Your search keyword '"Blotting, Southern veterinary"' showing total 259 results

1. Detection of monoclonal integration of bovine leukemia virus proviral DNA as a malignant marker in two enzootic bovine leukosis cases with difficult clinical diagnosis.

Author

Miura S, Horiuchi N, Matsumoto K, Kobayashi Y, Kawazu S, and Inokuma H

Subjects

Animals, Biomarkers, Tumor blood, Blotting, Southern veterinary, Cattle, DNA, Viral blood, DNA, Viral genetics, Enzootic Bovine Leukosis virology, Female, Proviruses genetics, Virus Integration, Enzootic Bovine Leukosis diagnosis, Leukemia Virus, Bovine genetics

Abstract

Monoclonal integration of bovine leukemia virus (BLV) proviral DNA into bovine genomes was detected in peripheral blood from two clinical cases of enzootic bovine leukosis (EBL) without enlargement of superficial lymph nodes. A BLV-specific probe hybridized with 1 to 3 EcoRI and HindIII fragments in these 2 atypical EBL cattle by Southern blotting and hybridization, as well as in 3 typical EBL cattle. The probe also hybridized to a large number of EcoRI and HindIII fragments in 5 cattle with persistent leukosis. These results suggest that the detection of monoclonal integration of BLV provirus into the host genome may serve as a marker of monoclonal proliferation and malignancy in difficult to diagnose EBL cattle.

Published

2015

2. Ornamental fish as a source of plasmid-mediated quinolone resistance genes and antibiotic resistance plasmids.

Author

Dobiasova H, Kutilova I, Piackova V, Vesely T, Cizek A, and Dolejska M

Subjects

Animals, Anti-Bacterial Agents pharmacology, Aquaculture, Base Sequence, Blotting, Southern veterinary, Ciprofloxacin pharmacology, Czech Republic, DNA Primers genetics, Gram-Negative Bacterial Infections genetics, Humans, Microbial Sensitivity Tests veterinary, Molecular Sequence Data, Plasmids genetics, Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Aeromonas genetics, Carps microbiology, Drug Resistance, Bacterial genetics, Fish Diseases microbiology, Gram-Negative Bacterial Infections veterinary

Abstract

Growing ornamental fish industry is associated with public health concerns including extensive antibiotic use accompanied by increasing antibiotic resistance. The aim of this study was to analyze Aeromonas isolates from imported tropical ornamental fish and coldwater koi carps bred in the Czech Republic to assess the potential risk of ornamental fish as a source of plasmid-mediated quinolone resistance genes (PMQR) and antibiotic resistance plasmids. A collection of Aeromonas spp. with reduced susceptibility to ciprofloxacin (MIC ≥ 0.05 mg/L) was selected for the detection of PMQR genes. Isolates harbouring PMQR genes were further analyzed for the additional antibiotic resistance, integron content, clonality, biofilm production and transferability of PMQR genes by conjugation and transformation. Comparative analysis of plasmids carrying PMQR genes was performed. Fifteen (19%, n=80) isolates from koi carps and 18 (24%, n=76) isolates from imported ornamental fish were positive for qnrS2, aac(6')-Ib-cr or qnrB17 genes. PMQR-positive isolates from imported ornamental fish showed higher MIC levels to quinolones, multiresistance and diverse content of antibiotic resistance genes and integrons compared to the isolates from the carps. Related IncU plasmids harbouring qnrS2 and aac(6')-Ib-cr genes were found in Aeromonas spp. from imported ornamental fish and koi carps from various geographical areas. Ornamental fish may represent a potential source of multiresistant bacteria and mobile genetic elements for the environment and for humans., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published

2014

3. Identification and characterization of a Trypanosoma congolense 46 kDa protein as a candidate serodiagnostic antigen.

Author

Zhou M, Suganuma K, Ruttayaporn N, Nguyen TT, Yamasaki S, Igarashi I, Kawazu S, Suzuki Y, and Inoue N

Subjects

Animals, Blotting, Southern veterinary, Blotting, Western veterinary, Cattle, Enzyme-Linked Immunosorbent Assay veterinary, Escherichia coli, Glutathione Transferase metabolism, Microscopy, Confocal veterinary, Open Reading Frames, Serologic Tests methods, Trypanosomiasis, African diagnosis, Antigens, Protozoan genetics, Cattle Diseases diagnosis, Cattle Diseases parasitology, Serologic Tests veterinary, Trypanosoma congolense genetics, Trypanosomiasis, African veterinary

Abstract

Trypanosoma congolense is a major livestock pathogen in Africa, causing large economic losses with serious effects on animal health. Reliable serodiagnostic tests are therefore urgently needed to control T. congolense infection. In this study, we have identified one T. congolense protein as a new candidate serodiagnostic antigen. The 46.4 kDa protein (TcP46, Gene ID: TcIL3000.0.25950) is expressed 5.36 times higher in metacyclic forms than epimastigote forms. The complete nucleotide sequences of TcP46 contained an open reading frame of 1,218 bp. Southern blot analysis indicated that at least two copies of the TcP46 gene were tandemly-arranged in the T. congolense genome. The recombinant TcP46 (rTcP46) was expressed in Escherichia coli as a glutathione S-transferase (GST) fusion protein. Western blot analysis and confocal laser scanning microscopy revealed that the native TcP46 protein is expressed in the cytoplasm during all life-cycle stages of the parasite. Moreover, an enzyme-linked immunosorbent assay (ELISA) based on rTcP46 detected the specific antibodies as early as 8 days post-infection from mice experimentally infected with T. congolense. No cross-reactivity was observed in the rTcP46-based ELISA against serum samples from cattle experimentally infected with Babesia bigemina, B. bovis and Anaplasma marginale. These results suggest that rTcP46 could be used as a serodiagnostic antigen for T. congolense infection.

Published

2014

4. Generation of transgenic pigs by cytoplasmic injection of piggyBac transposase-based pmGENIE-3 plasmids.

Author

Li Z, Zeng F, Meng F, Xu Z, Zhang X, Huang X, Tang F, Gao W, Shi J, He X, Liu D, Wang C, Urschitz J, Moisyadi S, and Wu Z

Subjects

Animals, Animals, Genetically Modified, Animals, Newborn, Blotting, Southern veterinary, DNA chemistry, DNA genetics, Embryo Transfer veterinary, Female, Genetic Vectors administration & dosage, Genetic Vectors genetics, Male, Microinjections veterinary, Plasmids genetics, Polymerase Chain Reaction veterinary, Transposases administration & dosage, Zygote physiology, Gene Transfer Techniques veterinary, Plasmids administration & dosage, Swine genetics, Swine surgery, Transgenes, Transposases genetics

Abstract

The process of transgenesis involves the introduction of a foreign gene, the transgene, into the genome of an animal. Gene transfer by pronuclear microinjection (PNI) is the predominant method used to produce transgenic animals. However, this technique does not always result in germline transgenic offspring and has a low success rate for livestock. Alternate approaches, such as somatic cell nuclear transfer using transgenic fibroblasts, do not show an increase in efficiency compared to PNI, while viral-based transgenesis is hampered by issues regarding transgene size and biosafety considerations. We have recently described highly successful transgenesis experiments with mice using a piggyBac transposase-based vector, pmhyGENIE-3. This construct, a single and self-inactivating plasmid, contains all the transpositional elements necessary for successful gene transfer. In this series of experiments, our laboratories have implemented cytoplasmic injection (CTI) of pmGENIE-3 for transgene delivery into in vivo-fertilized pig zygotes. More than 8.00% of the injected embryos developed into transgenic animals containing monogenic and often single transgenes in their genome. However, the CTI technique was unsuccessful during the injection of in vitro-fertilized pig zygotes. In summary, here we have described a method that is not only easy to implement, but also demonstrated the highest efficiency rate for nonviral livestock transgenesis.

Published

2014

5. Perfrin, a novel bacteriocin associated with netB positive Clostridium perfringens strains from broilers with necrotic enteritis.

Author

Timbermont L, De Smet L, Van Nieuwerburgh F, Parreira VR, Van Driessche G, Haesebrouck F, Ducatelle R, Prescott J, Deforce D, Devreese B, and Van Immerseel F

Subjects

Amino Acid Sequence, Animals, Antimicrobial Cationic Peptides isolation & purification, Antimicrobial Cationic Peptides metabolism, Bacterial Toxins genetics, Bacterial Toxins metabolism, Bacteriocins isolation & purification, Bacteriocins metabolism, Base Sequence, Blotting, Southern veterinary, Clostridium Infections microbiology, Clostridium perfringens genetics, Electrophoresis, Gel, Pulsed-Field veterinary, Enteritis microbiology, Enteritis veterinary, Enterotoxins genetics, Enterotoxins metabolism, Molecular Sequence Data, Necrosis microbiology, Necrosis veterinary, Polymerase Chain Reaction veterinary, Sequence Homology, Antimicrobial Cationic Peptides genetics, Bacteriocins genetics, Chickens, Clostridium Infections veterinary, Clostridium perfringens physiology, Poultry Diseases microbiology

Abstract

Necrotic enteritis in broiler chickens is associated with netB positive Clostridium perfringens type A strains. It is known that C. perfringens strains isolated from outbreaks of necrotic enteritis are more capable of secreting factors inhibiting growth of other C. perfringens strains than strains isolated from the gut of healthy chickens. This characteristic could lead to extensive and selective presence of a strain that contains the genetic make-up enabling to secrete toxins that cause gut lesions. This report describes the discovery, purification, characterization and recombinant expression of a novel bacteriocin, referred to as perfrin, produced by a necrotic enteritis-associated netB-positive C. perfringens strain. Perfrin is a 11.5 kDa C-terminal fragment of a 22.9 kDa protein and showed no sequence homology to any currently known bacteriocin. The 11.5 kDa fragment can be cloned into Escherichia coli, and expression yielded an active peptide. PCR detection of the gene showed its presence in 10 netB-positive C. perfringens strains of broiler origin, and not in other C. perfringens strains tested (isolated from broilers, cattle, sheep, pigs, and humans). Perfrin and NetB are not located on the same genetic element since NetB is plasmid-encoded and perfrin is not. The bacteriocin has bactericidal activity over a wide pH-range but is thermolabile and sensitive to proteolytic digestion (trypsin, proteinase K). C. perfringens bacteriocins, such as perfrin, can be considered as an additional factor involved in the pathogenesis of necrotic enteritis in broilers.

Published

2014

6. Genomic organization and functional diversification of two warm-temperature-acclimation-associated 65-kDa protein genes in rockbream (Oplegnathus fasciatus; Perciformes).

Author

Lee SY, Kim BS, Noh CH, and Nam YK

Subjects

Amino Acid Sequence, Analysis of Variance, Animals, Blotting, Southern veterinary, Cluster Analysis, Computational Biology, Hemopexin immunology, Humans, Liver metabolism, Molecular Sequence Data, Perciformes immunology, Protein Isoforms genetics, Real-Time Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Temperature, Acclimatization genetics, Gene Components genetics, Hemopexin genetics, Perciformes genetics

Abstract

Two paralogue genes of warm-temperature-acclimation-associated 65-kDa protein were characterized and their mRNA expression patterns during various experimental stimulations were examined in the rockbream (Oplegnathus fasciatus; Perciformes). Rockbream Wap65 isoforms (rbWap65-1 and rbWap65-2) share basically common structural features with other teleostean orthologues and human hemopexin (HPX) at both amino acid (conserved cysteine and histidine residues) and genomic levels (ten-exon structure), although the rbWap65-2 reveals more homologous characteristics to human HPX than does rbWap65-1 isoform. Southern blot analysis indicates that each rbWap65 isoform exists as a single copy gene in the rockbream genome. Both rbWap65 genes were predicted to possess various transcription factor (TF) binding motifs related with stress and innate immunity in their 5ʹ-upstream regions, in which inflammation-related motifs were more highlighted in the rbWap65-2 than in rbWap65-1. Based on the RT-PCR assay, the liver-predominant expression pattern was more apparent in rbWap65-1 than rbWap65-2 isoform. During thermal elevation, clear upregulation was found only for the rbWap65-1. In contrast, immune stimulations (bacterial challenges, viral infection and iron overload) activated more preferentially the rbWap65-2 isoform in overall, although the inducibility was affected by the kinds of stimulators and tissue types. Taken together, our data suggest that the two paralogue rbWap65 isoforms have experienced subfunctionalization and/or neofunctionalization during their evolutionary history, in which the rbWap65-2 has retained closer, functional orthology to the human HPX while the rbWap65-1 have been diversified to be more related with thermal acclimation physiology., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published

2014

7. Transposon mutagenesis in Mycoplasma hyopneumoniae using a novel mariner-based system for generating random mutations.

