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1. Ribosomal protein SA and its pseudogenes in ruminants: an extremely conserved gene family

Author

A. Van den Broeke, M. Van Poucke, A. Van Zeveren, and L.J. Peelman

Subjects
laminin receptor, mutation detection, prion, polymorphism, rpsa, sequence conservation, 37 kda laminin receptor precursor/67-kda laminin receptor, Animal culture, SF1-1100
Abstract

The ribosomal protein SA (RPSA), also known as 37-kDa laminin receptor precursor/67-kDa laminin receptor (LRP/LR), has been identified as a multifunctional protein, playing an important role in multiple pathologies like cancer and prion diseases. Since RPSA is involved in the binding and internalization of the prion protein, mutations in the ovine RPSA gene, influencing the RPSA-PrPC/PrPSc binding, can potentially play a part in the resistance to prion diseases. Our goal was to further characterize the complex RPSA gene family and to detect structural mutations which can play a role in this disease. In a prior study, 11 ovine pseudogenes were detected experimentally. As the whole genome shotgun ovine genome became accessible, an in silico genome-wide screening was performed and 37 new pseudogenes (36 processed and one semi-processed pseudogene) were detected, bringing the total to 48 ovine RPSA pseudogenes. Additionally, the complete bovine genome was screened in silico and 56 pseudogenes were identified. Once these sequences were known, it was possible to analyze the presence of mutations in the coding sequence and exon-flanking regions of the ovine functional full-length RPSA gene without the interference of pseudogenic sequences. Nineteen mutations were found: one in the 5' UTR, a silent one in the coding region, and seventeen in the exon-flanking regions, including an interesting mutation in the SNORA62 gene, localized in intron 4 of RPSA, leading to potential ribosomal defects. Structural mutations of the RPSA gene can be ruled out to play a role in transmissible spongiform encephalopathies but regulatory mutations still can have an effect on these diseases.

Published
2013
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2. Association analysis of PPARGC1A mutations with meat quality parameters in a commercial hybrid pig population

Author

T. Erkens, S. De Smet, K. Van den Maagdenberg, A. Stinckens, N. Buys, A. Van Zeveren, and L.J. Peelman

Subjects
association analysis, carcass composition, meat quality, pig, ppargc1a, snp, Animal culture, SF1-1100
Abstract

Peroxisome proliferator-activated receptor γ coactivator 1α (PPARGC1A) is a promising candidate gene for selection on meat and carcass quality traits in the pig industry. In the pig, several SNPs have been reported in both coding and regulatory regions of this gene, some of which were associated with fat characteristics, but none of these associations have been confirmed and many SNPs have not yet been evaluated. Therefore, 18 PPARGC1A SNPs were genotyped in 65 slaughter pigs of a commercial hybrid population and used in an association analysis with multiple muscle and carcass traits. Several SNPs located in the 3'UTR and exon 8 and 9 of PPARGC1A were significantly (P < 0.05-0.001) associated with various carcass composition, tenderness and muscle fibre traits. They could potentially serve as DNA selection markers, if their impact was to be confirmed by a functional analysis.

Published
2010
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3. SNP detection in the porcine PPARGC1A promoter region and 3'UTR, and an association analysis in a Landrace-Duroc-Yorkshire population

Author

T. Erkens, G.A. Rohrer, A. Van Zeveren, and L.J. Peelman

Subjects
association analysis, fat deposition, meat quality, pig, ppargc1a, promoter region, snp, 3'utr, Animal culture, SF1-1100
Abstract

Meat quality is of increasing economic importance to the pork industry today, which is in contrast with the more traditional focus of pig selection for lean growth. Meat quality is however determined by many factors with a complex mutual relationship. In this regard, PPARGC1A is a very interesting candidate gene because it not only plays a crucial role in energy and fat metabolism but also has an important influence on the muscle fibre type composition. However, only little is known about the regulation of expression of this gene in the pig and its usefulness in pig selection. In order to get a better understanding of the regulation of PPARGC1A expression, 1 898 base pairs (bp) from the promoter region and the complete 3'UTR (3 826 bp) were sequenced and screened for mutations in 7 diverse pig breeds. Respectively 5 and 6 new mutations were discovered in these regions, of which several were in complete linkage disequilibrium with each other. None of the detected SNPs appeared to be located in any conserved part of the sequence when comparing different species. In an association analysis with intramuscular fat percentage, leaf fat weight or last rib backfat depth carried out in a Landrace-Duroc-Yorkshire commercial research population (n = 960), no associations were detected for the new SNPs from this study or for 2 previously described SNPs in exon 8 and 9. The results from this study provide essential information on the sequence of the promoter region and 3'UTR of porcine PPARGC1A, necessary for unravelling the complex regulation of expression and functioning of this gene in the pig. Although no association with meat quality and fat deposition parameters was found for the newly discovered SNPs in the regulatory regions, these need to be used in future studies to (further) assess their usefulness as new selection criteria for improving meat quality while maintaining the leanness of the carcass.

