Your search keyword '"G, Comach"' showing total 7 results

1. [Cloning alphavirus and flavivirus sequences for use as positive controls in molecular diagnostics].

Author

Camacho D, Reyes J, Franco L, Comach G, and Ferrer E

Subjects

Dengue, Humans, Zika Virus Infection, Chikungunya virus genetics, Dengue Virus genetics, Flavivirus genetics, Pathology, Molecular, Zika Virus genetics

Abstract

The purpose of the study was to obtain a positive control to validate molecular techniques (reverse transcription- polymerase chain reaction [RT-PCR]) used in the diagnosis and research of viral infections. From strains of Chikungunya virus (CHIKV), Zika virus, and Dengue virus (DENV-1, DENV-2, DENV- 3, and DENV-4) viral RNAs were extracted to obtain complementary DNA using RT-PCR from the nsP4 (CHIKV), NS5 (Zika virus), C/prM-M, and 5'UTR-C (DENV-1, DENV-2, DENV-3, DENV-4) sequences, which were cloned into pGEM®-T Easy. Cloning was confirmed through colony PCR, from which plasmid DNA was extracted for fragment cloning verification. Cloning of cDNA corresponding to nsP4, NS5, C/prM-M, and 5'UTR-C of the different viral agents was achieved. In conclusion, recombinant plasmids were obtained with each of the sequences specified for further assessment as positive controls in molecular techniques in an effort to avoid the use of cell cultures, which can be costly, time-consuming, and potentially dangerous.

Published

2016

2. [Laboratory diagnosis of dengue virus infections in Aragua State, Venezuela: October 1997-December 1998].

Author

Camacho DE, Alvarez M, Rodríguez-Henríquez F, de Quintana M, Soler M, Chiarello A, Sierra G, and Comach G

Subjects

Dengue blood, Dengue epidemiology, Dengue Virus classification, Dengue Virus genetics, Enzyme-Linked Immunosorbent Assay, Hemagglutinins, Viral blood, Humans, Immunoglobulin M blood, RNA, Viral analysis, RNA, Viral genetics, Reverse Transcriptase Polymerase Chain Reaction, Serologic Tests, Serotyping, Severe Dengue blood, Severe Dengue diagnosis, Severe Dengue epidemiology, Venezuela epidemiology, Dengue diagnosis, Dengue Virus isolation & purification

Abstract

The efficacy of a proactive dengue surveillance system to predict epidemics depends on the laboratory diagnostic capacity for an early detection of virus circulation. This study shows the results of the dengue virologic and serologic surveillance accomplished in Aragua State (Venezuela) from October 1997 to December 1998. Five hundred and forty seven sera from suspected dengue patients were tested using the techniques of Virus Isolation and Immunofluorescence Serotyping (VIIS), Reverse Transcriptase-Polymerase Chain Reaction (RT-PCR), Anti-dengue IgM Capture Enzyme Immunoassay (MAC-ELISA) and Haemagglutination Inhibition test (HI). Of the tested sera, 97.4% resulted positive to at least one technique; of these, 60.4% were classified as confirmed cases (virologically positives) and 39.6% as probable cases (virologically negatives/serologically positives). Though the majority of positive cases occurred during the 1997 and 1998 epidemic periods, the gradual increase of the seropositive rates between both periods suggested the incoming 1998 outbreak. Den-1 (51.2%), Den-2 (37.9%) and Den-4 (10.6%) infected patients were detected as well as one dual infection of Den-2 and Den-4 (0.3%). Dengue hyperendemicity (co-circulation of Den-1, Den-2 and Den-4) in Aragua State was confirmed together with the detection of few cases (6.5%) of Dengue Hemorrhagic Fever/Dengue Shock Syndrome cases (HF/DSS); 38.1% of these cases occurred in patients with secondary infections. The high percentage (85.7%) of DHF/DSS cases infected by Den-2 virus supports the reported virulence of this serotype.

Published

2003

3. [Biological behavior of 3 strains of the dengue-2 virus in 2 cell lines of mosquitoes].

Author

Morier L, Camacho DE, Guzmán MG, Alvarez M, Rodríguez R, and Comach G

Subjects

Animals, Cell Line virology, Aedes virology, Dengue Virus classification, Dengue Virus physiology

Abstract

Strains A-15 (isolated in Cuba, 1981), Jamaica (isolated in Jamaica, 1981) and Nueva Guinea "C" (standard) from dengue-2 virus were compared according to the time of appearance of the cytopathic effect (CPE), to the time of appearance of specific fluorescence and to the kynetics of viral multiplication on being innoculated in the cell lines AP-61 (Aedes pseudoscutellaris) and C6/36 HT (Aedes albopictus). The results showed that the CPE of highest intensity and earliest appearance was for A-15, followed by Jamaica and Nueva Guinea "C" (NGC). AP-61 seems to favor the CPE of Jamaica with respect to that of the same strain in C6/36 HT. The fluorescence was earlier for Jamaica and A-15 and more intensive for the latter, whereas NGC manifested late. This behaviour was similar in the 2 cellular systems. The greatest titres during the kinetics of viral multiplication were obtained from A-15 in both lines, although in AP-61 they tend to be equal from the 4th day on. The strain A-15 showed a particular behaviour of these biological properties on comparing them with the other strains under study, which may be related to changes found in its neucleotide sequence.

Published

2000

4. [Ultrastructural identification of Ehrlichia sp in an experimentally infected dog in Venezuela].