Author

Maglennon GA, Cook BS, Deeney AS, Bossé JT, Peters SE, Langford PR, Maskell DJ, Tucker AW, Wren BW, and Rycroft AN

Subjects

Animals, Blotting, Southern veterinary, Mycoplasma hyopneumoniae metabolism, Pneumonia of Swine, Mycoplasmal microbiology, Polymerase Chain Reaction veterinary, Swine, Swine Diseases microbiology, DNA Transposable Elements, Mutagenesis, Mycoplasma hyopneumoniae genetics

Abstract

Mycoplasma hyopneumoniae is the cause of enzootic pneumonia in pigs, a chronic respiratory disease associated with significant economic losses to swine producers worldwide. The molecular pathogenesis of infection is poorly understood due to the lack of genetic tools to allow manipulation of the organism and more generally for the Mycoplasma genus. The objective of this study was to develop a system for generating random transposon insertion mutants in M. hyopneumoniae that could prove a powerful tool in enabling the pathogenesis of infection to be unraveled. A novel delivery vector was constructed containing a hyperactive C9 mutant of the Himar1 transposase along with a mini transposon containing the tetracycline resistance cassette, tetM. M. hyopneumoniae strain 232 was electroporated with the construct and tetM-expressing transformants selected on agar containing tetracycline. Individual transformants contained single transposon insertions that were stable upon serial passages in broth medium. The insertion sites of 44 individual transformants were determined and confirmed disruption of several M. hyopneumoniae genes. A large pool of over 10 000 mutants was generated that should allow saturation of the M. hyopneumoniae strain 232 genome. This is the first time that transposon mutagenesis has been demonstrated in this important pathogen and could be generally applied for other Mycoplasma species that are intractable to genetic manipulation. The ability to generate random mutant libraries is a powerful tool in the further study of the pathogenesis of this important swine pathogen.

Published

2013

8. Deletion of the GI-2 integrase and the wbkA flanking transposase improves the stability of Brucella melitensis Rev 1 vaccine.

Author

Mancilla M, Grilló MJ, de Miguel MJ, López-Goñi I, San-Román B, Zabalza-Baranguá A, and Moriyón I

Subjects

Animals, Bacterial Proteins metabolism, Bacterial Vaccines immunology, Blotting, Southern veterinary, Brucella melitensis cytology, Brucella melitensis enzymology, Brucellosis microbiology, Brucellosis therapy, Chromosomes, Bacterial, Female, Gene Deletion, Genomic Islands, Glycosyltransferases genetics, Glycosyltransferases metabolism, Integrases genetics, Integrases metabolism, Mice, Mice, Inbred BALB C, Mutagenesis, Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Bacterial Proteins genetics, Bacterial Vaccines genetics, Brucella melitensis genetics, Brucella melitensis immunology, Brucellosis veterinary, Gene Expression Regulation, Bacterial

Abstract

Brucella melitensis Rev 1 is the best vaccine available for the prophylaxis of small ruminant brucellosis and, indirectly, for reducing human brucellosis. However, Rev 1 shows anomalously high rates of spontaneous dissociation from smooth (S) to rough (R) bacteria, the latter being inefficacious as vaccines. This S-R instability results from the loss of the O-polysaccharide. To overcome this problem, we investigated whether some recently described mechanisms promoting mutations in O-polysaccharide genes were involved in Rev 1 S-R dissociation. We found that a proportion of Rev 1 R mutants result from genome rearrangements affecting the wbo O-polysaccharide loci of genomic island GI-2 and the wbkA O-polysaccharide glycosyltransferase gene of the wbk region. Accordingly, we mutated the GI-2 int gene and the wbk IS transposase involved in those arrangements, and found that these Rev 1 mutants maintained the S phenotype and showed lower dissociation levels. Combining these two mutations resulted in a strain (Rev 2) displaying a 95% decrease in dissociation with respect to parental Rev 1 under conditions promoting dissociation. Rev 2 did not differ from Rev 1 in the characteristics used in Rev 1 typing (growth rate, colonial size, reactivity with O-polysaccharide antibodies, phage, dye and antibiotic susceptibility). Moreover, Rev 2 and Rev 1 showed similar attenuation and afforded similar protection in the mouse model of brucellosis vaccines. We conclude that mutations targeting genes and DNA sequences involved in spontaneous O-polysaccharide loss enhance the stability of a critical vaccine phenotype and complement the empirical stabilization precautions taken during S Brucella vaccine production.

Published

2013

9. Two thioredoxin-superfamily members from sea bass (Dicentrarchus labrax, L.): characterization of PDI (PDIA1) and ERp57 (PDIA3).

Author

Pinto RD, Moreira AR, Pereira PJ, and dos Santos NM

Subjects

Amino Acid Sequence, Animals, Base Sequence, Bass metabolism, Blotting, Southern veterinary, Cloning, Molecular, DNA, Complementary genetics, DNA, Complementary metabolism, Fish Proteins chemistry, Fish Proteins metabolism, Gene Dosage, Models, Molecular, Molecular Sequence Data, Phylogeny, Polymerase Chain Reaction veterinary, Protein Disulfide-Isomerases chemistry, Protein Disulfide-Isomerases metabolism, Protein Sorting Signals, Protein Structure, Secondary, RNA, Messenger genetics, RNA, Messenger metabolism, Sequence Alignment veterinary, Thioredoxins chemistry, Thioredoxins metabolism, Bass genetics, Fish Proteins genetics, Protein Disulfide-Isomerases genetics, Thioredoxins genetics

Abstract

PDI (PDIA1) and ERp57 (PDIA3), members of the PDI family and of the thioredoxin (Trx) superfamily, are multifunctional proteins with wide physiological roles and have been implicated in several pathologies. Importantly, they are both involved in the MHC class I antigen presentation pathway. This paper reports the isolation and characterization of full cDNA and genomic clones from sea bass (Dicentrarchus labrax, L.) PDI (Dila-PDI) and ERp57 (Dila-ERp57). The genes are ~12.4 and ~7.1 kb long, originating 2155 and 2173 bp transcripts and encoding 497 and 484 amino acids mature proteins, for Dila-PDI and -ERp57, respectively. The PDI gene consists of eleven exons and ERp57 of thirteen. As described in other species, both molecules are composed of four Trx-like domains (abb'a') followed by a C-terminal tail, retaining two CGHC active sites and an ER-signalling sequence, suggestive of a conserved function. Additionally, three-dimensional homology models further support Dila-PDI and Dila-ERp57 as orthologs of mammalian PDI and ERp57, respectively. Finally, high similarity is observed to their vertebrate counterparts (>69% identity), especially among the few ones from closely related teleosts (>79% identity). Hence, these results provide relevant primary data and will enable further studies to clarify the roles of PDI and ERp57 in European sea bass immunity., (Copyright © 2013 Elsevier Ltd. All rights reserved.)

Published

2013

10. Cerulenin upregulates heat shock protein-70 gene expression in chicken muscle.

Author

Dridi S, Decuypere E, and Buyse J

Subjects

Animals, Blotting, Southern veterinary, Cerulenin administration & dosage, Ceruloplasmin metabolism, Chickens metabolism, Fatty Acid Synthesis Inhibitors administration & dosage, Ferric Compounds blood, HSP70 Heat-Shock Proteins metabolism, Organ Specificity, Oxidation-Reduction, Radioimmunoassay veterinary, Reverse Transcriptase Polymerase Chain Reaction veterinary, Thiobarbituric Acid Reactive Substances metabolism, Cerulenin pharmacology, Chickens genetics, Fatty Acid Synthesis Inhibitors pharmacology, Gene Expression Regulation drug effects, HSP70 Heat-Shock Proteins genetics

Abstract

Lines of evidence suggested that systems involved in the regulation of the stress responses and energy homeostasis are highly integrated. Because cerulenin, the natural antibiotic product of the fungus Cephalosporium ceruleans and a broad-spectrum fatty acid synthesis (FAS) inhibitor, has been shown to affect food intake and energy balance, and because the biomarker of stress Hsp-70 gene was found to interact directly with fatty acids, we hypothesized that cerulenin may regulate Hsp-70 gene expression. Therefore, the present study was undertaken to examine this issue. Cerulenin administration significantly (P < 0.05) decreased food intake and induced Hsp-70 mRNA levels in muscle, but not in liver or hypothalamus of 2-wk-old broiler chickens. These changes were accompanied by an unpregulation of muscle uncoupling protein and carnitine palmitoyltransferase 1 mRNA levels. This result indicated that the regulation of Hsp-70 gene expression in normal chickens, as estimated by oxidative stress indices [TBA reacting substances, ferric reducing/antioxidant power, and ceruloplasmin oxidase activity] levels, is tissue-specific. In attempt to discriminate between the effect of cerulenin and cerulenin-reduced food intake on Hsp-70 gene expression, we also evaluated the effect of food deprivation on the same cellular responses. Food deprivation for 16 h did not affect Hsp-70 gene expression in all tissues examined, indicating that the effect of cerulenin is independent of the inhibition of food intake. To ascertain whether the effect of cerulenin is direct or indirect, we carried out in vitro studies. Cerulenin treatment did not affect Hsp-70 gene expression in Leghorn male hepatoma and quail myoblast cell lines, suggesting that the observed effect in vivo may be mediated through the central nervous system.

Published

2013

11. Occurrence of the transferable copper resistance gene tcrB among fecal enterococci of U.S. feedlot cattle fed copper-supplemented diets.

Author

Amachawadi RG, Scott HM, Alvarado CA, Mainini TR, Vinasco J, Drouillard JS, and Nagaraja TG

Subjects

Animal Feed analysis, Animals, Bacterial Proteins metabolism, Blotting, Southern veterinary, Cattle, Copper administration & dosage, Dietary Supplements, Drug Resistance, Multiple, Bacterial, Enterococcus faecium drug effects, Enterococcus faecium metabolism, Enterococcus faecium pathogenicity, Feces microbiology, Female, Gene Transfer, Horizontal, Methyltransferases metabolism, Minisatellite Repeats, Molecular Sequence Data, Multilocus Sequence Typing veterinary, Multiplex Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Tetracycline pharmacology, Tylosin pharmacology, Vancomycin pharmacology, Virulence Factors genetics, Virulence Factors metabolism, Anti-Bacterial Agents pharmacology, Bacterial Proteins genetics, Copper pharmacology, Drug Resistance, Bacterial, Enterococcus faecium genetics, Methyltransferases genetics

Abstract

Copper, an essential micronutrient, is supplemented in the diet at elevated levels to reduce morbidity and mortality and to promote growth in feedlot cattle. Gut bacteria exposed to copper can acquire resistance, which among enterococci is conferred by a transferable copper resistance gene (tcrB) borne on a plasmid. The present study was undertaken to investigate whether the feeding of copper at levels sufficient to promote growth increases the prevalence of the tcrB gene among the fecal enterococci of feedlot cattle. The study was performed with 261 crossbred yearling heifers housed in 24 pens, with pens assigned randomly to a 2×2 factorial arrangement of treatments consisting of dietary copper and a commercial linseed meal-based energy protein supplement. A total of 22 isolates, each identified as Enterococcus faecium, were positive for tcrB with an overall prevalence of 3.8% (22/576). The prevalence was higher among the cattle fed diets supplemented with copper (6.9%) compared to normal copper levels (0.7%). The tcrB-positive isolates always contained both erm(B) and tet(M) genes. Median copper MICs for tcrB-positive and tcrB-negative enterococci were 22 and 4 mM, respectively. The transferability of the tcrB gene was demonstrated via a filter-mating assay. Multilocus variable number tandem repeat analysis revealed a genetically diverse population of enterococci. The finding of a strong association between the copper resistance gene and other antibiotic (tetracycline and tylosin) resistance determinants is significant because enterococci remain potential pathogens and have the propensity to transfer resistance genes to other bacteria in the gut.

Published

2013

12. Identification and characterization of the genomic termini and cleavage/packaging signals of gallid herpesvirus type 2.

Author

Volkening JD and Spatz SJ

Subjects

Animals, Blotting, Southern veterinary, Cells, Cultured, Chick Embryo, Cloning, Molecular, Conserved Sequence, DNA, Viral metabolism, Herpesvirus 2, Gallid physiology, Molecular Sequence Data, Nucleocapsid metabolism, Poultry Diseases virology, Repetitive Sequences, Nucleic Acid, Sequence Alignment veterinary, Sequence Analysis, DNA veterinary, Terminator Regions, Genetic, Virus Replication, Chickens, DNA, Viral genetics, Herpesvirus 2, Gallid genetics, Marek Disease virology, Nucleocapsid genetics

Abstract

Herpesvirus replication within host cells results in concatemeric genomic DNA, which is cleaved into unit-length genomes and packaged into the capsid by a complex of proteins. The sites of cleavage have been identified for many herpesviruses, and conserved signaling sequences involved in cleavage and packaging have been characterized. The cleavage/packaging motifs pac-1, pac-2, and DR1 and two distinct groups of telomeric repeat sequences (static TRS and variable TRS) have been identified. By sequencing the termini of the gallid herpesvirus type 2 (GaHV-2) strain CU-2, two different cleavage sites (classical and aberrant) have been identified. Unlike classical cleavage of human herpesvirus type 1, which occurs within the DR1 site, classical cleavage of the GaHV-2 concatemers occurs 8.5 bp upstream of the DR1 site and results in an S-terminus containing telomeric repeats. Aberrant cleavage occurs the same distance from the DR1 site and generates a telomeric S-terminus but an L-terminus lacking an a sequence. These results are consistent with previous findings in other herpesviruses and should prove useful in the future study and manipulation of the GaHV-2 genome.