Published
2009
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26. Characterization of the ovine ribosomal protein SA gene and its pseudogenes

Author

Van Zeveren Alex, Bertaud Maud, Hayes Hélène, Hugot Karine, Marcos-Carcavilla Ane, Van Poucke Mario, Van den Broeke Alice, and Peelman Luc J

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background The ribosomal protein SA (RPSA), previously named 37-kDa laminin receptor precursor/67-kDa laminin receptor (LRP/LR) is a multifunctional protein that plays a role in a number of pathological processes, such as cancer and prion diseases. In all investigated species, RPSA is a member of a multicopy gene family consisting of one full length functional gene and several pseudogenes. Therefore, for studies on RPSA related pathways/pathologies, it is important to characterize the whole family and to address the possible function of the other RPSA family members. The present work aims at deciphering the RPSA family in sheep. Results In addition to the full length functional ovine RPSA gene, 11 other members of this multicopy gene family, all processed pseudogenes, were identified. Comparison between the RPSA transcript and these pseudogenes shows a large variety in sequence identities ranging from 99% to 74%. Only one of the 11 pseudogenes, i.e. RPSAP7, shares the same open reading frame (ORF) of 295 amino acids with the RPSA gene, differing in only one amino acid. All members of the RPSA family were annotated by comparative mapping and fluorescence in situ hybridization (FISH) localization. Transcription was investigated in the cerebrum, cerebellum, spleen, muscle, lymph node, duodenum and blood, and transcripts were detected for 6 of the 11 pseudogenes in some of these tissues. Conclusions In the present work we have characterized the ovine RPSA family. Our results have revealed the existence of 11 ovine RPSA pseudogenes and provide new data on their structure and sequence. Such information will facilitate molecular studies of the functional RPSA gene taking into account the existence of these pseudogenes in the design of experiments. It remains to be investigated if the transcribed members are functional as regulatory non-coding RNA or as functional proteins.

Published
2010
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29. Molecular cloning and characterization of the porcine prostaglandin transporter (SLCO2A1): evaluation of its role in F4 mediated neonatal diarrhoea

Author

Cox Eric, Van Zeveren Alex, Erkens Tim, Melkebeek Vesna, Van Poucke Mario, and Peelman Luc J

Subjects
Genetics, QH426-470
Abstract

Abstract Background Because prostaglandins are involved in many (patho)physiological processes, SLCO2A1 was already characterized in several species in an attempt to unravel specific processes/deficiencies. Here, we describe the molecular cloning and characterization of the porcine ortholog in order to evaluate its possible involvement in F4 enterotoxigenic E. coli mediated neonatal diarrhoea, based on a positional candidate gene approach study. Results Porcine SLCO2A1 is organized in 14 exons, containing an open reading frame of 1935 bp, encoding a 12-transmembrane organic anion cell surface transporter of 644 aa. The -388 to -5 upstream region comprises a (CpG)48 island containing a number of conserved promoter elements, including a TATA box. A potential alternative promoter region was found in the conserved -973 to -700 upstream region. No consensus polyadenylation signal was discovered in the 3' UTR. Repeat sequences were found in 15% of all the non coding sequences. As expected for a multifunctional protein, a wide tissue distribution was observed. mRNA expression was found in the adrenal gland, bladder, caecum, colon (centripetal coil/centrifugal coil), diaphragm, duodenum, gallbladder, heart, ileum, jejunum, kidney, liver, longissimus dorsi muscle, lung, lymph node, mesenterium, rectum, spleen, stomach, tongue and ureter, but not in the aorta, oesophagus and pancreas. The promoter region and the exons (including the splice sites) of SLCO2A1 were resequenced in 5 F4ab/ac receptor positive and 5 F4ab/ac receptor negative pigs. Two silent and 2 missense (both S → L at position 360 and 633) mutations were found, but none was associated with the F4ab/ac receptor phenotype. In addition, no phenotype associated differential mRNA expression or alternative/abberant splicing/polyadenylation was found in the jejunum. Conclusion The molecular cloning and characterization of porcine SLCO2A1 not only contributes to the already existing knowledge about the transporter in general, but enables studies on porcine prostaglandin related processes/deficiencies as patient and/or model. Here we examined its possible involvement as receptor in F4 enterotoxigenic E. coli mediated neonatal diarrhoea. Because no phenotype associated differences could be found in the gene sequence nor in its jejunal transcription profile of F4ab/ac receptor positive/negative pigs, SLCO2A1 can most likely be excluded as receptor for F4 bacteria.

