ABSTRACT
ABSTRACT Chromosome-specific probes have been widely used in molecular cytogenetics, being obtained with different methods. In this study, a reproducible protocol for construction of chromosome-specific probes is proposed which associates in situ amplification (PRINS), micromanipulation and degenerate oligonucleotide-primed PCR (DOP-PCR). Human lymphocyte cultures were used to obtain metaphases from male and female individuals. The chromosomes were amplified via PRINS, and subcentromeric fragments of the X chromosome were microdissected using microneedles coupled to a phase contrast microscope. The fragments were amplified by DOP-PCR and labeled with tetramethyl-rhodamine-5-dUTP. The probes were used in fluorescent in situ hybridization (FISH) procedure to highlight these specific regions in the metaphases. The results show one fluorescent red spot in male and two in female X chromosomes and interphase nuclei.
Subject(s)
Humans , Polymerase Chain Reaction/methods , DNA Primers/genetics , Primed In Situ Labeling/methods , Cytogenetic Analysis/methods , DNA Probes/genetics , Reproducibility of Results , In Situ Hybridization, Fluorescence/methods , Chromosomes, Human, X/genetics , Microdissection/methodsABSTRACT
The diagnosis of any pathology is fundamentally based on the microscopic structure of cells and tissues and this remains as the standard by which all other diagnostic tests are measured. In this era, the pathologists are relying on the examination of tissue section stained by histochemical means and it is supported by the advanced immunological, biochemical and molecular techniques. This review will provide the information about one of the way that can be followed to unravel the molecular mechanism in spotting the disease process. Technologies used to study the cellular process are same for the normal and the abnormal cell. Experimental strategy briefed here is also applicable for both. The cellular process can be studied either from protein to gene or from gene to protein. Earlier days biochemical analysis (isolation of protein, protein sequencing) was separate and genetic analysis (genomic mapping) was separate. But now with advent of recombinant DNA technology it is possible to have a link between the biochemical and genetic analysis. Intermediary step of development of oligonucleotide synthesis, complementary DNA probe and cloning has revolutionized the research process. Identified gene can be compared with the normal gene by comparative genomics or expressed proteins by expression proteomics.
Subject(s)
DNA Probes/genetics , Gene Expression Profiling , Genes/genetics , Genetic Variation/analysis , Proteins/genetics , Review Literature as TopicABSTRACT
Alpha-thalassemia is the most common inherited disorder of hemoglobin synthesis. Genomic deletions involving the alpha-globin gene cluster on chromosome 16p13.3 are the most frequent molecular causes of the disease. Although common deletions can be detected by a single multiplex gap-PCR, the rare and novel deletions depend on more laborious techniques for their identification. The multiplex ligation-dependent probe amplification (MLPA) technique has recently been used for this purpose and was successfully used in the present study to detect the molecular alterations responsible for the alpha-thalassemic phenotypes in 8 unrelated individuals (3 males and 5 females; age, 4 months to 30 years) in whom the molecular basis of the disease could not be determined by conventional methods. A total of 44 probe pairs were used for MLPA, covering approximately 800 kb from the telomere to the MSLN gene in the 16p13.3 region. Eight deletions were detected. Four of these varied in size from 240 to 720 kb and affected a large region including the entire alpha-globin gene cluster and its upstream regulatory element (alpha-MRE), while the other four varied in size from 0.4 to 100 kb and were limited to a region containing this element. This study is the first in Brazil to use the MLPA method to determine the molecular basis of alpha-thalassemia. The variety of rearrangements identified highlights the need to investigate all cases presenting microcytosis and hypochromia, but without iron deficiency or elevated hemoglobin A2 levels and suggests that these rearrangements may be more frequent in our population than previously estimated.
