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2. Histologic, Serologic, and Molecular Analysis of Persistent Ehrlichiosis in a Murine Model

Author

David H. Walker, Hui-Min Feng, Jere W. McBride, Gary Wen, and Juan P. Olano

Subjects
DNA, Bacterial, Human monocytotropic ehrlichiosis, Immunoblotting, Ehrlichia, Spleen, Polymerase Chain Reaction, Pathology and Forensic Medicine, Serology, law.invention, Immunoenzyme Techniques, Mice, Mice, Inbred AKR, law, medicine, Animals, Ehrlichia chaffeensis, Fluorescent Antibody Technique, Indirect, Lung, Polymerase chain reaction, Ehrlichia muris, Antigens, Bacterial, biology, Ehrlichiosis, biology.organism_classification, medicine.disease, Virology, Mice, Inbred C57BL, Disease Models, Animal, medicine.anatomical_structure, Liver, Ehrlichiosis (canine), Animal Model
Abstract

Human monocytotropic ehrlichiosis caused by Ehrlichia chaffeensis was reported in 1987. An animal model to study acute fatal ehrlichiosis in mice that has been developed closely resembles the fatal form of human monocytotropic ehrlichiosis. However, animal models for persistent infection in the genus Ehrlichia in immunocompetent mice have not been characterized. We report the histopathological progression of Ehrlichia muris infection in immunocompetent mice (AKR and C57BL/6 strains) correlated with their antibody response determined by indirect immunofluorescence and Western immunoblotting, and the distribution and quantity of the ehrlichial load by immunohistochemistry, polymerase chain reaction (PCR), and real-time PCR in lungs, liver, and spleen. Mild to moderate correlation was observed between histopathological grading in these organs and relative ehrlichial loads. The highest ehrlichial loads were present between days 4 and 14 after infection. E. muris was detected in tissues examined up to 150 days after infection by real-time PCR. Analysis of the serological response revealed several immunodominant antigens, including 200-, 180-, 100-, 73/75-, 45-, and 28-kd proteins. In conclusion, we have provided for the first time a complete histopathological, serological, immunohistochemical, and quantitative analysis of an animal model for the study of persistent ehrlichial infection.

Published
2004
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3. GLUT-3 expression in human skeletal muscle

Author

Gary Wen, Charles A. Stuart, S. David Hudnall, Bi Hung Peng, Gerald A. Campbell, and Vsevolod L. Popov

Subjects
Adult, Muscle tissue, endocrine system, medicine.medical_specialty, Monosaccharide Transport Proteins, endocrine system diseases, Physiology, Endocrinology, Diabetes and Metabolism, Fluorescent Antibody Technique, Nerve Tissue Proteins, Biology, Myelin, Physiology (medical), Internal medicine, medicine, Humans, Myocyte, Peripheral Nerves, RNA, Messenger, Axon, Muscle, Skeletal, In Situ Hybridization, NADH Tetrazolium Reductase, Muscle biopsy, Glucose Transporter Type 3, medicine.diagnostic_test, nutritional and metabolic diseases, Skeletal muscle, Immunohistochemistry, carbohydrates (lipids), Sarcoplasmic Reticulum, Muscle Fibers, Slow-Twitch, Spinal Nerves, Endocrinology, medicine.anatomical_structure, Peripheral nervous system, Muscle Fibers, Fast-Twitch, Perineurium, hormones, hormone substitutes, and hormone antagonists
Abstract