Published
2009
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31. Two new splice variants in porcine PPARGC1A

Author

Peelman Luc J, Van Zeveren Alex, Bilek Karel, and Erkens Tim

Subjects
Medicine, Biology (General), QH301-705.5, Science (General), Q1-390
Abstract

Abstract Background Peroxisome proliferator-activated receptor γ coactivator 1α (PPARGC1A) is a coactivator with a vital and central role in fat and energy metabolism. It is considered to be a candidate gene for meat quality in pigs and is involved in the development of obesity and diabetes in humans. How its many functions are regulated, is however still largely unclear. Therefore a transcription profile of PPARGC1A in 32 tissues and 4 embryonic developmental stages in the pig was constructed by screening its cDNA for possible splice variants with exon-spanning primers. Findings This led to the discovery of 2 new splice variants in the pig, which were subsequently also detected in human tissues. In these variants, exon 8 was either completely or partly (the last 66 bp were conserved) spliced out, potentially coding for a much shorter protein of respectively 337 and 359 amino acids (aa), of which the first 291 aa would be the same compared to the complete protein (796 aa). Conclusion Considering the functional domains of the PPARGC1A protein, it is very likely these splice variants considerably affect the function of the protein and alternative splicing could be one of the mechanisms by which the diverse functions of PPARGC1A are regulated.

Published
2008
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34. Characterization of the genomic region containing the Shadow of Prion Protein (SPRN) gene in sheep

Author

Van Zeveren Alex, Hayes Hélène, Hugot Karine, Van Poucke Mario, Lampo Evelyne, and Peelman Luc J

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background TSEs are a group of fatal neurodegenerative diseases occurring in man and animals. They are caused by prions, alternatively folded forms of the endogenous prion protein, encoded by PRNP. Since differences in the sequence of PRNP can not explain all variation in TSE susceptibility, there is growing interest in other genes that might have an influence on this susceptibility. One of these genes is SPRN, a gene coding for a protein showing remarkable similarities with the prion protein. Until now, SPRN has not been described in sheep, a highly relevant species in prion matters. Results In order to characterize the genomic region containing SPRN in sheep, a BAC mini-contig was built, covering approximately 200,000 bp and containing the genes ECHS1, PAOX, MTG1, SPRN, LOC619207, CYP2E1 and at least partially SYCE1. FISH mapping of the two most exterior BAC clones of the contig positioned this contig on Oari22q24. A fragment of 4,544 bp was also sequenced, covering the entire SPRN gene and 1206 bp of the promoter region. In addition, the transcription profile of SPRN in 21 tissues was determined by RT-PCR, showing high levels in cerebrum and cerebellum, and low levels in testis, lymph node, jejunum, ileum, colon and rectum. Conclusion Annotation of a mini-contig including SPRN suggests conserved linkage between Oari22q24 and Hsap10q26. The ovine SPRN sequence, described for the first time, shows a high level of homology with the bovine, and to a lesser extent with the human SPRN sequence. In addition, transcription profiling in sheep reveals main expression of SPRN in brain tissue, as in rat, cow, man and mouse.