Published

2013

13. The cloning and inducible expression of the rainbow trout ERp57 gene.

Author

Sever L, Bols NC, and Dixon B

Subjects

Amino Acid Sequence, Analysis of Variance, Animals, Base Sequence, Blotting, Northern veterinary, Blotting, Southern veterinary, Blotting, Western veterinary, Cloning, Molecular, Cluster Analysis, Conserved Sequence genetics, DNA Primers genetics, DNA, Complementary genetics, Endoplasmic Reticulum metabolism, Gene Expression Profiling veterinary, Gene Expression Regulation genetics, Gene Expression Regulation immunology, Molecular Chaperones metabolism, Molecular Sequence Data, Oncorhynchus mykiss immunology, Phylogeny, Protein Disulfide-Isomerases metabolism, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Sequence Homology, Species Specificity, Molecular Chaperones genetics, Oncorhynchus mykiss genetics, Protein Disulfide-Isomerases genetics

Abstract

ERp57 is a member of a protein disulfide isomerase family and is a chaperone responsible for the correct folding of newly synthesized glycoproteins in the endoplasmic reticulum and in the assembly of the major histocompatibility complex class I in the endogenous pathway of antigen presentation. This study reports the identification of a full length ERp57 cDNA in rainbow trout that encodes a putative 477aa mature protein with an additional signal sequence of 16aa. The trout protein shared 75% identity with the human homolog, but interestingly did not include either a C terminal endoplasmic reticulum retention signal, Q/KEDL in humans, or a nuclear localization signal which is highly conserved in mammals. Amino acid sequence alignment revealed conservation of four classical domains in trout ERp57 and two conserved active CXXC redox motifs. Trout ERp57 protein was identified as a single band around 57 kDa. Southern blotting analysis revealed that there two copies of the ERp57 gene in the trout genome and northern blotting showed a wide tissue distribution of gene expression in various tissues with the highest expression in liver and egg. This study showed for the first time in teleost that ERp57 transcript is upregulated in response to immune stimuli such as double stranded RNA or phytohemagglutinin. Furthermore, upon treatment with ER stress inducer A23187, trout ERp57 protein expression levels were increased both in peripheral blood leukocytes and the RTS11 macrophage like cell line after 6 and 8 h respectively. These findings suggest a possible conserved function for trout ERp57 in the ER and during the activation of the immune response., (Copyright © 2012 Elsevier Ltd. All rights reserved.)

Published

2013

14. Prevalence and characterization of plasmid-mediated quinolone resistance genes in Salmonella isolated from poultry in Korea.

Author

Kim JH, Cho JK, and Kim KS

Subjects

Animals, Blotting, Southern veterinary, Ciprofloxacin, DNA Primers genetics, Electrophoresis, Gel, Pulsed-Field veterinary, Escherichia coli, Gene Transfer, Horizontal physiology, Levofloxacin, Microbial Sensitivity Tests, Nalidixic Acid, Plasmids genetics, Polymerase Chain Reaction veterinary, Poultry, Republic of Korea epidemiology, Drug Resistance, Bacterial genetics, Poultry Diseases epidemiology, Poultry Diseases microbiology, Quinolones, Salmonella genetics, Salmonella Infections, Animal epidemiology

Abstract

The purpose of this study was to investigate the prevalence and characteristics of plasmid-mediated quinolone resistance (PMQR) genes qnr, aac(6')-Ib-cr, and qepA in a total of 185 non-duplicate Salmonella spp. isolated from hatcheries, poultry farms, and poultry slaughterhouses during the period 2001 to 2010 in Korea. Additionally, mutation analysis of quinolone resistance determining regions (QRDRs), conjugation experiments, and plasmid analysis were performed in the PMQR-positive isolates. Among the 185 isolates, six (3.2%) contained qnr genes (two qnrB4 and four qnrS1) but none carried the aac(6')-Ib-cr or qepA genes. Among the six PMQR-positive isolates, one showed a single mutation (Ser83-Phe substitution) in the QRDRs of gyrA. Among them, three were non-susceptible (intermediate or resistant) to nalidixic acid (minimum inhibitory concentration [MIC] ≥256 µg/ml), ciprofloxacin (MIC 2 µg/ml), and levofloxacin (MIC 4 µg/ml), but others were susceptible to all of the three fluoroquinolones. They were resistant to six or more antimicrobial agents tested and were able to transfer quinolone resistance to recipient Escherichia coli J53 by conjugation. By performing a hybridization test, plasmids harbouring qnrB4 and qnrS1 genes were less than 8 kb and about 70 kb in size, respectively. The horizontal dissemination of qnrS1 gene was mediated by IncN plasmid. Compared with the recipient strain, MICs of the transconjugants increased two-fold to four-fold for nalidixic acid, and eight-fold to 16-fold for ciprofloxacin and levofloxacin. This report is the first to describe the detection of qnr genes in Salmonella spp. isolated from poultry in Korea. Widespread horizontal transfer of these genes among bacteria may be a serious public health concern because these can rapidly increase fluoroquinolone resistance. To ensure the public health, it is essential to continuously survey and carefully monitor the spread of PMQR genes in Salmonella from poultry.

Published

2013

15. Booster responses by oral vaccination with transgenic plants against chicken leucocytozoonosis.

Author

Ito A, Gotanda T, Himeno N, Itchoda N, Tabayashi N, Ike K, Sugimoto C, and Matsumura T

Subjects

Administration, Oral, Animals, Antigens, Protozoan immunology, Blotting, Southern veterinary, Blotting, Western veterinary, Chickens, DNA Primers genetics, Plant Leaves immunology, Polymerase Chain Reaction veterinary, Solanum tuberosum genetics, Vaccines, Synthetic administration & dosage, Haemosporida, Immunization, Secondary veterinary, Plants, Genetically Modified chemistry, Poultry Diseases parasitology, Poultry Diseases prevention & control, Protozoan Infections, Animal prevention & control, Vaccines, Synthetic virology

Abstract

We developed a transgenic potato (TrP/R7) expressing the recombinant R7 (rR7) antigen for use as an oral vaccine to protect against a chicken protozoan disease, chicken leucocytozoonosis. The TrP/R7 potato was produced by Agrobacterium tumefaciens-mediated transformation and regeneration, and the R7 gene insertion into potato chromosomes was confirmed by genomic polymerase chain reaction and Southern hybridization. rR7 antigen expression in TrP/R7 potato was also confirmed by sandwich enzyme-linked immunosorbent assay and western blotting using an antibody against the second-generation schizont of Leucocytozoon caulleryi. A transgenic potato clone with the highest rR7 antigen expression (3 µg rR7 antigen per gram of fresh-weight potato leaves) was selected, cultivated, and used in oral administration experiments to examine its ability to boost immunity. Chickens were immunized with chicken leucocytozoonosis vaccine "Hokken" by injection, and chickens that developed moderate levels of antibody titres were fed with TrP/R7 leaves. Chickens fed with TrP/R7 leaves showed increased antibody responses. In contrast, chickens fed with non-transgenic potato leaves showed a continuous decrease in antibody titres. Furthermore, chickens fed with TrP/R7 potato leaves showed strong resistance against experimental challenge with L. caulleryi infection. This study demonstrates the use of a plant-based oral vaccine to boost immunity against a protozoan disease.

Published

2013

16. Genetic basis of penicillin resistance of S. aureus isolated in bovine mastitis.

Author

Bagcigil AF, Taponen S, Koort J, Bengtsson B, Myllyniemi AL, and Pyörälä S

Subjects

Animals, Blotting, Southern veterinary, Cattle, Electrophoresis, Gel, Pulsed-Field veterinary, Female, Finland, Genetic Variation, Phylogeny, Plasmids metabolism, Polymerase Chain Reaction veterinary, Sequence Analysis, Protein veterinary, Staphylococcal Infections microbiology, Sweden, beta-Lactamases genetics, beta-Lactamases metabolism, Mastitis, Bovine microbiology, Penicillin Resistance, Penicillins pharmacology, Plasmids genetics, Staphylococcal Infections veterinary, Staphylococcus aureus drug effects, Staphylococcus aureus genetics

Abstract

Background: The blaZ gene encoding penicillin resistance can be located either chromosomally or on plasmids. The aim of this study was to investigate the genetic relationships and to determine the location of the blaZ gene in S. aureus isolated in bovine mastitis in Finland and Sweden., Methods: Seventy-eight β-lactamase positive S. aureus isolates from bovine mastitis (34 from Finland and 44 from Sweden) were included in the study. The localization of blaZ gene was determined by Southern blotting. The blaZ genes of the isolates were sequenced and the sequences were translated to beta-lactamase proteins and further grouped as different protein signatures. The isolates and, as control, 33 Swedish and 36 Finnish beta-lactamase negative isolates were typed with pulsed-field gel electrophoresis (PFGE)., Results: In 26 out of 34 Finnish isolates (76.5%) and in 25 out of 44 Swedish isolates (56.8%) the blaZ gene was localized on a plasmid. Six different protein signatures were found. One signature was found only in four Swedish isolates, but all other signatures were found both in Finnish and Swedish isolates. The PFGE results revealed a diversity of S. aureus clones. The protein signatures were not clearly associated with certain pulsotypes., Conclusions: The plasmid location of the blaZ gene was not statistically significantly more common in Finland than in Sweden, and hence does not explain the higher proportion of penicillin-resistant isolates of S. aureus causing bovine mastitis in Finland compared to Sweden.

Published

2012

17. A multicancer-like syndrome in a dog characterized by p53 and cell cycle-checkpoint kinase 2 (CHK2) mutations and sirtuin gene (SIRT1) down-regulation.

Author

Marfe G, De Martino L, Tafani M, Irno-Consalvo M, Pasolini MP, Navas L, Papparella S, Gambacurta A, and Paciello O

Subjects

Animals, Blotting, Southern veterinary, Dog Diseases pathology, Dogs, Down-Regulation genetics, Gene Expression Regulation, Neoplastic genetics, Jaw Neoplasms genetics, Jaw Neoplasms pathology, Jaw Neoplasms veterinary, Male, Neoplasms, Multiple Primary genetics, Neoplasms, Multiple Primary pathology, Reverse Transcriptase Polymerase Chain Reaction veterinary, Skin Neoplasms genetics, Skin Neoplasms pathology, Skin Neoplasms veterinary, Syndrome, Amino Acid Substitution genetics, Dog Diseases genetics, Genes, p53 genetics, Neoplasms, Multiple Primary veterinary, Protein Serine-Threonine Kinases genetics, Sirtuin 1 genetics

Abstract

Introduction: We have investigated SIRT1, p53 and cell cycle-checkpoint kinase 2 (CHK2) gene dysfunction in a dog with a multicancer syndrome-like in order to evaluate their potential role in the determinism of the disease and to establish a possible correlation between SIRT1 transcript level and p53 expression status., Material and Methods: Blood sample and tumour samples from a pure breed English Setter dog with different tumours were used for this study. Nucleotide sequence analysis was performed with a DNA autosequencer in order to examine p53 and CHK2 mutations. In addition, the expression level of SIRT1 was quantified by Southern Blot analysis of Reverse Transcriptase-Polymerase Chain Reaction (RT-PCR)., Results: Cytological examination revealed five different tumours: a cutaneous sebaceous epithelioma, a cutaneous mast cell tumour, a testicular Sertoli cell tumour, an oral malignant melanoma, and a cutaneous squamous cell carcinoma. Sequencing analysis revealed the presence of a nucleotide substitution, (CGG>CAG) exon 7 of the p53 gene in DNA from peripheral blood mononuclear cells (PBMCs) as well as in the melanoma; whereas the other four cancers showed the loss of the wild-type allele. Furthermore, CHK2 mutation at codon 311 has been identified in the melanoma and sebaceous epithelioma. In addition, SIRT1 cDNA expression decreased in all tumour samples compared to cDNA SIRT1expression level in peripheral blood mononuclear cells (PBMCs) in the same dog., Conclusions: These results suggest that the germ line mutation of the p53 gene at codon 248 might be, at least, one cause of the multicancer syndrome-like in our dog; furthermore, we show a possible correlation between SIRT1 transcript level and p53 mutations status. The regulatory role of SIRT1 in tumour suppressor pathways suggests that the net effect seen may represent both direct and indirect downstream regulation and it is likely to depend on the presence or absence of functional p53., (Copyright © 2011 Elsevier Ltd. All rights reserved.)