Muscle biopsy homogenates contain GLUT-3 mRNA and protein. Before these studies, it was unclear where GLUT-3 was located in muscle tissue. In situ hybridization using a midmolecule probe demonstrated GLUT-3 within all muscle fibers. Fluorescent-tagged antibody reacting with affinity-purified antibody directed at the carboxy-terminus demonstrated GLUT-3 protein in all fibers. Slow-twitch muscle fibers, identified by NADH-tetrazolium reductase staining, possessed more GLUT-3 protein than fast-twitch fibers. Electron microscopy using affinity-purified primary antibody and gold particle-tagged second antibody showed that the majority of GLUT-3 was in association with triads and transverse tubules inside the fiber. Strong GLUT-3 signals were seen in association with the few nerves that traversed muscle sections. Electron microscopic evaluation of human peripheral nerve demonstrated GLUT-3 within the axon, with many of the particles related to mitochondria. GLUT-3 protein was found in myelin but not in Schwann cells. GLUT-1 protein was not present in nerve cells, axons, myelin, or Schwann cells but was seen at the surface of the peripheral nerve in the perineurium. These studies demonstrated that GLUT-3 mRNA and protein are expressed throughout normal human skeletal muscle, but the protein is predominantly found in the triads of slow-twitch muscle fibers.

Published
2000
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4. GLUT3 protein and mRNA in autopsy muscle specimens

Author

Gary Wen, Charles A. Stuart, and Jie Jiang

Subjects
medicine.medical_specialty, Time Factors, Monosaccharide Transport Proteins, Endocrinology, Diabetes and Metabolism, Immunoblotting, Nerve Tissue Proteins, Autopsy, chemistry.chemical_compound, Endocrinology, Glyceraldehyde, Internal medicine, Cadaver, medicine, Humans, RNA, Messenger, Muscle, Skeletal, Glyceraldehyde 3-phosphate dehydrogenase, Messenger RNA, Glucose Transporter Type 3, biology, RNA, Skeletal muscle, medicine.anatomical_structure, chemistry, Postmortem Changes, biology.protein, GLUT4, GLUT3
Abstract

GLUT3 is expressed in rat muscle, but this glucose transporter protein has not been identified previously in adult human skeletal muscle. We quantified the rapidity of disappearance of mRNA and protein from human skeletal muscle at room temperature and at 4 degrees C. Fifty percent of the immunologically detectable GLUT3 protein disappeared by 1 hour at 20 degrees C and by 2 hours at 4 degrees C. mRNA for GLUT3 was decreased 50% by 2.2 hours at 20 degrees C and by 24 hours at 4 degrees C. Half of the measurable mRNAs for GLUT4, glyceraldehyde 3-phosphate dehydrogenase (GAPDH), alpha-actin, and beta-myosin disappeared by 0.8 to 2.1 hours at 20 degrees C and by 5.0 to 16.6 hours at 4 degrees C. Previous conclusions that GLUT3 is not expressed in human muscle were likely drawn because of artifacts related to degradation of GLUT3 protein in the specimens prior to study. Because of the rapid degradation of protein and mRNA, autopsy specimens of muscle must be obtained within 6 hours of death, and even then, protein and mRNA data will likely dramatically underestimate their expression in fresh muscle. Some previously published conclusions and recommendations regarding autopsy specimens are not stringent enough to consistently yield useful protein and mRNA.

Published
1999
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5. Interaction of human gallbladder mucin with calcium hydroxyapatite: Binding studies and the effect on hydroxyapatite formation*1

Author

Roger S. Crowther, Roger D. Soloway, Sui-Min Qiu, Gary Wen, and Julie Wen

Subjects
chemistry.chemical_classification, Hepatology, medicine.diagnostic_test, Proteolysis, Mucin, chemistry.chemical_element, Calcium, Phosphate, Glycopeptide, In vitro, Amino acid, chemistry.chemical_compound, stomatognathic system, chemistry, Biochemistry, In vivo, medicine
Abstract

Calcium hydroxyapatite (HAP) crystals formed in vitro in the presence of polymeric human gallbladder mucin (1.0 mg/mL) were smaller (0.75 ± 0.39 μm) than control crystals (7.86 ± 2.76 μm), but the mucin did not affect the kinetics of crystal formation or alter the amount of mineral phase present at equilibrium. In contrast, glycopeptide subunits produced by proteolysis of the native mucin had no effect on HAP crystal size. Both native mucin and glycopeptides bound to mature HAP crystals, but the glycopeptides were much more readily displaced by phosphate ions. Therefore, in experiments where HAP was being formed, the phosphate ions inhibited the interaction of glycopeptides with the nascent HAP. These results indicate that gallbladder mucin may modulate HAP formation in vivo, and that this ability may be altered during pathological states, such as neutrophil infiltration or bacterial colonization, that may cause the release of proteinases capable of digesting mucin.