Published
2007
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35. Development of a new set of reference genes for normalization of real-time RT-PCR data of porcine backfat and longissimus dorsi muscle, and evaluation with PPARGC1A

Author

Van Zeveren Alex, Goossens Karen, Vandesompele Jo, Van Poucke Mario, Erkens Tim, and Peelman Luc J

Subjects
Biotechnology, TP248.13-248.65
Abstract

Abstract Background An essential part of using real-time RT-PCR is that expression results have to be normalized before any conclusions can be drawn. This can be done by using one or multiple, validated reference genes, depending on the desired accuracy of the results. In the pig however, very little information is available on the expression stability of reference genes. The aim of this study was therefore to develop a new set of reference genes which can be used for normalization of mRNA expression data of genes expressed in porcine backfat and longissimus dorsi muscle, both representing an economically important part of a pig's carcass. Because of its multiple functions in fat metabolism and muscle fibre type composition, peroxisome proliferative activated receptor γ coactivator 1α (PPARGC1A) is a very interesting candidate gene for meat quality, and was an ideal gene to evaluate our developed set of reference genes for normalization of mRNA expression data of both tissue types. Results The mRNA expression stability of 10 reference genes was determined. The expression of RPL13A and SDHA appeared to be highly unstable. After normalization to the geometric mean of the three most stably expressed reference genes (ACTB, TBP and TOP2B), the results not only showed that the mRNA expression of PPARGC1A was significantly higher in each of the longissimus dorsi muscle samples than in backfat (P < 0.05), but also that the expression was significantly higher in the most cranial of the three muscle samples (P < 0.05). Conclusion This study provides a new set of reference genes (ACTB, TBP and TOP2B) suitable for normalization of real-time RT-PCR data of backfat and longissimus dorsi muscle in the pig. The obtained PPARGC1A expression results, after application of this set of reference genes, are a first step in unravelling the PPARGC1A expression pattern in the pig and provide a basis for possible selection towards improved meat quality while maintaining a lean carcass.

Published
2006
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36. Comparative analysis of a BAC contig of porcine chromosome 13q31-q32 and human chromosome 3q21-q22

Author

Van Zeveren Alex, Mattheeuws Marc, Piumi François, Bourry David, Van Poucke Mario, Chardon Patrick, and Peelman Luc J

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background The gene(s) encoding the ETEC F4ab/ac receptors, involved in neonatal diarrhoea in pigs (a disease not yet described in humans), is located close to the TF locus on Sscr13. In order to reveal and characterize possible candidate genes encoding these receptors, a porcine physical map of the TF region is indispensable. Results A contig of 33 BAC clones, covering approximately 1.35 Mb surrounding the TF locus on Sscr13q31-q32, was built by chromosome walking. A total of 22,552 bp from the BAC contig were sequenced and compared with database sequences to identify genes, ESTs and repeat sequences, and to anchor the contig to the syntenic region of the human genome sequence (Hsap3q21-q22). The contig was further annotated based on this human/porcine comparative map, and was also anchored to the Sanger porcine framework map and the integrated map of Sscr13 by RH mapping. Conclusion The annotated contig, containing 10 genes and 2 ESTs, showed a complete conservation of linkage (gene order and orientation) with the human genome sequence, based on 46 anchor points. This underlines the importance of the human/porcine comparative map for the identification of porcine genes associated with genetic defects and economically important traits, and for assembly of the porcine genome sequence.

Published
2005
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37. A dual fluorescent multiprobe assay for prion protein genotyping in sheep

Author

Van Zeveren Alex, Mattheeuws Marc, Vandesompele Jo, Van Poucke Mario, and Peelman Luc J

Subjects
Infectious and parasitic diseases, RC109-216
Abstract

Abstract Background Scrapie and BSE belong to a group of fatal, transmissible, neurodegenerative diseases called TSE. In order to minimize the risk of natural scrapie and presumed natural BSE in sheep, breeding programmes towards TSE resistance are conducted in many countries based on resistance rendering PRNP polymorphisms at codons 136 (A/V), 154 (R/H) and 171 (R/H/Q). Therefore, a reliable, fast and cost-effective method for routine PRNP genotyping in sheep, applicable in standard equipped molecular genetic laboratories, will be a vital instrument to fulfill the need of genotyping hundreds or thousands of sheep. Methods A dual fluorescent multiprobe assay consisting of 2 closed tube PCR reactions containing respectively 4 and 3 dual-labelled fluorescent ASO probes for the detection in real-time of the 7 allelic variants of sheep PRNP mentioned above. Results The assay is succesfully performed using unpurified DNA as a template for PCR, without any post-PCR manipulations and with semi-automatic determination of the PRNP genotypes. The performance of the assay was confirmed via PCR-RFLP and sequencing in a cross-validation study with 50 sheep. Conclusions We report the development and validation of a robust, reliable and reproducible method for PRNP genotyping of a few to many sheep samples in a fast, simple and cost-effective way, applicable in standard equipped molecular genetic laboratories. The described primer/probe design strategy can also be applied for the detection of other polymorphisms or disease causing mutations.