Subject(s)
Adolescent , Adult , Child, Preschool , Female , Humans , Infant , Male , Young Adult , DNA Probes/genetics , Multiplex Polymerase Chain Reaction , Mutation/genetics , alpha-Globins/genetics , alpha-Thalassemia/genetics , Brazil , Genotype , Pedigree , Phenotype , Sensitivity and Specificity , alpha-Thalassemia/diagnosisABSTRACT
LWD is associated to SHOX haploinsufficiency, in most cases, due to gene deletion. Generally FISH and microsatellite analysis are used to identify SHOX deletion. MLPA is a new method of detecting gene copy variation, allowing simultaneous analysis of several regions. Here we describe the presence of a SHOX intragenic deletion in a family with LWD, analyzed through different methodologies. Genomic DNA of 11 subjects from one family were studied by microsatellite analysis, direct sequencing and MLPA. FISH was performed in two affected individuals. Microsatellite analysis showed that all affected members shared the same haplotype suggesting the involvement of SHOX. MLPA detected an intragenic deletion involving exons IV-VIa, which was not detected by FISH and microsatellite analysis. In conclusion, the MLPA technique was proved to be the best solution on detecting this small deletion, it has the advantage of being less laborious also allowing the analysis of several regions simultaneously.
Discondrosteose de Léri-Weill (DLW) está associada à haploinsuficiência do gene SHOX resultante, principalmente, de deleções. Geralmente, o FISH e a análise de microssatélites são os métodos utilizados para a identificação destas deleções. MLPA é um novo método para detectar variações do número de cópias gênicas, permitindo uma análise simultânea de várias regiões. Aqui, descrevemos uma pequena deleção intragênica no SHOX em uma família com DLW analisada por diferentes metodologias. DNA genômico de 11 membros de uma família foram estudados por microssatélites, seqüenciamento direto e MLPA. FISH foi realizado em dois indivíduos afetados. Os microssatélites demonstraram que todos os membros afetados apresentavam o mesmo haplotipo, sugerindo o envolvimento do SHOX. MLPA identificou uma deleção intragênica envolvendo os éxons IV-VIa, que não foi detectada pelo FISH e pelos microssatélites. Conclui-se que o MLPA demonstrou melhor resolução para detectar esta pequena deleção, com a vantagem de ser menos trabalhoso e permitir a análise de várias regiões simultaneamente.
Subject(s)
Child , Female , Humans , Male , DNA Probes/genetics , Gene Deletion , Homeodomain Proteins/genetics , Nucleic Acid Amplification Techniques/methods , Osteochondrodysplasias/genetics , Case-Control Studies , Microsatellite Repeats , Pedigree , Sequence Analysis, DNA/methodsABSTRACT
Hereditary hemochromatosis (HH) is a common autosomal disorder of iron metabolism mainly affecting Caucasian populations. Three recurrent disease-associated mutations have been detected in the hemochromatosis gene (HFE): C282Y, H63D, and S65C. Although HH phenotype has been associated with all three mutations, C282Y is considered the most relevant mutation responsible for hemochromatosis. Clinical complications of HH include cirrhosis of the liver, congestive cardiac failure and cardiac arrhythmias, endocrine pancreatic disease, which can be prevented by early diagnosis and treatment. Therefore, a reliable genotyping method is required for presymptomatic diagnosis. We describe the simultaneous detection of the C282Y, H63D and S65C mutations in the hemochromatosis gene by real-time PCR followed by melting curve analysis using fluorescence resonance energy transfer (FRET) probes. The acceptor fluorophore may be replaced by a quencher, increasing multiplex possibilities. Real-time PCR results were compared to the results of sequencing and conventional PCR followed by restriction digestion and detection by agarose gel electrophoresis (PCR-RFLP). Genotypes from 80 individuals obtained both by the conventional PCR-RFLP method and quenched-FRET real-time PCR were in full agreement. Sequencing also confirmed the results obtained by the new method, which proved to be an accurate, rapid and cost-effective diagnostic assay. Our findings demonstrate the usefulness of real-time PCR for the simultaneous detection of mutations in the HFE gene, which allows a reduction of a significant amount of time in sample processing compared to the PCR-RFLP method, eliminates the use of toxic reagents, reduces the risk of contamination in the laboratory, and enables full process automation.