Published
1995
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7. Early diagnosis of rickettsioses by electrochemiluminscence

Author

Jere W. McBride, Juan P. Olano, Xiaofeng Zhang, and Gary Wen

Subjects
biology, General Neuroscience, Rickettsia Infections, Typhus, Endemic Flea-Borne, Disease, biology.organism_classification, Antibodies, Bacterial, General Biochemistry, Genetics and Molecular Biology, History and Philosophy of Science, Polyclonal antibodies, Biotinylation, Rickettsia typhi, Immunology, Luminescent Measurements, biology.protein, Electrochemistry, Animals, Humans, Rabbits, Antibody
Abstract

The diagnosis of acute rickettsioses during the acute phase of the disease is challenging. We present preliminary evidence that antigen-capture using streptavidin-coated magnetic beads with biotinylated anti-rickettsia typhi rabbit polyclonal antibodies followed by electrochemiluminescent detection with ruthenylated antibodies of the same specificity could be used for the diagnosis of rickettsial diseases in the acute phase.

Published
2006

9. Altered GLUT1 and GLUT3 gene expression and subcellular redistribution of GLUT4: protein in muscle from patients with acanthosis nigricans and severe insulin resistance

Author

Mary E. Williamson, Jie Jiang, Charles A. Stuart, Manubai Nagamani, Steven J. Blackwell, Charles R. Gilkison, Arny A. Ferrando, and Gary Wen

Subjects
Adult, Male, medicine.medical_specialty, Monosaccharide Transport Proteins, Endocrinology, Diabetes and Metabolism, Glucose uptake, medicine.medical_treatment, Muscle Proteins, Nerve Tissue Proteins, Endocrinology, Insulin resistance, Internal medicine, medicine, Myocyte, Humans, Acanthosis Nigricans, Muscle, Skeletal, Glucose Transporter Type 1, Glucose Transporter Type 4, biology, Glucose Transporter Type 3, Insulin, Glucose transporter, nutritional and metabolic diseases, medicine.disease, Gene Expression Regulation, biology.protein, GLUT1, Female, Insulin Resistance, hormones, hormone substitutes, and hormone antagonists, GLUT4, GLUT3
Abstract

Multiple isoforms of glucose transporters are found in muscle, the tissue that normally accounts for 85% of insulin-stimulated glucose uptake. Glucose uptake into muscle cells in the fasting state is mediated primarily by GLUT1 and GLUT3 glucose transporters, whereas postprandial (insulin-stimulated) and exercise-related increments in muscle glucose uptake are mediated primarily by GLUT4. To determine if glucose transporters are abnormally expressed in muscle from insulin-resistant subjects, muscle samples were obtained from 10 normal subjects and 6 obese, nondiabetic subjects with severe insulin resistance and acanthosis nigricans. Both GLUT4 total protein and mRNA were normal in the insulin-resistant subjects. Muscle GLUT3 protein and mRNA were lower than controls by 62% and 71%, respectively. GLUT1 mRNA was twice normal, whereas GLUT1 protein content was not significantly increased. GLUT4 protein was markedly redistributed to the muscle plasma membrane in subjects with severe insulin resistance compared with normals (92% v 40% GLUT4 in plasma membrane-enriched fractions, P

