse lines analysed. In 50% of these lines expression levels in milk exceeded 1 mg/ml. Three lines displayed expression levels comparable with or well above (20 mg/ml) the beta-casein levels in bovine milk. Transgene expression was restricted to the mammary gland. Strong induction of expression occurred at parturition and thus resembled the bovine rather than the murine pattern. In spite of this high-level tissue-specific and developmentally regulated expression, beta-casein expression levels were integration-site-dependent, suggesting that not all elements involved in regulation of expression were included in this beta-casein clone. Neither the bovine alpha s2- nor the kappa-casein gene, including 8 kb and 5 kb of 5'- and 1.5 kb and 19 kb of 3'-flanking sequences respectively, were properly expressed in transgenic mice. However, they were transcribed in stably transfected mouse mammary epithelial cells. This indicates that regulatory elements required for high-level, mammary gland-specific expression are not present in the alpha s2- and kappa-casein clones used in this study and are probably located elsewhere in the casein gene locus.

Published

1995

8. Expression of human lactoferrin in milk of transgenic mice

Author

P M Kooiman, Shelley L. Woloshuk, Rein Strijker, Erika P. A. Kootwijk, Herman A. de Boer, Frank Pieper, Jan H. Nuijens, Paul Krimpenfort, and Gerard Platenburg

Subjects

Male, Recombinant Fusion Proteins, Genetic Vectors, Molecular Sequence Data, Mice, Transgenic, Regulatory Sequences, Nucleic Acid, Mice, Mammary Glands, Animal, Lactation, Gene expression, Genetics, medicine, Animals, Humans, Northern blot, RNA, Messenger, Gene, biology, Base Sequence, Lactoferrin, RNA, Caseins, Molecular biology, medicine.anatomical_structure, Milk, Gene Expression Regulation, Regulatory sequence, Polyclonal antibodies, Organ Specificity, biology.protein, Animal Science and Zoology, Cattle, Female, Agronomy and Crop Science, Biotechnology

Abstract

The expression of human lactoferrin (hLF) in the milk of transgenic mice is described. Regulatory sequences derived from the bovine alpha S1-casein gene were fused to the coding sequence of the hLF cDNA and several lines of transgenic mice were generated. Human LF RNA was detected exclusively in the mammary gland of lactating females and only after the onset of lactation. No aberrant RNA products could be detected using northern blotting and primer extension analysis. The hLF concentrations in the milk ranged from less than 0.1 to 36 micrograms ml-1. Human LF thus expressed did not differ from human milk derived LF, with respect to molecular mass and immunoreactivity with monoclonal and polyclonal antibodies.

Published

1994