Subject(s)
Adolescent , Adult , Aged , Child , Female , Humans , Male , Middle Aged , Young Adult , Hemochromatosis/genetics , Histocompatibility Antigens Class I/genetics , Mutation/genetics , DNA Probes/genetics , Fluorescence Resonance Energy Transfer , Genotype , Membrane Proteins/genetics , Phenotype , Polymorphism, Restriction Fragment Length , Polymorphism, Single Nucleotide , Polymerase Chain Reaction/methods , Reproducibility of Results , Young AdultABSTRACT
Leptospirosis, a major health problem worldwide, is known to be endemic in the northeastern part of Thailand with the risk of infection by exposure to pathogenic Leptospira in contaminated aquatic environment. A method based on PCR-hybridization detection of pathogenic Leptospira in water was established. The method included filtration of water sample through membrane filters of two pore sizes, DNA extraction from filters using a guanidine thiocyanate extraction method, a duplex-PCR assay with two primer pairs, and hybridization with a synthetic LipL32 DNA probe. The duplex-PCR allowed detection of two products of 279 bp for LipL32 gene and 430 bp for 16S rRNA gene. In water samples artificially seeded with serovar bratislava, at least 10(3) cells could be analyzed by PCR-agarose gel electrophoresis and 1-10 cells by PCR-Southern blot hybridization. The protocol was applied to the detection of pathogenic Leptospira in environmental waters collected from endemic areas in the northeast region of Thailand. Of 100 water samples analyzed, 23 samples were positive for pathogenic Leptospira with PCR performed with Southern blot hybridization only, but none was detected by PCR-agarose gel-electrophoresis. However, PCR performed with the chemiluminescent LipL32 probe using the Fluorescein ULS labeling facilitated the detection of low numbers of pathogenic Leptospira in water. This method should prove useful for monitoring of pathogenic Leptospira pollution in environmental waters, and has the potential to become a valuable tool to the surveillance of leptospirosis in endemic areas, thus leading to enhanced public health protection.
Subject(s)
Animals , Blotting, Southern , DNA/isolation & purification , DNA Probes/genetics , Electrophoresis, Agar Gel , Environmental Monitoring/statistics & numerical data , Fresh Water/parasitology , Leptospira/genetics , Polymerase Chain Reaction , ThailandABSTRACT
Homologies of minicircle kDNA of 27 Mexican stocks were studied by cross-hybridization with four kDNA probes derived from three reference stocks belonging to groups Trypanosoma cruzi I (SO34 cl4 and Silvio) and T. cruzi II (MN) and one Mexican stock. High homologies were only observed with Silvio (six stocks) and Mexican probes (11 stocks). After 30 min exposure (low homology) additional stocks were recognized with SO34 cl4 (three stocks) and Silvio (six stocks) probes; with the Mexican probe only five stocks remained non-reactive. All the stocks were typed by isoenzyme (16 loci) and Mexican stocks belonged to T. cruzi I. Hybridization patterns were not strictly correlated with the observed clustering and cross-hybridization of kDNA minicircles is not available to distinct Mexican stocks.
Subject(s)
Animals , DNA, Kinetoplast/analysis , DNA, Protozoan/genetics , Sequence Homology, Nucleic Acid , Trypanosoma cruzi/genetics , DNA Probes/genetics , Insect Vectors/parasitology , Mexico , Nucleic Acid Hybridization , Polymerase Chain ReactionABSTRACT
When the first group of DNA puffs is active in the salivary gland regions S1 and S3 of Bradysia hygida larvae, there is a large increase in the production and secretion of new salivary proteins demonstrable by [3H]-Leu incorporation. The present study shows that protein separation by SDS-PAGE and detection by fluorography demonstrated that polypeptides range in molecular mass from about 23 to 100 kDa. Furthermore, these proteins were synthesized mainly in the S1 and S3 salivary gland regions where the DNA puffs C7,C5,C4 and B10 are conspicuous, while in the S2 region protein synthesis was very low. Others have shown that the extent of amplification for DNA sequences that code for mRNA in the DNA puffs C4 and B10 was about 22 and 10 times, respectively. The present data for this group of DNA puffs are consistent with the proposition that gene amplification is necessary to provide some cells with additional gene copies for the production of massive amounts of proteins within a short period of time (Spradling AC and Mahowald AP (1980) Proccedings of the National Academy of Sciences, USA, 77: 1096-1100).