Published
2001

10. Comparison of GLUT1, GLUT3, and GLUT4 mRNA and the subcellular distribution of their proteins in normal human muscle

Author

W. Clay Gustafson, Gary Wen, Charles A. Stuart, and E. Aubrey Thompson

Subjects
Adult, Male, medicine.medical_specialty, Monosaccharide Transport Proteins, Endocrinology, Diabetes and Metabolism, Glucose uptake, Nerve Tissue Proteins, Endocrinology, Reference Values, Internal medicine, medicine, Humans, RNA, Messenger, Muscle, Skeletal, Glucose Transporter Type 2, Glucose Transporter Type 1, biology, Glucose Transporter Type 3, Glucose transporter, Skeletal muscle, Membrane transport, medicine.anatomical_structure, Biochemistry, biology.protein, GLUT1, Female, GLUT4, GLUT3, Subcellular Fractions
Abstract

Basal, "insulin-independent" glucose uptake into skeletal muscle is provided by glucose transporters positioned at the plasma membrane. The relative amount of the three glucose transporters expressed in muscle has not been previously quantified. Using a combination of qualitative and quantitative ribonuclease protection assay (RPA) methods, we found in normal human muscle that GLUT1, GLUT3, and GLUT4 mRNA were expressed at 90 +/- 10, 46 +/- 4, and 156 +/- 12 copies/ng RNA, respectively. Muscle was fractionated by DNase digestion and differential sedimentation into membrane fractions enriched in plasma membranes (PM) or low-density microsomes (LDM). GLUT1 and GLUT4 proteins were distributed 57% to 67% in LDM, whereas GLUT3 protein was at least 88% in the PM-enriched fractions. These data suggest that basal glucose uptake into resting human muscle could be provided in part by each of these three isoforms.

Published
2001

11. Glycochenodeoxycholic acid inhibits calcium phosphate precipitation in vitro by preventing the transformation of amorphous calcium phosphate to calcium hydroxyapatite

Author

Gary Wen, Nan Kang Hong, Roger D. Soloway, Nobuyuki Hirakawa, Roger S. Crowther, and Sui Min Qiu

Subjects
Calcium Phosphates, Taurocholic Acid, Taurine, Bile acid, Fourier Analysis, medicine.drug_class, Inorganic chemistry, chemistry.chemical_element, Black pigment gallstones, General Medicine, Calcium, Phosphate, Taurocholic acid, chemistry.chemical_compound, Durapatite, chemistry, Glycochenodeoxycholic Acid, medicine, Glycochenodeoxycholic acid, Chemical Precipitation, Amorphous calcium phosphate, Hydroxyapatites, Micelles, Research Article
Abstract

Calcium hydroxyapatite can be a significant component of black pigment gallstones. Diverse molecules that bind calcium phosphate inhibit hydroxyapatite precipitation. Because glycine-conjugated bile acids, but not their taurine counterparts, bind calcium phosphate, we studied whether glycochenodeoxycholic acid inhibits calcium hydroxyapatite formation. Glycochenodeoxycholic acid (2 mM) totally inhibited transformation of amorphous calcium phosphate microprecipitates to macroscopic crystalline calcium hydroxyapatite. This inhibition was not mediated by decreased Ca2+ activity. Taurocholic acid (2-12 mM) did not affect hydroxyapatite formation, but antagonized glycochenodeoxycholic acid. Both amorphous and crystalline precipitates contained a surface fraction relatively rich in phosphate. The surface phosphate content was diminish by increasing glycochenodeoxycholic acid concentrations, and this relationship was interpreted as competition between bile acid and HPO4(-4) for binding sites on the calcium phosphate surface. A phosphate-rich crystal surface was associated with rapid transition from amorphous to crystalline states. These results indicate that glycochenodeoxycholic acid prevents transformation of amorphous calcium phosphate to crystalline hydroxyapatite by competitively inhibiting the accumulation of phosphate on the crystal embryo surface.