Published

2012

18. Prevalence of feline leukemia virus infection in domestic cats in Rio de Janeiro.

Author

de Almeida NR, Danelli MG, da Silva LH, Hagiwara MK, and Mazur C

Subjects

Animals, Blood Cell Count veterinary, Blotting, Southern veterinary, Brazil epidemiology, Cats, Enzyme-Linked Immunosorbent Assay veterinary, Polymerase Chain Reaction veterinary, Prevalence, Risk Factors, Leukemia Virus, Feline isolation & purification, Leukemia, Feline diagnosis, Leukemia, Feline epidemiology

Abstract

Peripheral blood smears of 1094 domestic cats were collected and tested by indirect immunofluorescence antibody assay for p27 antigen in cells to study the prevalence and risk factors for feline leukemia virus (FeLV) in the state of Rio de Janeiro. Sex, age, breed, outdoor access, neutering status, type of habitation (household, shelter, veterinary clinics and other places), number of household cats and clinical signs were registered on a form. Among the tested samples, 11.52% were positive. Risk factors for FeLV infection included outdoor access, age range between 1 and 5 years old, and cohabitation with numerous cats.

Published

2012

19. Selection of a recombinant Marek's disease virus in vivo through expression of the Marek's EcoRI-Q (Meq)-encoded oncoprotein: characterization of an rMd5-based mutant expressing the Meq of strain RB-1B.

Author

Kumar P, Dong H, Lenihan D, Gaddamanugu S, Katneni U, Shaikh S, Tavlarides-Hontz P, Reddy SM, Peters W, and Parcells MS

Subjects

Animals, Blotting, Southern veterinary, Cell Line, Transformed, Chick Embryo, Fibroblasts virology, Flow Cytometry veterinary, Mardivirus pathogenicity, Marek Disease genetics, Molecular Sequence Data, Oncogene Proteins, Viral chemistry, Oncogene Proteins, Viral metabolism, Poultry Diseases genetics, Recombination, Genetic, Specific Pathogen-Free Organisms, Chickens, Mardivirus genetics, Marek Disease virology, Oncogene Proteins, Viral genetics, Poultry Diseases virology, Transfection veterinary

Abstract

Marek's disease (MD) is a highly contagious viral disease of chickens (Gallus gallus domesticus) caused by MD virus (MDV), characterized by paralysis, neurologic signs, and the rapid onset of T-cell lymphomas. MDV-induced T-cell transformation requires a basic leucine zipper protein called Marek's EcoRI-Q-encoded protein (Meq). We have identified mutations in the coding sequence of Meq that correlated with virus pathotype (virulent, very virulent, and very virulent plus). The aim of this study was to determine whether recombinant viruses could be isolated based on Meq expression through in vivo selection. Chicken embryo fibroblasts (CEFs) were cotransfected with an rMd5 strain-based Meq deletion virus (rMd5deltaMeq) and meq loci from strains representing different pathotypes of MDV. Transfected CEFs were inoculated into chickens in two independent studies. We were able to isolate a single recombinant virus, rMDV-1137, in a contact-exposed chicken. rMDV-1137 had recombined two copies of the meq gene of RB-1B and was found to have pathogenicity similar to both RB-1B and rMd5 parental strains. We found the RB-1B- and rMd5-induced lymphomas showed differences in composition and that rMDV-1137-induced lymphomas were intermediate in their composition. We were able to establish cell lines from both RB-1B- (MDCC-UD35, -UD37) and rMDV-1137 (MDCC-UD36, -UD38)-induced, but not rMd5-induced, lymphomas. To date, no rMd5- or parent Md5-transformed T-cell lines have been reported. Our results suggest that 1) a recombinant MDV can be selected on the basis of oncogenicity; 2) changes in Meq sequence seem to affect tumor composition and the ability to establish cell lines; and 3) in addition to meq, other genomic loci affect MDV pathogenicity and oncogenicity.

Published

2012

20. Molecular characterization of hepcidin gene from mud loach (Misgurnus mizolepis; Cypriniformes).

Author

Nam YK, Cho YS, Lee SY, Kim BS, and Kim DS

Subjects

Amino Acid Sequence, Animals, Antimicrobial Cationic Peptides immunology, Base Sequence, Blotting, Southern veterinary, Computational Biology, Copper metabolism, Cypriniformes immunology, Gene Components, Gene Expression Regulation drug effects, Hepcidins, Iron metabolism, Kidney metabolism, Lipopolysaccharides, Liver metabolism, Molecular Sequence Data, Poly I-C immunology, Polymerase Chain Reaction veterinary, Polymorphism, Restriction Fragment Length, RNA, Messenger metabolism, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Spleen metabolism, Alleles, Antimicrobial Cationic Peptides genetics, Cypriniformes genetics, Gene Expression Regulation immunology

Abstract

The gene encoding hepcidin, an antimicrobial peptide, was isolated and characterized in the mud loach Misgurnus mizolepis (Cypriniformes). Mud loach hepcidin shows a considerable degree of structural homology to other vertebrate hamp1 orthologues at both the gene and protein levels, particularly with respect to its tripartite genomic organization, typical transcription-factor-binding motifs in its promoter, and conserved cysteine residues in the mature cationic peptide. The mud loach possesses at least two allelic forms of hamp1, which are expected to be translated into the same hepcidin preproprotein. The two alleles are transmitted from parental fish to offspring with a Mendelian inheritance pattern, as demonstrated with polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) genotyping. Southern blot hybridization analysis showed a high degree of polymorphisms in the restriction patterns of individuals. Mud loach hamp1 mRNA is predominantly expressed in the liver, although many other tissues showed detectable levels of hamp1 transcripts in RT-PCR assay. Lipopolysaccharide and bacterial challenges induced significant hamp1 expression, whereas hamp1 was not clearly stimulated by polyinosinic:polycytidylic acid [poly(I:C)] injection. Iron overload and Cu exposure also elevated hamp1 transcripts in various tissues. The transcriptional activation of mud loach hamp1 in response to these stimuli varied among tissue types, and the liver appears predominantly involved in hepcidin-mediated iron regulation. However, hepcidin expression in the kidney and spleen was preferentially modulated by inflammation-mediated signals produced by immune challenges. Our results suggest that mud loach hepcidin has two basic functions, in iron regulation and antimicrobial activity, and that its transcription is also modulated by other environmental perturbations, including heavy metal exposure., (Copyright © 2011 Elsevier Ltd. All rights reserved.)

Published

2011

21. Exogenous DNA internalisation by sperm cells is improved by combining lipofection and restriction enzyme mediated integration.

Author

Churchil RR, Gupta J, Singh A, and Sharma D

Subjects

Animals, Blotting, Southern veterinary, DNA metabolism, DNA Restriction Enzymes metabolism, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Immunoblotting veterinary, Lac Operon, Liposomes, Male, Polymerase Chain Reaction veterinary, Transfection veterinary, Chickens genetics, DNA genetics, DNA Restriction Enzymes genetics, Gene Transfer Techniques veterinary, Spermatozoa, Transfection methods

Abstract

1. Three types of exogenous DNA inserts, i.e. complete linearised pVIVO2-GFP/LacZ vector (9620 bp), the LacZ gene (5317 bp) and the GFP gene (2152 bp) were used to transfect chicken spermatozoa through simple incubation of sperm cells with insert. 2. PCR assay, Dot Blot hybridisation and Southern hybridisation showed the successful internalisation of exogenous DNA by chicken sperm cells. 3. Lipofection and Restriction Enzyme Mediated Integration (REMI) were used to improve the rate of internalisation of exogenous DNA by sperm cells. 4. Results from dot blot as well as Southern hybridisation were semi-quantified and improved exogenous DNA uptake by sperm cells through lipofection and REMI. Stronger signals were observed from hybridisation of LacZ as well as GFP specific probe with the DNA from lipofected exogenous DNA transfected sperm DNA in comparison with those transfected with nude exogenous DNA.

Published

2011

22. A new variant of Actinobacillus pleuropneumoniae serotype 3 lacking the entire apxII operon.

Author

Kuhnert P, Rohde J, and Korczak BM

Subjects

Actinobacillus Infections microbiology, Actinobacillus Infections veterinary, Actinobacillus pleuropneumoniae classification, Animals, Blotting, Southern veterinary, Genes, Bacterial genetics, Genotype, Operon genetics, Phenotype, Polymerase Chain Reaction veterinary, Serotyping veterinary, Swine, Swine Diseases microbiology, Actinobacillus pleuropneumoniae genetics, Bacterial Proteins genetics, Hemolysin Proteins genetics

Abstract

Actinobacillus pleuropneumoniae is an important respiratory pathogen causing pleuropneumonia in pig. The species is genetically characterized by the presence of 4 RTX (Repeats in the Structural ToXin) toxin genes: apxI, apxII, and apxIII genes are differentially present in various combinations among the different serotypes, thereby defining pathogenicity; the apxIV gene is present in all serotypes. Polymerase chain reaction (PCR)-based apx gene typing is done in many veterinary diagnostic laboratories, especially reference laboratories. The present report describes the isolation of atypical A. pleuropneumoniae from 4 independent cases from 2 countries. All isolates were beta-nicotinamide adenine dinucleotide (β-NAD) dependent and nonhemolytic but showed strong co-hemolysis with the sphingomyelinase of Staphylococcus aureus on sheep blood agar. Classical biochemical tests as well as Matrix-assisted laser desorption ionization time-of-flight mass spectrometry and sequence-based analysis (16S ribosomal RNA [rRNA] and rpoB genes) identified them as A. pleuropneumoniae. Apx-toxin gene typing using 2 different PCR systems showed the presence of apxIV and only the apxIII operon (apxIIICABD). None of the apxI or apxII genes were present as confirmed by Southern blot analysis. The 16S rRNA and rpoB gene analyses as well as serotype-specific PCR indicate that the isolates are variants of serotype 3. Strains harboring only apxIV and the apxIII operon are possibly emerging types of A. pleuropneumoniae and should therefore be carefully monitored for epidemiological reasons., (© 2011 The Author(s))

Published

2011

23. Resurrection of an alpha-1,3-galactosyltransferase gene-targeted miniature pig by recloning using postmortem ear skin fibroblasts.

Author

Ahn KS, Kim YJ, Kim M, Lee BH, Heo SY, Kang MJ, Kang YK, Lee JW, Lee KK, Kim JH, Nho WG, Hwang SS, Woo JS, Park JK, Park SB, and Shim H

Subjects

Animals, Blotting, Southern veterinary, Cloning, Organism methods, Ear, Embryo Transfer veterinary, Female, Fibroblasts ultrastructure, Gene Targeting veterinary, Oocytes physiology, Oocytes ultrastructure, Polymerase Chain Reaction veterinary, Pregnancy, Swine, Cloning, Organism veterinary, Galactosyltransferases genetics, Nuclear Transfer Techniques veterinary, Swine, Miniature

Abstract

Animals with a targeted disruption of genes can be produced by somatic cell nuclear transfer (SCNT). However, difficulties in clonal selection of somatic cells with a targeted mutation often result in heterogeneous nuclear donor cells, including gene-targeted and non-targeted cells, and impose a risk of producing undesired wildtype cloned animals after SCNT. In addition, the efficiency of cloning by SCNT has remained extremely low. Most cloned embryos die in utero, and the few that develop to term show a high incidence of postnatal death and abnormalities. In the present study, resurrection of an alpha-1,3-galactosyltransferase (αGT) gene-targeted miniature pig by recloning using postmortem ear skin fibroblasts was attempted. Three cloned piglets were produced from the first round of SCNT, including one stillborn and two who died immediately after birth due to respiratory distress syndrome and cardiac dysfunction. Among the three piglets, two were confirmed to be αGT gene-targeted. Fibroblasts derived from postmortem ear skin biopsies were used as nuclear donor cells for the second round of SCNT, and a piglet was produced. As expected, PCR and Southern analyses confirmed that the piglet produced from recloning was αGT gene-targeted. Currently, the piglet is fourteen months of age, and no overt health problems have been observed. Results from the present study demonstrate that loss of an invaluable animal, such as a gene-targeted miniature pig, may be rescued by recloning, with assurance of the desired genetic modification., (Copyright © 2011 Elsevier Inc. All rights reserved.)

Published

2011

24. Molecular cloning of sea bass (Dicentrarchus labrax L.) caspase-8 gene and its involvement in Photobacterium damselae ssp. piscicida triggered apoptosis.