Author

Gutiérrez N, Martínez M, Arraga-Alvarado C, Bretaña A, Pacheco I, and Comach G

Subjects

Animals, Cytoplasmic Granules ultrastructure, Dogs, Ehrlichia isolation & purification, Ehrlichiosis blood, Ehrlichiosis diagnosis, Ehrlichiosis microbiology, Female, Hematocrit, Inclusion Bodies ultrastructure, Male, Vacuoles ultrastructure, Venezuela, Blood microbiology, Ehrlichia ultrastructure, Microscopy, Electron

Abstract

This study is the first report made in Venezuela concerning the ultrastructural characteristics of Ehrlichia sp in mononuclear blood cells from an experimentally infected dog. The animal developed clinical manifestations characteristic of the infection, and typical intracitoplasmic inclusion bodies were clearly seen in blood smears stained with modified Giemsa examined by light microscopy. Microorganisms were visualized by transmission electron microscopy. The cytoplasmic inclusions, consisted of membrane-lined vacuole-containing elementary bodies. The organisms were extremely pleomorphic. Elementary bodies were surrounded by two distinct membranes and each was constituted by electro-dense granules. These findings corresponded to the described electron microscopy morphology which characterizes the Ehrlichia genus.

Published

1999

5. [Study of various biological properties of 3 strains of dengue 2 with differences in their nucleotide sequences].

Author

Camacho DE, Guzmán MG, Morier L, Alvarez M, Rodríguez R, and Comach G

Subjects

Animals, Base Sequence, Mice, DNA, Viral analysis, Dengue Virus genetics

Abstract

Some biological properties of Dengue-2 strains such as A-15 (isolated in Cuba in 1981); Jamaica (isolated in Jamaica in 1981) and New Guinea "C" (NG"C") standard strain differing in their nucleotide sequences were studied. The results showed that the cytopathic effect in C6/36 HT cell line occurred earlier in A-15 strain and that fluorescence was first detected in Jamaica and A-15 strains. This seems to indicate that rapid detection of strains does not have any relation to neither their history of passage nor the original isolation system. A-15 and NG"C" strains exhibited an heterogeneous pattern formed by big and small plaques but average size of plaques in NG"C" was lower whereas Jamaica showed only small plaques. The most neurovirulent strain in mice was NG"G" followed by A-15 whereas Jamaica was not neurovirulent at all. These results indicate that A-15 has a different biological behaviour which is probably due to intrinsic differences. It should be taken into account that 7 amino acid changes were found in the envelope protein which may have affected the expression of some biological properties.

Published

1999

6. [Immunoenzyme assay using micro Dot on nitrocellulose (Dot-ELISA) in the diagnosis of Chagas' disease. I. Comparative study of 2 antigenic preparations of Trypanosoma cruzi].

Author

De Hubsch RM, Chiechie N, Comach G, Rangel Aldao R, and Gusmao RD

Subjects

Adult, Animals, Antibodies, Protozoan immunology, Female, Humans, Male, Middle Aged, Serologic Tests, Antigens, Protozoan immunology, Chagas Disease diagnosis, Enzyme-Linked Immunosorbent Assay methods, Trypanosoma cruzi immunology

Abstract

Using the Dot-ELISA technique, two antigenic preparations of Trypanosoma cruzi epimastigote forms have been compared for the diagnosis of Chagas' disease: (1) The cytoplasmic fraction (cytoplasmic antigen) and (2) whole formalin fixed epimastigotes (integral antigen). There was been used sera from 95 chagasic patients with chronic cardiomyopathy, positive conventional serology and either positive or negative xenodiagnosis; 74 subjects with negative conventional serology, and either clinically normal or presenting cardiomyopathy; 74 patients with different diseases including syphilis, toxoplasmosis, leishmaniasis or autoantibodies such as rheumatoid factor and antinuclear antibodies. By defining the diagnostic titers (cut off): 1:512 for cytoplasmic antigen and 1:128 for the integral antigen, a sensitivity of 100% has been obtained with both antigenic preparations, being the specificity of 96% for the former and 100% for the latter when leishmaniasis sera were not included. A comparative study with conventional serology was carried out using 147 sera from a Laboratory of Chagas' diagnosis; Dot-ELISA with cytoplasmic antigen showed co-positivity index of 1.0, co-negativity 0.989 and efficiency of 0.993, and Dot-ELISA with integral antigen 1.0, 0.979 and 0.986 respectively. According to this evaluation, Dot-ELISA using whole formalin fixed epimastigotes might be a practical alternative for the serological diagnosis of Chagas' disease.

Published

1988

7. [The Dot immunoenzymatic assay on nitrocellulose (Dot-ELISA) in the diagnosis of Chagas disease. II. Seroepidemiologic study in 4 rural communities of Venezuela].

Author

de Hubsch RM, Chiechie N, Comach G, Aldao RR, and Gusmao RD

Subjects

Adolescent, Adult, Chagas Disease epidemiology, Child, Child, Preschool, Fluorescent Antibody Technique, Hemagglutination Tests, Humans, Infant, Predictive Value of Tests, Rural Health, Venezuela epidemiology, Chagas Disease diagnosis, Immunoblotting

Abstract

A survey of human Trypanosoma cruzi infection in four rural communities of two Venezuelan states with different epidemiological Chagas' disease situations was carried out using the Dot-ELISA and conventional serology. In the two hamlets of Zulia state, no seropositives were found in the under-15 age group whereas seropositivity in the over-15 group was 15.6%. In Cojedes state, the two hamlets studied exhibited a seropositivity of 8.9% in the under-15 group and 51.6% in the over-15 group. Upon comparison with conventional methods, Dot-ELISA evidenced high co-positivity, co-negativity and efficiency indexes. In the samples taken from Zulia, the predictive value of the test was 66% and 60% for cytoplasmatic and integral antigens, respectively; with the Cojedes samples, 100% and 95%. The results suggest that Dot-ELISA could be a practical alternative for seroepidemiological Chagas' disease studies in underdeveloped regions.

Published

1989