Published
1991

12. Isolation, chemical composition, and properties of the major mucin component of normal human tracheobronchial secretions

Author

Raoul Carubelli, Franklin J. Myers, Gary Wen, Robert M. Rogers, Frank O. Horton, Owen F. Fox, and Goverdhan P. Sachdev

Subjects
Adult, Electrophoresis, Agar Gel, Male, Chromatography, Mucin, Carbohydrates, Mucins, Bronchi, Fractionation, Chromatography, Ion Exchange, Biochemistry, Fucose, Sialic acid, Molecular Weight, Trachea, chemistry.chemical_compound, chemistry, Glucosamine, Sephadex, Galactosamine, Humans, Amino Acids, Threonine, Glycoproteins
Abstract

The major mucin-type glycoprotein component of normal human tracheobronchial secretions was isolated in electrophoretically homogeneous form, and subjected to physical and chemical characterization. The respiratory mucus, collected from healthy young male volunteers by fiberoptic bronchoscopy, was subjected to initial fractionation on a column of Sephadex G-200. The excluded fraction (mucins) was then chromatographed on a column of Bio-Gel A-15m. Gel electrophoretic examination of the material from the included peak of the latter column indicated the presence of a single mucin component, whereas the pattern of the excluded peak showed two bands, a minor component with the mobility of the included mucin and a major band of slower-migrating, large-molecular-weight mucin. Chemical analysis of the electrophoretically homogeneous mucin present in the included peak showed 73% carbohydrate (galactose, fucose, glucosamine, galactosamine, and sialic acid), 4% sulfate monoester, and 23% protein. The amino acid composition showed a high content (29%) of serine plus threonine, and the presence of carbohydrate chains linked to these hydroxyamino acids was demonstrated by reductive β-elimination. A molecular weight of 69,400 daltons was estimated by sedimentation equilibrium.

Published
1980
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13. Isolation and characterization of glycoproteins from canine tracheal mucus

Author

Goverdhan P. Sachdev, Owen F. Fox, Raoul Carubelli, Gary Wen, Ronald C. Elkins, and Terry Schroeder

Subjects
Alanine, chemistry.chemical_classification, Chromatography, Size-exclusion chromatography, Sulfuric Acids, Biochemistry, Genetics and Molecular Biology (miscellaneous), Fucose, Amino acid, Sialic acid, Molecular Weight, Trachea, Mucus, chemistry.chemical_compound, Dogs, chemistry, Biochemistry, Sephadex, Sialic Acids, Animals, Glycosides, Amino Acids, Threonine, Glycoprotein, Glycoproteins, Hexoses
Abstract

Three homogeneous glycoproteins were isolated from reduced and S-carboxy-methylated canine tracheal pouch mucus by gel filtration and ion-exchange chromatography. Initial fractionation was carried out on Sephadex G-200; chromatography of the excluded Sephadex G-200 fraction on Bio-Gel A-15 m yielded two high molecular weight glycoprotein fractions. Following rechromatography on the same column, the main fraction behaved as an electrophoretically homogeneous high molecular weight (581 600) glycoprotein, with a high carbohydrate content (80%) and a single amino-terminal amino acid (arginine). Ion-exchange chromatography (DEAE-cellulose) of the included Sephadex G-200 fraction yielded two electrophoretically homogeneous glycoproteins of lower molecular weight (20 800 and 24 600, respectively). A single amino-terminal amino acid, glycine and alanine, respectively, was detected for each glycoprotein. Chemical analysis of these three glycoproteins revealed the presence of fucose, galactose, N-acetylgalactosamine, N-acetylglucosamine, N-acetylneuraminic acid and sulfate monoester. The high molecular weight glycoprotein had a higher hexose, sialic acid and sulfate content, per mg of protein, than the low molecular weight glycoproteins. The results of the alkaline borohydride treatment indicated that the majority of the carbohydrate chains of these glycoproteins are linked to the protein core through O-glycosidic bonds involving N-acetylgalactosamine and serine or threonine.