Author

Reis MI, Costa-Ramos C, do Vale A, and dos Santos NM

Subjects

Amino Acid Sequence, Animals, Base Sequence, Bass genetics, Bass microbiology, Blotting, Southern veterinary, Caspase 8 genetics, Cloning, Molecular, Molecular Sequence Data, Phylogeny, RNA chemistry, RNA genetics, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Alignment, Sequence Analysis, DNA, Apoptosis immunology, Bass immunology, Caspase 8 immunology, Photobacterium immunology

Abstract

Caspase-8 is an initiator caspase that plays a crucial role in some cases of apoptosis by extrinsic and intrinsic pathways. Caspase-8 structure and function have been extensively studied in mammals, but in fish the characterization of that initiator caspase is still scarce. In this work, the sea bass counterpart of mammalian caspase-8 was sequenced and characterized, and its involvement in the apoptogenic activity of a toxin from a fish pathogen was assessed. A 2472 bp cDNA of sea bass caspase-8 was obtained, consisting of 1455 bp open reading frame coding for 484 amino acids and with a predicted molecular weight of 55.2 kDa. The sea bass caspase-8 gene has 6639 bp and is organized in 11 introns and 12 exons. Several distinctive features of sea bass caspase-8 were identified, which include two death effector domains, the caspase family domains p20 and p10, the caspase-8 active-site pentapeptide and potential aspartic acid cleavage sites. The sea bass caspase-8 sequence revealed a significant degree of similarity to corresponding sequences from several vertebrate taxonomic groups. A low expression of sea bass caspase-8 was detected in various tissues of non-stimulated sea bass. Furthermore, it is shown that stimulation of sea bass with mid-exponential phase culture supernatants from Photobacterium damselae ssp. piscicida (Phdp), known to induce selective apoptosis of macrophages and neutrophils, resulted in an increased expression of caspase-8 in the spleen, one of the main affected organs by Phdp infection., (2010 Elsevier Ltd. All rights reserved.)

Published

2010

25. Genetic diversity of porcine Pasteurella multocida strains from the respiratory tract of healthy and diseased swine.

Author

Bethe A, Wieler LH, Selbitz HJ, and Ewers C

Subjects

Animals, Blotting, Southern veterinary, DNA, Bacterial genetics, Electrophoresis, Agar Gel veterinary, Genes, Bacterial genetics, Genetic Variation genetics, Pasteurella Infections microbiology, Polymerase Chain Reaction, Rhinitis, Atrophic microbiology, Ribotyping veterinary, Swine microbiology, Pasteurella Infections veterinary, Pasteurella multocida genetics, Respiratory System microbiology, Rhinitis, Atrophic veterinary, Swine Diseases microbiology

Abstract

A total of 382 porcine Pasteurella multocida strains, isolated from cases of pneumonia and progressive atrophic rhinitis (PAR) as well as from clinically healthy pigs of more than 150 German husbandries were characterized by detection of virulence-associated genes (VAGs) and ribotyping to understand the relationships between "commensal" and "pathogenic" strains, enabling a rational choice of vaccine strains. The diversity of the strains according to VAGs was low and mainly limited to capsular type genes (capA: 53.4%; capD: 45.8%; capF: 0.3%; cap-negative: 0.5%; hssB: 95.3%), dermonecrotoxin gene toxA (3.4%), as well as adhesion-related genes pfhaB (20.9%) and hgbB (84.3%). Ribotyping identified 13 patterns, but the vast majority of strains (95.8%) clustered in only three of these, namely IA-1 (45.5%), IA-7 (30.1%), and IIA-1 (20.2%). Pattern IA-1 was associated with capD(+) strains (93.6%) and harboured the majority of toxA(+) strains (84.6%). Pattern IA-7 mostly contained pfhaB(-), toxA(-)capA(+) strains (93.9%), while pattern IIA-1 was predominantly composed of pfhaB(+), toxA(-)capA(+) strains (87.0%). Clinical strains associated with pneumonia or PAR shared the above mentioned major ribotypes in comparable proportions with strains derived from healthy pigs, suggesting P. multocida to act more as an opportunistic than as an obligate pathogen in pigs. The limited number of subpopulations may either reflect a recent evolution of P. multocida in pigs or a selection by means of horizontal transfer of capsular genes, toxA or pfhaB. These data enforce further phylogenetic and epidemiological studies, examining the properties of different subpopulations of porcine P. multocida strains as well as factors of the porcine hosts themselves, which might be involved in disease susceptibility.

Published

2009

26. Genetic diversity of major surface protein 1a of Anaplasma marginale in beef cattle.

Author

Molad T, Fleidrovich L, Mazuz M, Fish L, Leibovitz B, Krigel Y, and Shkap V

Subjects

Anaplasma marginale growth & development, Animals, Base Sequence, Blotting, Southern veterinary, Cattle, Cloning, Molecular, DNA, Bacterial chemistry, DNA, Bacterial genetics, Genetic Variation, Microsatellite Repeats, Molecular Sequence Data, Polymerase Chain Reaction veterinary, Sequence Analysis, DNA, Anaplasma marginale genetics, Anaplasmosis microbiology, Bacterial Outer Membrane Proteins genetics, Cattle Diseases microbiology

Abstract

The present study was aimed to demonstrate genotypic diversity of Anaplama marginale in infected beef herds grazing within anaplasmosis endemic regions. The genotypic diversity was identified among different herds, within each herd, and also within single animals. The Israeli strains revealed unique characteristics of MSP1a repeats and, in addition to the published repeats, six new tandem repeats designated Is1-5, and Is9 were identified. The superinfections of individual Anaplama centrale vaccinated animals with two genotypically different A. marginale strains were detected. Six out of 43 vaccinated animals in the G herd were each infected with two A. marginale strains carrying two distinct genotypes; in this herd the follow-up during years 2003-2007 demonstrated that several animals carried different msp1a genotypes at different time points. Coinfection with two different genotypes of A. marginale in A. centrale vaccinated cattle was observed in another herd, as well. It appears that A. marginale is composed of a heterogeneous changing bacterial population that evolves in the host or, the genotypic diversity implies high transmission intensity by the vector, or both. Learning how this diversity is generated and identification of distinct A. marginale strains coupled with high sequence variation of MSP1a will aid in understanding Anaplasma transmission and disease development.

Published

2009

27. Importance of the porcine ADAM3 disintegrin domain in sperm-egg interaction.

Author

Kim E, Park KE, Kim JS, Baek DC, Lee JW, Lee SR, Kim MS, Kim SH, Kim CS, Koo DB, Kang HS, Ryoo ZY, and Chang KT

Subjects

ADAM Proteins genetics, Amino Acid Sequence, Animals, Blotting, Southern veterinary, Blotting, Western veterinary, DNA chemistry, DNA genetics, Female, Fertilization in Vitro veterinary, Gene Dosage, Male, Molecular Sequence Data, Polymerase Chain Reaction veterinary, Protein Isoforms, Protein Structure, Tertiary, Sequence Alignment, Swine genetics, ADAM Proteins physiology, Sperm-Ovum Interactions physiology, Swine physiology

Abstract

In the mouse, ADAM3, a well-characterized testis-specific protein of the A disintegrin and metalloprotease (ADAM) family, has a crucial role in fertilization by mediating sperm binding to the egg zona pellucida. However, little is known about ADAM3 in other species, such as domestic pigs. We have identified porcine ADAM3 and analyzed the protein. RT-PCR and trypsinization of sperm surface proteins revealed that porcine ADAM3 is expressed at high levels in the testis and on the sperm surface. Furthermore, an IVF inhibition assay with a recombinant porcine ADAM3 disintegrin domain showed that treatment of the disintegrin domain effectively prevented pig sperm-egg interactions. In the present study, we demonstrated the presence of ADAM3a and ADAM3b molecules in the pig and examined their roles in fertilization.

Published

2009

28. Detection of Foxp3 protein expression in porcine T lymphocytes.

Author

Käser T, Gerner W, Hammer SE, Patzl M, and Saalmüller A

Subjects

Animals, Antibodies, Monoclonal chemistry, Antibodies, Monoclonal immunology, Antibody Specificity, Blotting, Southern veterinary, Blotting, Western veterinary, CD4 Antigens biosynthesis, CD4 Antigens immunology, CD8 Antigens biosynthesis, CD8 Antigens immunology, Cross Reactions, Flow Cytometry veterinary, Forkhead Transcription Factors genetics, Interleukin-2 Receptor alpha Subunit biosynthesis, Interleukin-2 Receptor alpha Subunit immunology, RNA, Messenger biosynthesis, RNA, Messenger genetics, Reverse Transcriptase Polymerase Chain Reaction veterinary, Swine blood, T-Lymphocyte Subsets immunology, Forkhead Transcription Factors biosynthesis, Swine immunology, T-Lymphocytes, Regulatory immunology

Abstract

Regulatory T cells (Tregs) are potent regulators of various immune reactions. Due to the lack of Treg-specific markers their analysis had often been challenging until the discovery of the transcription factor Forkhead-box p3 (Foxp3) which serves as this highly demanded marker. So far, antibodies staining human and murine Foxp3 have been developed. This study describes the analysis of four commercially available anti-Foxp3 antibodies for reactivity with their specific antigen in cells derived from porcine lymphoid tissues. One out of the four antibodies showed selective reactivity with porcine CD25(+) T lymphocytes. The intracellular antigen was expressed on a small subset of CD25(dim) cells and the majority of the CD25(high) positive T-cell subpopulation. Intracellular antigen positive cells showed a heterogeneous expression of other leukocyte differentiation antigens. The majority belonged to the CD4(+)CD8(+) T-lymphocyte subpopulation, but were also found in the CD4(+)CD8(-) subpopulation. Another small minority was included in the CD4(-)CD8(+) T-lymphocyte subpopulation. Additionally, a small fraction of the putative Foxp3(+) cells showed an expression of MHC-II molecules. These staining patterns in three and four colour flow cytometry analyses indicated that the cells detected by a rat anti-mouse/rat-Foxp3 antibody expressed the porcine Foxp3. The expression of the putative Foxp3 protein in distinct leukocyte subsets was confirmed by molecular analysis of Foxp3 mRNA expression. Using Western blot analysis specific protein bands could only be detected in fractions that also exhibited the corresponding Foxp3 mRNA expression. These experiments also revealed that the antibody recognized a single chain protein with a molecular mass of about 45kDA similar to Foxp3 described for other species. In summary, these data strongly indicate the reactivity of this antibody with porcine Foxp3. Thereby, this rat anti-mouse/rat Foxp3 antibody presents a powerful tool for the identification of porcine regulatory T cells.

Published

2008

29. cDNA cloning, genomic structure, expression analysis and biological activity of porcine A Proliferation-Inducing Ligand (APRIL).

Author

Shui Y, Guan ZB, Zhang JX, and Zhang SQ

Subjects

Amino Acid Sequence, Animals, B-Lymphocytes immunology, Base Sequence, Blotting, Southern veterinary, Blotting, Western veterinary, Cell Proliferation drug effects, Cloning, Molecular, DNA, Complementary genetics, Formazans chemistry, Molecular Sequence Data, RNA chemistry, RNA genetics, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Alignment, Swine immunology, Tetrazolium Salts chemistry, Tumor Necrosis Factor Ligand Superfamily Member 13 biosynthesis, Swine genetics, Tumor Necrosis Factor Ligand Superfamily Member 13 genetics

Abstract

A Proliferation-Inducing Ligand (APRIL) is a novel member of the tumor necrosis factor (TNF) superfamily. In this study, a novel cDNA has been isolated from pig spleen by homology cloning and 3'- and 5'-rapid amplification of cDNA ends (RACE) strategies and designates porcine APRIL (pAPRIL). The open reading frame (ORF) of this cDNA covers 756 bases, encoding 251 amino acids. The soluble part of pAPRIL shows 89% identity with its human counterpart at the level of the primary protein structure. The pAPRIL gene is approximately 2.1kb in size and comprises six exons and five introns. Southern blotting analysis indicated that the pAPRIL gene is a single copy gene. Real-time PCR analysis revealed that pAPRIL is constitutively expressed in various tissues. Recombinant His(6)-tagged psAPRIL protein was efficiently expressed in Escherichia coli BL21 (DE3) and its expression was confirmed by SDS-PAGE and Western blotting analysis. In vitro, purified recombinant psAPRIL protein co-stimulated the proliferation of porcine splenic B-cells in response to formalin-fixed Staphylococcus aureus Cowan 1 (SAC).

Published

2008

30. Prevalence and risk factors for hemoplasmas in domestic cats naturally infected with feline immunodeficiency virus and/or feline leukemia virus in Rio de Janeiro--Brazil.