Subject(s)
Animals , Female , Diptera/genetics , DNA Probes/genetics , Gene Amplification/genetics , In Vitro Techniques , Peptides/biosynthesis , Salivary Glands/physiology , Saliva/chemistry , Electrophoresis , Electrophoresis, Polyacrylamide Gel , RadioactivityABSTRACT
The Salmonella specific DNA fragment from genomic DNA of S. typhimurium ATCC 23566 was cloned in E. coli and successfully used as a digoxigenin labeled probe for detecting the presence of Salmonella serotypes in both artificially contaminated food and natural contaminated food samples.
Subject(s)
Cloning, Molecular , Colony Count, Microbial , DNA Probes/genetics , DNA, Bacterial/genetics , Digoxigenin , Escherichia coli/genetics , Food Microbiology , Humans , Immunoblotting , Salmonella Food Poisoning/microbiology , Salmonella typhimurium/geneticsABSTRACT
Laminin is a major glycoprotein specific to basement membranes. Hepatocellular carcinoma tissue synthesize and secrete abundant laminin. By DNA-protein interaction assays, we have identified nuclear factors specific to hepatocellular carcinoma cells. The comparison of nuclear factor binding by Southwestern analysis with B1 and B2 laminin promoters revealed different patterns of nuclear factor binding in different cells types. In hepatocellular carcinoma, HepG2 cells, a specific pair of proteins (P105 and P98) consisting of 105 and 98 kDa were identified as common nuclear factors for both B1 and B2 laminin promoters, while in completely diverse human glioma cells (U251), various different and greater number of nuclear proteins ranging from 212 to 68 kDa were detected to interact separately with laminin B1 and B2 genes.
Subject(s)
Base Sequence , Carcinoma, Hepatocellular/genetics , DNA Probes/genetics , Humans , Laminin/genetics , Nuclear Proteins/chemistry , Promoter Regions, Genetic , Protein Binding , Tumor Cells, CulturedABSTRACT
El operon lac de escherichia coli, es un sistema genético que ha sido útil para elucidar principios básicos de variación y expresión genética y para la construcción de cepas microbianas de proyección industrial. En este contexto, hemos derivado por clonación in vivo, un plasmidio de amplio rango de hospedero (pUCV3), que contiene los genes lac de e. coli, los cuales pueden ser ahora transmitidos con facilidad a todos los microorganismos capaces de incorporar replicones IncPa, grupo de compatibilidad al que pertenece pUCV3. Como ejemplo este plasmidio fue transmitido a bacterias marinas y a cytophaga johsonae, microorganismos en los cuales se apreció la expresión regulada del sistema lac. En consecuencia, pUCV3, puede ser usado como sonda para evaluar en comportamiento del operón lac en variados transfondos genéticos microbianos
Subject(s)
DNA Probes/genetics , Escherichia coli/genetics , Lac Operon/genetics , Cloning, Molecular , Plasmids/geneticsABSTRACT
The present study describes a nonisotopic DNA-DNA hybridization assay for the detection of enterotoxigenic Escherichia coli (ETEC) in which the probes were labelled with the hapten molecule digoxigenin and after hybridization, DNA hybrids were detected by antidigoxigenin alkaline phosphatase conjugate. A blinded study carried out on a battery of enterotoxigenic and nonenterotoxigenic Esch. coli by dig-probe hybridization assay were compared with the results of a radiolabelled toxin gene probe hybridization assay (performed earlier). The three digoxigenin labelled probes gave a 100 per cent specificity and sensitivities of 95.45, 100 and 100 per cent for LT, STh and STp respectively. These results were comparable to those with the radioactive probes.