Published
2005
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40. Differential microRNA expression analysis in blastocysts by whole mount in situ hybridization and reverse transcription quantitative polymerase chain reaction on laser capture microdissection samples

Author

Luc Peelman, Ann Van Soom, Alex Van Zeveren, Karen Goossens, Pieter Cornillie, Ward De Spiegelaere, Christian Burvenich, Mieke Stevens, and Bart De Spiegeleer

Subjects
Biophysics, Laser Capture Microdissection, In situ hybridization, Biology, Biochemistry, microRNA, medicine, Animals, Inner cell mass, RNA, Messenger, Blastocyst, Molecular Biology, In Situ Hybridization, reproductive and urinary physiology, Laser capture microdissection, Reverse Transcriptase Polymerase Chain Reaction, Gene Expression Profiling, Cell Biology, Molecular biology, Embryonic stem cell, Reverse transcriptase, Cell biology, MicroRNAs, Real-time polymerase chain reaction, medicine.anatomical_structure, Gene Expression Regulation, embryonic structures, Cattle
Abstract

There is cumulating evidence that microRNAs (miRNAs) are important regulators of pluripotency and differentiation and, hence, of early lineage segregation in embryo development. To unravel the function of specific miRNAs, it is important not only to analyze miRNA expression in the entire blastocyst but also to determine the site and level of expression in the inner cell mass (ICM) versus trophectoderm (TE). A new strategy has been developed for miRNA expression analysis in ICM and TE using two complementary techniques. By whole mount in situ hybridization (WISH), it was visualized that bta-miR-155 is mainly expressed in the ICM. However, WISH does not provide quantitative data on expression differences between the two cell types. By reverse transcription quantitative polymerase chain reaction (RT–qPCR) on ICM and TE isolates taken from single blastocysts with laser capture microdissection (LCM), it was quantified that bta-miR-155 was 50-fold higher expressed in ICM than in TE. The possibility to quantify both miRNAs and messenger RNAs (mRNAs) in LCM samples offers the opportunity to analyze the expression of both miRNAs and potential targets in one sample. This article shows that a combination of WISH with LCM and subsequent RT–qPCR is a robust strategy to qualitatively and quantitatively analyze differential miRNA expression in discrete cell types of a single blastocyst.

Published
2012

41. [Letter to the editor]Combined FAM-labeled TaqMan probe detection and SYBR green I melting curve analysis in multiprobe qPCR genotyping assays

Author

Mario Van Poucke, Alex Van Zeveren, and Luc Peelman

Subjects
Genotyping Techniques, Diamines, Real-Time Polymerase Chain Reaction, General Biochemistry, Genetics and Molecular Biology, Melting curve analysis, chemistry.chemical_compound, TaqMan, Animals, Humans, Transition Temperature, Taq Polymerase, Benzothiazoles, Organic Chemicals, Gene, Genotyping, In Situ Hybridization, Fluorescent Dyes, Binding Sites, Chemistry, Organic chemicals, Molecular biology, Reverse transcription polymerase chain reaction, Real-time polymerase chain reaction, Quinolines, SYBR Green I, Biotechnology
Published
2012

42. Association analysis of PPARGC1A mutations with meat quality parameters in a commercial hybrid pig population

Author

K. Van den Maagdenberg, Anneleen Stinckens, A. Van Zeveren, Luc Peelman, Nadine Buys, Tim Erkens, and S. De Smet

Subjects
0301 basic medicine, Genetics, Candidate gene, education.field_of_study, Population, Single-nucleotide polymorphism, Biology, Tenderness, 03 medical and health sciences, Exon, 030104 developmental biology, medicine, Animal Science and Zoology, PPARGC1A, medicine.symptom, education, Gene, Genetic association
Abstract