Author

Macieira DB, de Menezes Rde C, Damico CB, Almosny NR, McLane HL, Daggy JK, and Messick JB

Subjects

Animals, Blood Cell Count veterinary, Blotting, Southern veterinary, Brazil epidemiology, Cats, Comorbidity, DNA, Bacterial chemistry, DNA, Bacterial genetics, Enzyme-Linked Immunosorbent Assay methods, Enzyme-Linked Immunosorbent Assay veterinary, Female, Male, Mycoplasma isolation & purification, Mycoplasma Infections epidemiology, Polymerase Chain Reaction veterinary, Prevalence, Prospective Studies, Risk Factors, Cat Diseases epidemiology, Feline Acquired Immunodeficiency Syndrome epidemiology, Leukemia, Feline epidemiology, Mycoplasma Infections veterinary

Abstract

The aim of this study was to determine the prevalence and risk factors for Mycoplasma haemofelis (Mhf) and 'Candidatus Mycoplasma haemominutum' (Mhm) infections in domestic cats tested for feline immunodeficiency virus (FIV) and feline leukemia virus (FeLV) with a commercial enzyme-linked immunosorbent assay (ELISA) kit. Based on serological testing, cats were grouped as i) FIV-positive (n=25); ii) FeLV-positive (n=39); iii) FIV/FeLV-positive (n=8); and iv) FIV/FeLV-negative (n=77). Complete blood counts were followed by DNA extraction, species-specific polymerase chain reaction (16S rRNA gene) for Mhf and Mhm and Southern blotting for all animals. Mhf DNA was found in 4.0, 2.6, 12.5 and 7.8% of the cats from groups i, ii, iii and iv, respectively, while 32, 5.1, 50 and 5.2% of these animals had an Mhm infection. Cats with FIV (OR=4.25, P=0.009) and both FIV and FeLV (OR=7.56, P=0.014) were at greater risk of being hemoplasma infected than retroviral-negative cats, mainly due to Mhm infection (OR=8.59, P=0.001 and OR=18.25, P=0.001, respectively). Among pure-breed cats, FIV-positive status was associated with hemoplasma infection (OR 45.0, P=0.001).

Published

2008

31. Repeated high dose imidocarb dipropionate treatment did not eliminate Babesia caballi from naturally infected horses as determined by PCR-reverse line blot hybridization.

Author

Butler CM, Nijhof AM, van der Kolk JH, de Haseth OB, Taoufik A, Jongejan F, and Houwers DJ

Subjects

Animals, Antibodies, Protozoan blood, Antiprotozoal Agents standards, Babesia isolation & purification, Babesiosis diagnosis, Babesiosis drug therapy, Complement Fixation Tests standards, Complement Fixation Tests veterinary, DNA, Protozoan blood, Horse Diseases diagnosis, Horses, Imidocarb standards, Imidocarb therapeutic use, Theileria isolation & purification, Theileriasis diagnosis, Time Factors, Antiprotozoal Agents therapeutic use, Babesiosis veterinary, Blotting, Southern veterinary, Horse Diseases drug therapy, Imidocarb analogs & derivatives, Polymerase Chain Reaction veterinary

Abstract

Imidocarb treatment of horses infected with Babesia caballi is supposed to eliminate the infection, but data on the efficacy of this treatment is scarce. The study presented here concerns four Paso Fino horses, which were imported into the island of Curacao on the basis of a piroplasmosis negative complement fixation test (CFT). Upon re-testing with an indirect fluorescent antibody test immediately after arrival in Curacao, two horses appeared to have antibodies to B. caballi and all horses had antibodies to Theileria equi. Subsequent testing with polymerase chain reaction combined with a reverse line blot yielded positive results for both agents in all four horses. Treatment with five consecutive doses of imidocarb dipropionate (4.7 mg/kg BW im q 72 h), temporarily resulted in negative results, but B. caballi and T. equi were detected again in the samples taken at 6 and 18 weeks after completion of the treatment. These results confirm that the CFT is not a suitable test for pre-import testing and that even high dose treatment with imidocarb may not be capable of eliminating B. caballi and T. equi infections from healthy carriers.

Published

2008

32. Cloning the swamp buffalo SRY gene for embryo sexing with multiplex-nested PCR.

Author

Fu Q, Zhang M, Qin WS, Lu YQ, Zheng HY, Meng B, Lu SS, and Lu KH

Subjects

Animals, Base Sequence, Blotting, Southern veterinary, Buffaloes genetics, Cloning, Molecular, DNA Primers chemistry, Embryo, Mammalian physiology, Female, Male, Molecular Sequence Data, Phylogeny, Polymerase Chain Reaction methods, Reproducibility of Results, Sequence Analysis, DNA, Sex Determination Analysis methods, Buffaloes embryology, Genes, sry genetics, Polymerase Chain Reaction veterinary, Sex Determination Analysis veterinary

Abstract

The polymerase chain reaction (PCR) is an efficient method for sexing embryos. The objective of this study was to develop an accurate and reliable method for sexing swamp buffalo (Bubalus bubalis) embryos. The SRY gene from swamp buffalo genomic DNA was amplified by PCR, using primers based on the sequence of the Holstein SRY gene. This fragment was sequenced based on a BLAST search; the SRY gene was highly conserved. Using a Southern blot, there was a strong signal in genomic DNA only from male swamp buffalo. Two pairs of nested primers, targeted to amplify the swamp buffalo SRY conserved region, were designed for sex identification. Simultaneously, the G3PDH gene was co-amplified to serve as an internal control. A multiplex-nested PCR system was optimized by varying the following individually: concentrations of Mg(2+) and dNTPs, ratio of concentrations of primers and numbers of cycles. Biopsies of 27 IVF-derived embryos and 24 embryos fertilized with Y-chromosome-bearing sperm were examined. Using optimized procedures, clear signals following PCR amplification were obtained from all embryo samples; PCR amplification accuracy was further verified by comparing PCR and dot blots. We concluded that this PCR technique was highly reliable for sexing swamp buffalo embryos.

Published

2007

33. Persistence of cyprinid herpesvirus 3 in infected cultured carp cells.

Author

Dishon A, Davidovich M, Ilouze M, and Kotler M

Subjects

Animals, Blotting, Southern veterinary, Cells, Cultured, DNA Primers, Gene Expression Regulation, Viral genetics, Herpesviridae physiology, Reverse Transcriptase Polymerase Chain Reaction veterinary, Time Factors, Tissue Culture Techniques veterinary, Virus Cultivation veterinary, Carps, Fish Diseases virology, Gene Expression Regulation, Viral physiology, Herpesviridae genetics, Herpesviridae Infections veterinary, Temperature, Virus Activation physiology

Abstract

Cyprinid herpesvirus 3 (CyHV-3), previously designated carp interstitial nephritis and gill necrosis virus or koi herpesvirus, is the cause of a worldwide mortal disease of koi and carp. Morphologically, the virus resembles herpesviruses, yet it bears a genome of 277 to 295 kbp, which is divergent from most of the genomic sequences available in GenBank. The disease afflicts fish in the transient seasons, when the water temperature is 18 to 28 degrees C, conditions which permit virus propagation in cultured cells. Here we report that infectious virus is preserved in cultured cells maintained for 30 days at 30 degrees C. CyHV-3-infected vacuolated cells with deformed morphology converted to normal, and plaques disappeared following shifting up of the temperature and reappeared after transfer to the permissive temperature. Viral propagation and viral gene transcription were turned off by shifting cells to the nonpermissive temperature. Upon return of the cells to the permissive temperature, transcription of viral genes was reactivated in a sequence distinguished from that occurring in naïve cells following infection. Our results show that CyHV-3 persists in cultured cells maintained at the nonpermissive temperature and suggest that viruses could persist for long periods in the fish body, enabling a new burst of infection upon a shift to a permissive temperature.

Published

2007

34. Cloning and expression analysis of goldfish (Carassius auratus L.) prominin.

Author

Walsh JG, Barreda DR, and Belosevic M

Subjects

AC133 Antigen, Actins analysis, Actins biosynthesis, Amino Acid Sequence, Animals, Antigens, CD chemistry, Base Sequence, Blotting, Southern veterinary, DNA Primers chemistry, DNA, Complementary chemistry, Gene Expression Profiling veterinary, Glycoproteins chemistry, Goldfish immunology, Goldfish metabolism, Macrophages physiology, Molecular Sequence Data, Peptides chemistry, RNA, Messenger analysis, RNA, Messenger biosynthesis, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Homology, Amino Acid, Antigens, CD biosynthesis, Antigens, CD genetics, Cloning, Molecular, Glycoproteins biosynthesis, Glycoproteins genetics, Goldfish genetics, Peptides genetics

Abstract

The integral membrane protein known as prominin was first identified on the apical surface of mouse neural epithelial cells as well as on the surface of human haematopoietic progenitor cells. This report describes a prominin-like sequence and expression analysis of the prominin in the goldfish. The predicted amino acid sequence for goldfish prominin shares all of the hallmark structural characteristics of the prominin family, however the relatedness assessed using the percent amino acid identity indicated that goldfish prominin cannot be placed into the current mammalian dichotomy of type 1 or 2. The real time PCR analyses indicated that prominin was broadly expressed in different tissues with particularly high levels observed in the kidney and gill of the goldfish. Goldfish prominin was also found to be differentially expressed in subpopulations of in vitro-derived goldfish macrophages, with the highest expression observed in progenitor cells.

Published

2007

35. Gene structure and transcription of IRF-1 and IRF-7 in the mandarin fish Siniperca chuatsi.

Author

Sun BJ, Chang MX, Song Y, Yao WJ, and Nie P

Subjects

Amino Acid Sequence, Animals, Base Sequence, Blotting, Southern veterinary, Cloning, Molecular, Interferon Regulatory Factor-1 biosynthesis, Interferon Regulatory Factor-7 biosynthesis, Molecular Sequence Data, Perciformes immunology, Phylogeny, RNA chemistry, RNA genetics, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Alignment, Transcription, Genetic, Interferon Regulatory Factor-1 genetics, Interferon Regulatory Factor-7 genetics, Perciformes genetics

Abstract

The genes of IRF-1 and IRF-7 have been cloned from the mandarin fish (Siniperca chuatsi). The IRF-1 gene has 4919 nucleotides (nt) and contains 10 exons and 9 introns, with an open reading frame (ORF) of 903nt encoding 301aa. The IRF-7 gene has 6057nt and also contains 10 exons and 9 introns, with an ORF of 1308nt encoding 436aa. The IRF-1 and IRF-7 genes have only one copy each in the genome. The transcription of IRF-1 and IRF-7 in different organs was analyzed by real-time PCR, and both molecules were constitutively expressed. The IRF-1 and IRF-7 mRNAs were abundant in gill, spleen, kidney and pronephros. The temporal transcriptional changes for IRF-1, IRF-7 and Mx were investigated within 48h after poly I: C stimulation in liver, gill, spleen and pronephros. An increased transcription was detected for IRF-1 and IRF-7 12h post-stimulation, being earlier than the transcription of Mx protein; however, IRF-1 and IRF-7 transcription decreased while the Mx protein was stable at 48h post-stimulation.

Published

2007

36. Rapid and efficient screening of a Representational Difference Analysis library using reverse Southern hybridisation: identification of genetic differences between Haemophilus parasuis isolates.

Author

Lancashire JF, Turni C, Blackall PJ, and Jennings MP

Subjects

Animals, Blotting, Southern veterinary, DNA, Bacterial chemistry, DNA, Bacterial genetics, Gene Library, Genetic Variation, Haemophilus parasuis isolation & purification, Haemophilus parasuis pathogenicity, Polymerase Chain Reaction veterinary, Sequence Analysis, DNA, Swine, Virulence, Haemophilus Infections microbiology, Haemophilus Infections veterinary, Haemophilus parasuis genetics, Swine Diseases microbiology

Abstract

Representational Difference Analysis (RDA) is an established technique used for isolation of specific genetic differences between or within bacterial species. This method was used to investigate the genetic basis of serovar-specificity and the relationship between serovar and virulence in Haemophilus parasuis. An RDA clone library of 96 isolates was constructed using H. parasuis strains H425(P) (serovar 12) and HS1967 (serovar 4). To screen such a large clone library to determine which clones are strain-specific would typically involved separately labelling each clone for use in Southern hybridisation against genomic DNA from each of the strains. In this study, a novel application of reverse Southern hybridisation was used to screen the RDA library: genomic DNA from each strain was labelled and used to probe the library to identify strain-specific clones. This novel approach represents a significant improvement in methodology that is rapid and efficient.