Published
1978
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14. Selective isolation of human plasma low-density lipoprotein particles containing apolipoproteins B and E by use of a monoclonal antibody to apolipoprotein B

Author

Diana M. Lee, Nassrin Dashti, Petar Alaupovic, Hans U. Kloer, Gary Wen, and Eugen Koren

Subjects
Apolipoprotein B, medicine.drug_class, Antigen-Antibody Complex, Monoclonal antibody, Biochemistry, Chromatography, Affinity, Cell Line, chemistry.chemical_compound, Apolipoproteins E, Affinity chromatography, Blood plasma, medicine, Humans, Apolipoproteins B, Chromatography, biology, Cholesterol, Cell Membrane, Antibodies, Monoclonal, Lipoproteins, LDL, Electrophoresis, Microscopy, Electron, chemistry, Receptors, LDL, Low-density lipoprotein, biology.protein, lipids (amino acids, peptides, and proteins), Lipoprotein
Abstract

A monoclonal antibody to human plasma apolipoprotein B was used in a single-step immunoaffinity chromatography procedure to isolate a subpopulation of low-density lipoprotein particles from normolipidemic human plasma. The isolated particles were homogeneous in terms of size (20 nm), flotation coefficient (Sf = 9.5), and electrophoretic mobility (beta band). Their protein moiety consisted of apolipoproteins B and E in a molar ratio close to 2. The lipid moiety consisted of 47.3% cholesterol, 4.7% triglycerides, and 48.0% phospholipids. To indicate its characteristic apolipoprotein composition and hydrated density properties, this family of particles was named LP-B:EL2. In most normolipidemic subjects, LP-B:EL2 particles accounted for less than 10% of the total plasma apolipoprotein B content. The LP-B:EL2 particles bound to the membranes of the human hepatoma HepG2 cells in a specific and saturable manner indicative of receptor-mediated binding. Their binding was significantly higher than that of low-density lipoprotein particles containing only apolipoprotein B.

Published
1987

15. Characterization of a monoclonal antibody that binds equally to all apolipoprotein and lipoprotein forms of human plasma apolipoprotein B. II. Isolation of apolipoprotein B-containing lipoproteins from human plasma

Author

Lawrence E. DeBault, Carolyn Knight-Gibson, Eugen Koren, Petar Alaupovic, and Gary Wen

Subjects
Apolipoprotein B, medicine.drug_class, Lipoproteins, Biophysics, Lipoproteins, VLDL, Monoclonal antibody, Biochemistry, Mice, Endocrinology, Affinity chromatography, Blood plasma, medicine, Animals, Humans, Apolipoproteins B, biology, Chemistry, Antibodies, Monoclonal, Lipoproteins, LDL, Microscopy, Electron, Polyclonal antibodies, biology.protein, lipids (amino acids, peptides, and proteins), Ultracentrifuge, Antibody, Lipoprotein
Abstract

Monoclonal antibody (‘Pan B’ antibody) that binds equally to all major forms of human plasma apolipoprotein B was used in an immunoaffinity chromatography procedure to isolate apolipoprotein B-containing lipoproteins from hyperlipidemic human plasma. These lipoproteins were compared with lipoproteins in native plasma, with lipoproteins isolated by polyclonal antibodies and with lipoproteins isolated by the conventional ultracentrifugational method. Judged by the apolipoprotein and lipid composition, lipoproteins isolated with ‘Pan B’ antibody were virtually identical to those isolated by ultracentrifugation or polyclonal antibodies. Lipoproteins isolated by ‘Pan B’ antibody were comparable in size and shape to the lipoproteins in native plasma and to the lipoproteins isolated by polyclonal antibodies or ultracentrifugation. The immunoaffinity column with monoclonal ‘Pan B’ antibody retained all apolipoprotein B-containing lipoproteins and showed significantly higher capacity than polyclonal immunoaffinity column. The column with the highest capacity allowed the isolation from whole plasma of 0.144 mg of apolipoprotein B per ml of gel in less than 2 h.