Peroxisome proliferator-activated receptor gamma coactivator 1 alpha (PPARGC1A) is a promising candidate gene for selection on meat and carcass quality traits in the pig industry. In the pig, several SNPs have been reported in both coding and regulatory regions of this gene, some of which were associated with fat characteristics, but none of these associations have been confirmed and many SNPs have not yet been evaluated. Therefore, 18 PPARGC1A SNPs were genotyped in 65 slaughter pigs of a commercial hybrid population and used in an association analysis with multiple muscle and carcass traits. Several SNPs located in the 3'UTR and exon 8 and 9 of PPARGC1A were significantly (P < 0.05-0.001) associated with various carcass composition, tenderness and muscle fibre traits. They could potentially serve as DNA selection markers, if their impact was to be confirmed by a functional analysis.

Published
2010

43. Correlation between porcinePPARGC1A mRNA expression and its downstream target genes in backfat andlongissimus dorsi muscle

Author

Jo Vandesompele, A. Van Zeveren, Luc Peelman, and Tim Erkens

Subjects
Sus scrofa, Gene Expression, PDK4, Biology, Andrology, In vivo, Gene expression, Genetics, medicine, Animals, RNA, Messenger, Muscle, Skeletal, Gene, DNA Primers, Messenger RNA, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, Skeletal muscle, Lipid metabolism, General Medicine, Lipid Metabolism, medicine.anatomical_structure, Adipose Tissue, Biochemistry, PPARGC1A, Energy Metabolism, Transcription Factors
Abstract

Knowledge of in vivo relationship between the coactivator PPARGC1A and its target genes is very limited, especially in the pig. In this study, a real-time PCR experiment was performed on longissimus dorsi muscle (MLD) and backfat with 10 presumed PPARGC1A downstream target genes, involved in energy and fat metabolism, to identify possible relationships with PPARGC1A mRNA expression in vivo in the pig (n = 20). Except for UCP3 and LPL, a very significant difference in expression was found between MLD and backfat for all genes (P0.01). Hierarchical cluster analysis and the significant pairing of mRNA expression data between sampling locations suggested a genetic regulation of the expression of several target genes. A positive correlation with PPARGC1A was found for CPT1B, GLUT4, PDK4, and TFAM (P0.0001). A negative correlation was found for UCP2, FABP4, LEP (P0.0001), and TNF (P = 0.0071). No significant correlation was detected for UCP3 and LPL. This study provides evidence for a clear difference in mRNA expression of crucial genes in fat and energy metabolism between 2 important tissues. Our data suggest a clear impact of PPARGC1A on energy and lipid metabolism in vivo in the pig, through several of these downstream target genes.

Published
2009

44. Live weight assessment based on easily accessible morphometric characteristics in the double-muscled Belgian Blue beef breed

Author

Stefaan De Smet, Alex Van Zeveren, Hans Laevens, Luc Duchateau, and Frank Coopman

Subjects
Animal science, General Veterinary, Shoulders, Belgian Blue, Withers, Coefficient of variation, Linear regression, Linear model, Animal Science and Zoology, Biology, Breed, Girth (geometry)
Abstract

Live weight is an important trait in cattle farming. Weighing is not always feasible and therefore live weight is often estimated from easily accessible data. In this study, data on live weight, age and gender, and four body measurements, withers height (WH), heart girth (HG) and width of the shoulders (SW) and hind quarters (BcW) of double-muscled Belgian Blue beef (DM-BBB) farm animals were used to develop multivariable non-linear and linear regression models that predict live weight from these easily accessible data. The relationship between the logarithm of the live weight and the logarithm of time is adequately described by a general logistic function. The age period from 100 to 600 days of age is contained in the linear part of the logistic function. This region is of particular economic interest because it contains the yearling age and slaughter age that are important in DM-BBB breeding and management. Adding one of the body traits in the linear models that contain age and gender as fixed effects decreases the coefficient of variation. A model with withers height and shoulder width has the lowest coefficient of variation, with no further significant improvement when adding either heart girth or width of the hind quarters.