Published

2007

37. Exploratory study of Mycoplasma suis (Eperythrozoon suis) on four commercial pig farms in southern Brazil.

Author

Guimaraes AM, Biondo AW, Lara AC, and Messick JB

Subjects

Animals, Base Sequence, Blotting, Southern methods, Blotting, Southern veterinary, Brazil epidemiology, Cloning, Molecular, DNA, Bacterial genetics, Female, Gene Amplification, Hematocrit veterinary, Male, Molecular Sequence Data, Mycoplasma isolation & purification, Mycoplasma Infections epidemiology, Mycoplasma Infections microbiology, Polymerase Chain Reaction methods, Polymerase Chain Reaction veterinary, RNA, Ribosomal, 16S genetics, Sensitivity and Specificity, Sequence Analysis, DNA, Swine, DNA, Bacterial chemistry, Mycoplasma Infections veterinary, Swine Diseases epidemiology, Swine Diseases microbiology

Abstract

Mycoplasma suis (Eperythrozoon suis) was detected by PCR and Southern blot in 186 pigs (121 sows, 61 piglets and four boars) on four farms in southern Brazil. DNA was extracted from blood samples and a 16S rRNA gene fragment of M suis was amplified by PCR; Southern blot analysis was then performed on all the samples. Twenty-two of the sows (18.2 per cent) were positive by PCR, and 40 (33.1 per cent) were positive by Southern blot; only one piglet and one boar were positive. The packed cell volume and total plasma protein of the pigs and their PCR and Southern blot results were not significantly different on the four farms, but higher proportions of the pigs were positive by Southern blot than by PCR (P<0.05). The packed cell volume and total plasma protein concentrations of the M suis positive and negative sows were not significantly different.

Published

2007

38. Filamentous-haemagglutinin-like protein genes encoded on a plasmid of Moraxella bovis.

Author

Kakuda T, Sarataphan N, Tanaka T, and Takai S

Subjects

Animals, Bacterial Proteins, Base Sequence, Blotting, Southern veterinary, DNA, Bacterial chemistry, DNA, Bacterial genetics, Immunoglobulin Fab Fragments, Molecular Sequence Data, Open Reading Frames, Plasmids, Reverse Transcriptase Polymerase Chain Reaction veterinary, Transcription Factors, Hemagglutinins chemistry, Hemagglutinins genetics, Moraxella bovis genetics

Abstract

The complete nucleotide sequence of a plasmid, pMBO-1, from Moraxella bovis strain Epp63 was determined. We identified 30 open reading frames (ORFs) encoded by the 44,215bp molecule. Two large ORFs, flpA and flpB, encoding proteins with similarity to Bordetella pertussis filamentous haemagglutinin (FHA), were identified on the same plasmid. The gene for a specific accessory protein (Fap), which may play a role in the secretion of Flp protein, was also identified. Reverse transcriptase PCR analysis of total RNA isolated from M. bovis Epp63 indicated that the flpA, flpB, and fap genes are all transcribed. Southern blot analysis indicated that the flp and fap genes are present in other clinical isolates of geographically diverse M. bovis.

Published

2006

39. Expression and phylogenetic analysis of the ninth complement component (C9) in rainbow trout.

Author

Chondrou MP, Londou AV, and Zarkadis IK

Subjects

Animals, Blotting, Southern veterinary, Gene Expression Profiling veterinary, Molecular Sequence Data, Reverse Transcriptase Polymerase Chain Reaction veterinary, Complement C9 biosynthesis, Complement C9 classification, Gene Expression immunology, Oncorhynchus mykiss physiology, Phylogeny

Published

2006

40. Functional characterisation of the Japanese flounder, Paralichthys olivaceus, Mx promoter.

Author

Ooi EL, Hirono I, and Aoki T

Subjects

Animals, Base Sequence, Blotting, Southern veterinary, Cattle, Cell Line, DNA Mutational Analysis veterinary, DNA, Recombinant, Electrophoretic Mobility Shift Assay veterinary, Flounder genetics, Humans, Luciferases analysis, Luciferases biosynthesis, Mice, Molecular Sequence Data, Myxovirus Resistance Proteins, Promoter Regions, Genetic genetics, Flounder physiology, GTP-Binding Proteins genetics, GTP-Binding Proteins physiology, Promoter Regions, Genetic physiology

Abstract

The Japanese flounder, Paralichthys olivaceus, genome appears to encode a single Mx gene based on Southern blotting and previous cDNA studies. The 5' flanking region of the Japanese flounder Mx gene was cloned and analysed for its regulatory regions. A TATA box (-24 to -30), two interferon-stimulated response elements (ISREs) (-69 to -80 and -508 to -521) and two Sp1 sites (-563 to -572 and -994 to -1003) were identified relative to the transcription start site. The effects of various stimuli, as well as the effects of various promoter mutations, were investigated in a transient expression system using Japanese flounder (hirame) natural embryo (HINAE) cells and luciferase reporter gene constructs. Although not sensitive to LPS, ConA or PMA, reporter gene expression increased more than 10-fold after stimulation by polyinosinic:polycytidilic acid (poly I:C), an established inducer of interferon. Deletion mutational analyses revealed the ISRE closest to the transcription start site to be crucial for promoter activity. The distal ISRE, despite its relatively distant location, contributed to induce maximal promoter activity, but when alone was not sufficient by itself to elicit any significant promoter activity. An electrophoretic mobility shift assay confirmed the binding of transcription factors to both ISREs. Induction of luciferase by poly I:C was inhibited by 2-Aminopurine, a protein kinase (PKR) inhibitor, in a dose-dependent (1-10 mM) manner, suggesting that PKR may be required as a signal transducer for type I IFN signaling in fish. This Mx reporter assay may be useful for quantifying the responses and elucidating the regulation pathways of IFN type I.

Published

2006

41. Cloning and nucleotide sequencing of three heat shock protein genes (hsp90, hsc70, and hsp19.5) from the diamondback moth, Plutella xylostella (L.) and their expression in relation to developmental stage and temperature.

Author

Sonoda S, Ashfaq M, and Tsumuki H

Subjects

Amino Acid Sequence, Animals, Base Sequence genetics, Blotting, Southern veterinary, Cloning, Molecular, DNA Primers chemistry, Female, HSC70 Heat-Shock Proteins biosynthesis, HSC70 Heat-Shock Proteins genetics, HSC70 Heat-Shock Proteins physiology, HSP90 Heat-Shock Proteins biosynthesis, HSP90 Heat-Shock Proteins genetics, HSP90 Heat-Shock Proteins physiology, Heat-Shock Proteins biosynthesis, Heat-Shock Proteins chemistry, Heat-Shock Proteins genetics, Male, Molecular Sequence Data, Moths genetics, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Alignment, Sequence Homology, Amino Acid, Gene Expression Regulation, Developmental physiology, Heat-Shock Proteins physiology, Moths physiology

Abstract

Heat shock protein genes, hsp90, hsc70, and hsp19.5, were cloned and sequenced from the diamondback moth, Plutella xylostella (L.) by RT-PCR and RACE method. The cDNA sequence analysis of hsp90 and hsp19.5 revealed open reading frames (ORFs) of 2,151 and 522 bp in length, which encode proteins with calculated molecular weights of 82.4 and 19.5 kDa, respectively. Analysis of cDNA from hsc70 revealed an ORF of 1,878 bp coding a protein with a calculated molecular weight of 69.3 kDa. Furthermore, the analysis of genomic DNA from hsc70 confirmed the presence of introns while no introns were apparent in hsp90 and hsp19.5. Southern blot analysis suggested the presence of multiple copies of each gene family in the DBM genome. Detectable expression of hsp19.5 was observed at the pupal stage while expression of hsp90 and hsc70 was detected at both pupal and adult stages. At adult stage, females showed a higher expression of hsp90 and hsc70 than males. An increased expression was observed in all three genes after exposure to a high temperature in both sexes. These results suggest that in addition to a heat shock response, these HSP genes might be involved in other functions during the course of development in DBM.

Published

2006

42. Construction of gender-enriched cDNA archives for adult Oesophagostomum dentatum by suppressive-subtractive hybridization and a microarray analysis of expressed sequence tags.

Author

Cottee PA, Nisbet AJ, Abs El-Osta YG, Webster TL, and Gasser RB

Subjects

Animals, Blotting, Northern veterinary, Blotting, Southern veterinary, Caenorhabditis elegans genetics, DNA Primers chemistry, Female, Gene Expression genetics, Gene Library, Male, Nucleic Acid Hybridization methods, Oligonucleotide Array Sequence Analysis veterinary, Reverse Transcriptase Polymerase Chain Reaction veterinary, Swine, Computational Biology, Expressed Sequence Tags, Gene Expression physiology, Oesophagostomum genetics, Oesophagostomum physiology

Abstract

In the present study, we constructed gender-enriched cDNA libraries for the adult stage of the parasitic nematode Oesophagostomum dentatum (order Strongylida) using suppressive-subtractive hybridization (SSH), sequenced clones from the female-library and male-library (480 from each) and conducted bioinformatic and microarray analyses of the expressed sequence tags (ESTs). In total, 873 ESTs (440 male and 433 female) were obtained, achieving a sequencing success of 91%The nucleotide sequences reported in this article (Tables 1-5) have been deposited in the EMBL, GenBank and DDJB databases under the Accession nos. AM157797-AM158083. Microarray analyses of 516 unique ESTs representing both gender-enriched libraries revealed differential hybridization for 391 of them (75.8%). Of these, 220 (56.3%) had significantly greater signal intensities in the female than in the male, and 154 (70%) of these were predicted to have homologues in C. elegans. These homologues were predicted to be involved in key biological processes, including embryonic nutrition, gametogenesis, molecular binding/transport or metabolism, nucleic acid synthesis and function, and signal transduction. Of the 171 ESTs with statistically higher signal intensities in male O. dentatum, 43.8% had homologues in C. elegans. These homologues included major sperm proteins (MSPs) or MSP-like molecules, keratin-like molecules, molecules involved in metabolism, PDZ domain-containing proteins, sugar binding proteins, protein kinases, serine proteases or protease inhibitors, molecules involved in proteolysis and other proteins, such as enzymes and various putative proteins. Of the 287 ESTs (from both gender-enriched cDNA libraries) with no known homologues in C. elegans, 50 (17.4%) had homologues in other nematodes, 8 had homologues in various other organisms and 104 (36.2%) had no homology to any sequence in current gene databases. The present study lays a foundation for the isolation and molecular, biochemical and functional characterization of selected genes from the gender-enriched cDNA archives established for O. dentatum.

Published

2006

43. Isolation, characterization, and expression analysis of three actin genes in the New Zealand black-footed abalone, Haliotis iris.

Author

Bryant MJ, Flint HJ, and Sin FY

Subjects

Actins analysis, Actins biosynthesis, Actins chemistry, Amino Acid Sequence, Animals, Base Sequence, Blotting, Southern veterinary, DNA chemistry, DNA Primers chemistry, Gene Expression Profiling veterinary, Growth and Development genetics, Growth and Development physiology, Larva growth & development, Molecular Sequence Data, Mollusca growth & development, Polymerase Chain Reaction veterinary, Sequence Alignment veterinary, Sequence Homology, Zygote physiology, Actins genetics, Mollusca genetics, Mollusca physiology

Abstract

Three actin genes -- H. irisA1, H. irisA2, and H. irisA3 -- from the mollusc Haliotis iris (New Zealand black-footed abalone) were isolated by polymerase chain reaction (PCR). The genes were similar to molluscan (84.1% to 94.9%) and vertebrate (84.5% to 86.6%) actins. The sequence similarity between the genes ranged from 88.5% to 93.2%. The greatest disparity, 32.3%, was found over a 99-nt region located at nt 808-906 of H. irisA1, corresponding to amino acids 212-244 of the three actins. The H. iris actin gene family contains at least eight members. Reverse transcription (RT)-PCR analysis of the three genes showed H. irisA1 and H. irisA2 were expressed at low levels in fertilized eggs and blastula stages and at high levels in trochophore and veliger larvae. H. irisA3 was detected in fertilized eggs; it was not detected in the blastula stages and at high levels in the trochophore and veliger larvae. The structure and expression of the three actin genes are discussed.

Published

2006

44. Isolation in cell culture and detection by PCR-based technology of IPNV-like virus from leucocytes of carrier turbot, Scophthalmus maximus (L.).

Author

Cutrín JM, López-Vázquez C, Olveira JG, Castro S, Dopazo CP, and Bandín I

Subjects

Animals, Base Sequence, Blotting, Southern veterinary, Cluster Analysis, DNA Primers, Molecular Sequence Data, Polymerase Chain Reaction veterinary, Polymorphism, Restriction Fragment Length, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Analysis, DNA veterinary, Spain, Aquaculture methods, Birnaviridae Infections veterinary, Fish Diseases virology, Flatfishes, Infectious pancreatic necrosis virus genetics, Phylogeny, Viremia veterinary

Abstract

A non-destructive procedure was utilized to determine the infectious pancreatic necrosis virus (IPNV) status of an apparently healthy turbot broodstock. Blood samples were used to detect IPNV by reverse transcriptase-polymerase chain reaction (RT-PCR), Southern blot hybridization and nested PCR. In addition, viral isolation from turbot leucocytes was performed. Around 22% of the fish were IPNV positive by RT-PCR, and this increased to close to 60% when nested PCR was performed. The present report supports the use of blood samples for the detection of IPNV-like viruses in brood fish. In addition, we demonstrate that it is possible to isolate the virus from the blood of carrier fish, as a non-lethal detection method, although it is much less sensitive than RT-PCR and nested PCR as a IPNV-like strain was isolated from only five of the 15 blood sample pools assayed. The viral isolate was identified as type Dry Mills (genogroup I) by means of restriction fragment length polymorphisms and DNA sequencing.