Published
1986

16. Chemical Composition of Pathological Human Tracheobronchial Mucus Collected by Fiberoptic Bronchoscopy

Author

Owen F. Fox, Robert M. Rogers, Goverdhan P. Sachdev, Gary Wen, Frank O. Horton, and Raoul Carubelli

Subjects
Chronic bronchitis, Pathology, medicine.medical_specialty, Respiratory mucus, business.industry, Medicine, Fiberoptic bronchoscopy, business, Pathological, Mucus
Abstract

In our previous work with normal tracheobronchial secretions, we have shown that fiberoptic bronchoscopy allows the collection of uncontaminated specimens in amounts suitable for chemical analysis and initial fractionation (Sachdev, et al., 1980). In this communication, we describe the chemical composition and electrophoretic profiles of respiratory mucus collected by fiberoptic bronchoscopy from patients with various chronic pulmonary diseases.

Published
1982
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19. Inventarios de algunos archivos locales de Colombia en los departamentos de Santander, Norte de Santander, Antioquia y Cundinamarca

Author

Gary Wendell Graef

Subjects
archivo general de indias, archivo nacional de colombia, centros eclesiásticos, History (General), D1-2009, Latin America. Spanish America, F1201-3799
Abstract

En los archivos locales de Colombia reposa una riqueza de documentos para el historiador. Ofrecen amplia documentación para estudios regionales, sociales e institucionales de tipo que no se encuentra en el Archivo Nacional de Colombia en Bogotá ni en el Archivo General de Indias en Sevilla, España. Aunque muchos de estos archivos están muy descuidados, uno se sorprende del número de archivos que están en buena condición. Los de los centros eclesiásticos especialmente están muy bien cuidados y están esperando el investigador serio.

Published
1970

20. Apuntes sobre procedimientos de microfilmación en archivos locales

Author

Gary Wendell Graef

Subjects
History (General), D1-2009, Latin America. Spanish America, F1201-3799
Abstract

En los últimos años el trabajo investigativo del historiador, el antropólogo y el sociólogo ha sido aliviado, en buena parte, gracias al uso del microfilm. A un precio módico el investigador puede obtener, hoy día, copias microfilmadas de documentos y libros de- positados en las más importantes bibliotecas del mundo. Sin embargo, los investigadores, hasta ahora, se han mostrado reticentes a tomar ellos mismos sus propias películas, a pesar de que con las cámaras modernas y la variedad de películas que se encuentran a la venta, les resultaría relativamente fácil emprender por sí mis- mos la microfilmación. En virtud de las facilidades existentes el investigador puede, actualmente, aprovechar los archivos localizados en áreas remotas y carentes de comodidades para una estadía larga. Más aún, con estas ventajas se elimina el inconveniente de cargar con los materiales de investigación en un viaje largo, puesto que bastará con pasar solo una reducida parte del tiempo por fuera del lugar donde habitualmente el investigador adelanta sus traba- jos. Al microfilmar los archivos locales el investigador cuenta, ade- más, con la garantía de tener en su poder la copia de un documento entero, eludiendo, de esta manera, los problemas que puede pre- sentar una toma defectuosa de notas. En este artículo se señalan el equipo básico requerido y el procedimiento a seguir para la toma de microfilms en archivos locales. Desde luego, se puede utilizar un equipo más complejo que el descrito, pero esto solo añadiría peso y bulto al equipaje que se lleve. El equipo de que vamos a ocuparnos a continuación es fácilmente transportable y cabe sin dificultad en una maleta corriente junto a los objetos personales. Tanto el equipo como los procedimientos que se enuncian están basados en la experiencia investigativa del autor en Boyacá y Santander.

Published
1970

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