Published
2009

45. SNP detection in the porcine PPARGC1A promoter region and 3'UTR, and an association analysis in a Landrace-Duroc-Yorkshire population

Author

Gary A. Rohrer, Tim Erkens, Luc Peelman, and A. Van Zeveren

Subjects
0301 basic medicine, Genetics, Candidate gene, education.field_of_study, Population, 0402 animal and dairy science, Single-nucleotide polymorphism, 04 agricultural and veterinary sciences, Biology, 040201 dairy & animal science, 03 medical and health sciences, 030104 developmental biology, Regulatory sequence, Animal Science and Zoology, PPARGC1A, Intramuscular fat, education, Gene, Genetic association
Abstract

Meat quality is of increasing economic importance to the pork industry today, which is in con - trast with the more traditional focus of pig selection for lean growth. Meat quality is however determined by many factors with a complex mutual relationship. In this regard, PPARGC1A is a very interesting candidate gene because it not only plays a crucial role in energy and fat metabolism but also has an important influence on the muscle fibre type composition. However, only little is known about the regulation of expression of this gene in the pig and its usefulness in pig selection. In order to get a better understanding of the regu - lation of PPARGC1A expression, 1 898 base pairs (bp) from the promoter region and the complete 3'UTR (3 826 bp) were sequenced and screened for mutations in 7 diverse pig breeds. Respectively 5 and 6 new mutations were discovered in these regions, of which several were in complete linkage disequilibrium with each other. None of the detected SNPs appeared to be located in any conserved part of the sequence when comparing different species. In an association analysis with intramuscular fat percentage, leaf fat weight or last rib backfat depth carried out in a Landrace-Duroc-Yorkshire commercial research population ( n = 960), no associations were detected for the new SNPs from this study or for 2 previously described SNPs in exon 8 and 9. The results from this study provide essential information on the sequence of the promoter region and 3'UTR of porcine PPARGC1A, necessary for unravelling the complex regulation of expression and fun - ctioning of this gene in the pig. Although no association with meat quality and fat deposition parameters was found for the newly discovered SNPs in the regulatory regions, these need to be used in future studies to (further) assess their usefulness as new selection criteria for improving meat quality while maintaining the leanness of the carcass.

Published
2009

46. The position of the epistatic S locus in the halothane linkage group in pigs

Author

H. Varewyck, Alex Van Zeveren, A. Weghe, and Yves Bouquet

Subjects
Male, S system, Heterozygote, Genotype, Genetic Linkage, Swine, Belgian Landrace, Alpha-Globulins, medicine, Animals, Alleles, Crosses, Genetic, Serum Albumin, Linkage (software), Genetics, biology, Phosphogluconate Dehydrogenase, Strain (biology), Glucose-6-Phosphate Isomerase, General Medicine, respiratory system, biology.organism_classification, Blood Group Antigens, Epistasis, Female, Halothane, Gene sequence, Recombination, medicine.drug
Abstract

Summary The linkage of the Phi, Pgd, Po2, S, H and halothane sensitivity loci was followed in a Belgian Landrace family, heterozygous for these systems over 6 generations. Recombination next to the S locus occurred mainly in pigs belonging to this particular family. From this investigation the position of the S locus is proved to be outwith the Phi-Pgd region, next to Phi. Therefore the gene sequence S - Phi - Hal -H- Po2 -Pgd is proposed. Higher recombination rates were observed in the female parental line of the multiheterozygous family when compared to the male parental line. Additional data from animals, unrelated to this strain, confirm the evidence of close linkage of the S system to the nearest marker loci.

Published
2009

47. Evolutionary conservation of the linkage between the structural loci for serum albumin and vitamin D binding protein (Gc) in cattle

Author

H. Varewyck, A. Van De Weghe, Yves Bouquet, and A. Van Zeveren

Subjects
Male, Linkage disequilibrium, Genotype, Genetic Linkage, Vitamin D-binding protein, Population, Serum albumin, Biology, Gene Frequency, Molecular evolution, Genetic linkage, Genetics, Animals, education, Serum Albumin, education.field_of_study, Vitamin D-Binding Protein, Haplotype, General Medicine, Biological Evolution, Phenotype, Belgian Blue, biology.protein, Cattle, Animal Science and Zoology
Abstract

Evidence is presented for close genetic linkage between the structural loci for serum albumin and the vitamin D binding protein (Gc) in Belgian Blue and White cattle. Five recombinants were observed in a total of 342 informative offspring. The recombination frequency between the two loci was estimated as 1.5% +/- 0.9. The observed distribution of the haplotypes deviated from the expected one in the population, probably due to selection and significant linkage disequilibrium.