Published

2005

45. Differences in tumor necrosis factor (TNF)alpha and TNF receptor-1-mediated intracellular signaling factors in normal, inflamed and scar-formed horse tendons.

Author

Hosaka Y, Kirisawa R, Ueda H, Yamaguchi M, and Takehana K

Subjects

Animals, Blotting, Southern veterinary, Blotting, Western veterinary, Caspase 3, Caspases metabolism, DNA Primers, Horse Diseases pathology, Horses, Immunohistochemistry veterinary, In Situ Hybridization veterinary, Inflammation metabolism, Inflammation pathology, Reverse Transcriptase Polymerase Chain Reaction veterinary, TNF Receptor-Associated Factor 2 metabolism, Tendons pathology, Horse Diseases metabolism, Inflammation veterinary, Receptors, Tumor Necrosis Factor, Type I metabolism, Signal Transduction physiology, Tendons metabolism, Tumor Necrosis Factor-alpha metabolism

Abstract

Tumor necrosis factor (TNF) receptors (TNF-R)-mediated cell survival or apoptosis has been demonstrated in many cells, but little is known about survival or apoptotic signals via TNF-R1 in tendinocytes. In this study, we focused on four signaling factors, TNFalpha, TNF-R1, TNFR-associated factor2 (TRAF2) and caspase-3, in order to elucidate the signaling events in tendinocytes. Samples were obtained from normal, inflamed and scar-formed equine superficial digital flexor tendons. To detect these signaling factors, samples were subjected to immunohistochemistry and Western blot analysis, and some samples were also subjected to reverse transcription-polymerase chain reaction (RT-PCR), PCR-Southern blot analysis and in situ hybridization to detect the expression of TNFalpha mRNA. Distribution of the four factors differed depending on the tendon condition, normal, inflamed or scar-formed. In the normal tendon, large amounts of TRAF2 were found in tendinocytes, but the amounts of TNF-R1 were small. TNFalpha mRNA was expressed most highly in the inflamed tendon. TNF-R1, which was only faintly detected in the normal tendon, was detected at a high level in the inflamed tendon, and the amounts of TRAF2 and caspase-3 also increased. Activated caspase-3 was only detected in the inflamed tendon. TNFalpha mRNA was also expressed in the scar-formed tendon, though it showed weak signals, and the expression levels of TNF-R1, TRAF2 and caspase-3 proteins were very low. Two distinct intracellular signaling pathways of TNFalpha, which lead to cell survival and apoptosis, might be present in tendinocytes mediated through TNF-R1. These results, which reflect the dynamism of TNFalpha, provide important clues for means to prevent tendinopathy.

Published

2005

46. Development of a new PCR assay to identify Brucella abortus biovars 5, 6 and 9 and the new subgroup 3b of biovar 3.

Author

Ocampo-Sosa AA, Agüero-Balbín J, and García-Lobo JM

Subjects

Animals, Base Sequence, Blotting, Southern veterinary, Brucella classification, Brucella genetics, Brucella isolation & purification, Brucella abortus isolation & purification, Brucellosis diagnosis, Brucellosis microbiology, Brucellosis veterinary, DNA Fragmentation, Phylogeny, Polymerase Chain Reaction methods, Brucella abortus classification, Brucella abortus genetics, DNA, Bacterial analysis, Polymerase Chain Reaction veterinary

Abstract

One hundred twenty-nine Brucella field strains isolated from cattle in Cantabria, Spain, from March 1999 to February 2003, were analysed by using the AMOS-ERY PCR assay and by Southern blot hybridisation with a probe from insertion sequence IS711. Most of the field isolates produced only the ery band in the AMOS-ERY assay and showed a hybridisation pattern identical to that exhibited by reference strains of biovars 5, 6 and 9 of Brucella abortus, but different from strain Tulya, belonging to biovar 3 of B. abortus. However, typing of these strains by standard methods demonstrated that they belonged to biovar 3 of B. abortus. These results indicated that B. abortus biovar 3 was not genetically homogeneous and at least could be divided in two. In one class, that we called biovar 3a, would be the Tulya strain, while the local field strains would belong to biovar 3b. Cloning and nucleotide sequencing of a DNA fragment containing an IS711 copy exclusive of the B. abortus field strains from biovar 3b and reference strains from biovars 5, 6 and 9, revealed the existence of a 5.4 kb deletion close to an IS711 copy. Based on these data, we designed a new primer, which together with the IS711 AMOS primer produced a PCR fragment of 1.7 kb only from the isolates of biovars 3b, 5, 6 and 9 of B. abortus. No amplification products were produced with these primers from strains of the rest of species and biovars of Brucella and from bacteria phylogenetically close to Brucella analysed in this work. Addition of this primer to the AMOS-ERY PCR primer cocktail allows the positive distinction of B. abortus biovars 3b, 5, 6 and 9 from the rest of Brucella species and biovars.

Published

2005

47. Biofilm production by Staphylococcus aureus associated with intramammary infection.

Author

Fox LK, Zadoks RN, and Gaskins CT

Subjects

Animals, Bacteriophage Typing veterinary, Blotting, Southern veterinary, Cattle, Cross-Sectional Studies, DNA, Bacterial chemistry, DNA, Bacterial genetics, Electrophoresis, Gel, Pulsed-Field veterinary, Female, Milk microbiology, Skin microbiology, Staphylococcal Infections microbiology, Statistics, Nonparametric, Washington, Biofilms growth & development, Mastitis, Bovine microbiology, Staphylococcal Infections veterinary, Staphylococcus aureus growth & development

Abstract

Biofilm production by 221 Staphylococcus aureus isolates from 45 dairy herds was evaluated. Isolates were from composite milk of 117 cows, from teat skin of 70 cows, and from 34 milking machine unit liners. Of S. aureus from milk samples, 41.4% were biofilm producers, as compared to 24.7 and 14.7% of the isolates collected from skin and liners. Pulsed field gel electrophoresis (PFGE) best categorized S. aureus biofilm producers as compared to phage typing and binary typing. PFGE types that were significantly associated with isolation from milk as opposed to teat skin or liners, had isolates that were more likely to produce biofilm than PFGE types that were isolated from milk, skin and liners at similar frequencies. By contrast, PFGE type A was significantly associated with isolation from teat skin and had few biofilm producers. PFGE type Q, which is exclusively a milk, isolate produced more biofilm as evidenced by absorbance values. Given S. aureus that are associated with milk are more likely to produce biofilm as compared to extramammary sources (teat skin and milking unit liners), suggests that biofilm production is a risk factor for infection.

Published

2005

48. The distribution of bmpB, a gene encoding a 29.7 kDa lipoprotein with homology to MetQ, in Brachyspira hyodysenteriae and related species.

Author

La T, Tan P, Phillips ND, and Hampson DJ

Subjects

Amino Acid Sequence, Animals, Bacterial Outer Membrane Proteins chemistry, Base Sequence, Blotting, Southern veterinary, Blotting, Western veterinary, DNA, Bacterial chemistry, DNA, Bacterial genetics, Lipoproteins chemistry, Multienzyme Complexes chemistry, Multienzyme Complexes genetics, NADH, NADPH Oxidoreductases chemistry, NADH, NADPH Oxidoreductases genetics, Polymerase Chain Reaction veterinary, Recombinant Proteins chemistry, Recombinant Proteins genetics, Sequence Alignment, Sequence Homology, Nucleic Acid, Swine, Bacterial Outer Membrane Proteins genetics, Lipoproteins genetics, Spirochaetaceae genetics, Swine Diseases microbiology

Abstract

The distribution of the bmpB gene encoding BmpB, a 29.7 kDa outer membrane lipoprotein of the intestinal spirochaete Brachyspira hyodysenteriae, was investigated. Using PCR, the gene was detected in all the 48 strains of B. hyodysenteriae examined and in Brachyspira innocens strain B256T, but not in 11 other strains of B. innocens nor in 42 strains of other Brachyspira spp. The gene was sequenced from B. innocens strain B256T and from 11 strains of B. hyodysenteriae. The B. hyodysenteriae genes shared 97.9-100% nucleotide sequence similarity and had 97.5-99.5% similarity with the gene of B. innocens strain B256T. Southern hybridisation indicated that bmpB was present on a 1.9 kb HindIII fragment of the B. hyodysenteriae genome and on a 3.1 kb fragment of the B. innocens B256T genome. The B. innocens lipoprotein did not react in Western blots with monoclonal antibody BJL/SH1 that reacts with the B. hyodysenteriae lipoprotein. The difference in binding with the monoclonal antibody may reside in the replacement of a serine residue with a tyrosine residue at base position 210 in the lipoprotein from B. innocens B256T. Comparison of the BmpB amino acid sequence with sequences in the SWISS-PROT protein database indicated that it has 33.9-39.9% similarity with the d-methionine binding proteins (MetQ) of a number of pathogenic bacterial species. The bmpB gene was confirmed to be the same as a gene of B. hyodysenteriae that was recently designated "blpA".

Published

2005

49. Insertion sequence profiling of UK Mycoplasma bovis field isolates.

Author

Miles K, McAuliffe L, Persson A, Ayling RD, and Nicholas RA

Subjects

Animals, Blotting, Southern veterinary, Cattle, Cluster Analysis, DNA, Bacterial chemistry, DNA, Bacterial genetics, Lung Diseases microbiology, Mycoplasma Infections microbiology, Mycoplasma bovis isolation & purification, Restriction Mapping veterinary, United Kingdom, Cattle Diseases microbiology, DNA Transposable Elements genetics, Lung Diseases veterinary, Mycoplasma Infections veterinary, Mycoplasma bovis genetics

Abstract

The presence and distribution of insertion sequences ISMbov2 and ISMbov3 within Mycoplasma bovis were investigated. Analysis was carried out by Southern blotting using specific probes of 221 bp and 185 bp, to detect ISMbov2 and ISMbov3, respectively, amplified from the homologous sequences ISMmy1 and IS1634 within Mycoplasma mycoides subspecies mycoides small colony type. We present data obtained from 49 field isolates of M. bovis, originating from pneumonic lungs, collected within the United Kingdom between 1996 and 2002. Hybridisation profiles show considerable variation between strains. ISMbov2 sequences are present between 2 and 17 copies while there are between 3 and 14 copies of the IS1634 homologue ISMbov3. These data also provide support for previous analysis by random amplified polymorphic DNA (RAPD) and amplified fragment length polymorphism (AFLP).

Published

2005

50. Molecular cloning of TRAF2 binding protein gene and its promoter region from the grass carp Ctenopharyngodon idellus.

Author

Chang MX, Nie P, Sun BJ, and Yao WJ

Subjects

Amino Acid Sequence, Animals, Base Sequence, Blotting, Southern veterinary, Carps parasitology, Cloning, Molecular, Copepoda growth & development, Gene Dosage, Molecular Sequence Data, Promoter Regions, Genetic genetics, Protein Binding, RNA, Messenger biosynthesis, RNA, Messenger genetics, Random Amplified Polymorphic DNA Technique veterinary, Reverse Transcriptase Polymerase Chain Reaction veterinary, Sequence Alignment, TNF Receptor-Associated Factor 2 metabolism, Adaptor Proteins, Signal Transducing genetics, Carps genetics, Receptors, Tumor Necrosis Factor genetics

Abstract

A tumor necrosis factor receptor-associated factor 2 binding protein (T2BP) gene was isolated from the grass carp (Ctenopharyngodon idellus) by utilizing suppression subtractive hybridization (SSH) and rapid amplification of cDNA ends (RACE). The grass carp T2BP (GT2BP) gene contains an open reading frame of 579 nucleotide(s) (nt), encoding 193 amino acids, with 23 nt 5'-untranslated region and a long 3'-untranslated region of 434 nt including poly (A), 1 AUUUA motif and 4 AUUUUA motifs. No signal peptide has been detected in the predicted GT2BP, but a characteristic forkhead associated domain is present. The GT2BP mRNA shares 83% identity with the zebrafish DNA sequence, and they both have no introns in the genomic DNA. The putative transcription factor binding sites of GT2BP include two C/EBP alpha binding sites, and one c-Jun binding, one AP-1 binding, and one nuclear factor kappaB (NF kappaB) binding sites. Southern blot analysis revealed that the GT2BP was a single-copy gene. Individual difference was observed in GT2BP expression in examined organs of healthy grass carp. However, the expression of GT2BP in all examined organs in a fish with the highest copepod infection level and the significantly higher expression level in spleen and liver in infected fish may indicate its up-regulation with the parasite infection.

Published

2005