Published
2009

48. Polymorphic CAC/T repetitive sequences in the pig genome 1

Author

Anna Depicker, Luc Peelman, Alex Van Zeveren, Alex Van De Weghe, Jeroen Coppieters, Yves Bouquet, and Wouter Coppieters

Subjects
Swine, Molecular Sequence Data, Biology, Polymerase Chain Reaction, DNA sequencing, Genetics, Animals, Genomic library, Cloning, Molecular, Gene Library, Repetitive Sequences, Nucleic Acid, Southern blot, Genome, Polymorphism, Genetic, Base Sequence, Hybridization probe, Nucleic acid sequence, General Medicine, DNA Fingerprinting, Molecular biology, Mutagenesis, Insertional, Minisatellite, DNA profiling, DNA Transposable Elements, Microsatellite, Animal Science and Zoology, DNA Probes
Abstract

Three genomic clones were isolated from a size-selected pig DNA library by hybridization with a DNA-fingerprint probe. Analysis at the sequence level revealed that all three clones contain interrupted stretches of triplet repeats mainly composed of CAC and CAT triplets. Evaluation of the corresponding loci for polymorphism by Southern blot hybridization showed considerable length variation. For two loci the polymorphism was also demonstrated by polymerase chain reaction (PCR) amplification. The PiGMaP reference pedigree was typed for all three loci.

Published
2009

49. Phenotype frequencies of vitamin D binding protein (Gc) and of posttransferrin-2 (Ptf-2) in Belgian cattle breeds*

Author

Yves Bouquet, Van Zeveren A, H. Varewyck, and Van de Weghe A

Subjects
Genetics, Vitamin D-binding protein, Vitamin D-Binding Protein, Transferrin, Genetic Variation, Posttransferrin, General Medicine, Biology, Phenotype, Molecular biology, Breed, White (mutation), Gene Frequency, Species Specificity, Animals, Cattle, Electrophoresis, Polyacrylamide Gel, Allele, Carrier Proteins, Polyacrylamide gel electrophoresis, Allele frequency
Abstract

Summary The vitamin D binding protein (Gc) and posttransferrin-2 (Ptf-2) phenotypes have been determined in a number of Belgian cattle breeds. A very slow migrating variant of the Gc protein — Gc C — has been found in White and Red East Flemish breed. This variant was absent from the other breeds studied. This slow variant was identified as a vitamin D binding protein by autoradiography. The Gc C protein was shown to be controlled by a codominant autosomal allele Gc C at the Gclocus. The Gc C protein is probably identical with a fraction previously described in buffalo and an Italian cattle breed. The allele frequencies for the Gc and Pft-2 systems are reported for several Belgian breeds of cattle.

Published
2009

50. Antigenes lymphocytaires des chevaux dans quatre populations majeures belges

Author

G. Guérin, H. Varewyck, Yves Bouquet, A. Weghe, S. Lazary, Alex Van Zeveren, Unité de recherche Génétique Biochimique et Cytogénétique (LGBC), Institut National de la Recherche Agronomique (INRA), and ProdInra, Migration

Subjects
Isoantigens, [SDV]Life Sciences [q-bio], biology.animal_breed, Biology, IMMUNOLOGIE, Serology, 03 medical and health sciences, 0302 clinical medicine, Belgium, Gene Frequency, Species Specificity, Antigen, otorhinolaryngologic diseases, Animals, Horses, Lymphocytes, Allele, Allele frequency, Alleles, health care economics and organizations, 030304 developmental biology, Genetics, 0303 health sciences, Horse, General Medicine, Breed, Histocompatibility, [SDV] Life Sciences [q-bio], Belgian horse, 030215 immunology
Abstract

158 Belgian Saddlebreds, 130 Belgian Trotters, 108 Belgian Draft horses and 92 Shetland ponies have been typed for serologically defined antigens at the ELA and ELY systems. Gene frequencies were estimated in each breed for the internationally established ELA, ELY-1 and ELY-2 alleles as well as for locally assigned additional ELA markers and for subtypes of ELA-W3, W9 and W11. The distribution of ELA alleles was in agreement with the expected Hardy-Weinberg equilibrium for the 4 horse breeds described here. Differences in gene frequencies between these main Belgian horse populations were observed.

Published
2009

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