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1. Avian dark cells

Author

Hara, J., Plymale, D. R., Shepard, D. L., Hara, H., Garry, Robert F., Yoshihara, T., Zenner, Hans-Peter, Bolton, M., Kalkeri, R., and Fermin, C. D.

Published
2002
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2. Both necrosis and apoptosis contribute to HIV-1-induced killing of CD4 cells

Author

Plymale, D. R, Tang, D. S, Comardelle, A. M, Fermin, C. D, Lewis, D. E, and Garry, R. F

Subjects
Life Sciences (General)
Abstract

BACKGROUND: Data currently available on HIV-1-induced cytopathology is unclear regarding the mechanism of cell killing. OBJECTIVE: To clarify the extent to which apoptosis or necrosis is involved in HIV-1-induced cell death in view of conflicting existing data. METHODS: T lymphoblastoid cells or peripheral blood mononuclear cells were infected by various strains of HIV-1 and the numbers of apoptotic or necrotic cells were quantified at various times after infection using video-image analysis techniques; the results were compared with the amount of fragmented DNA using a quantitative method. Measurement of mitochondrial transmembrane potential (deltapsi(m)) and intracellular calcium concentrations [Ca2+]i was performed with fluorescent probes and fluorescence concentration analysis (FCA). RESULTS: Although lymphoblastoid and monocytoid cells acutely infected by HIV-1 had increased levels of fragmented DNA, a marker of apoptotic cell death, few (<12%) had condensed chromatin and fragmented nuclei, the morphological features of apoptosis. The predominant alterations in acutely infected cells were distended endoplasmic reticulum and abnormal mitochondria; these ultrastructural changes are consistent with necrosis, although some infected cells simultaneously displayed features of both necrosis and apoptosis. Viability of cells persistently infected by HIV-1 was only minimally reduced from that of uninfected cells. This reduction was accounted for by an increased propensity of the persistently infected cells to die by apoptosis. Alterations in [Ca2+]i and deltapsi(m) occurred in both acutely and persistently infected cells. CONCLUSION: Both necrosis and apoptosis contribute to HIV-1-induced killing of CD4 cells.

Published
1999
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3. Otoconia biogenesis, phylogeny, composition and functional attributes

Author

Fermin, C. D, Lychakov, D, Campos, A, Hara, H, Sondag, E, Jones, T, Jones, S, Taylor, M, Meza-Ruiz, G, and Martin, D. S

Subjects
Life Sciences (General)
Abstract

This work consolidates data about these interesting organic crystals of vertebrate inner ears. It addresses 5 aspects of inner ear otoliths not completely understood to date: 1) embryological data that explains the formation of the crystals, 2) the significance of the organic and the inorganic phase of the otolith and the changing patterns of otoconia formation along the evolutionary tree, 3) otoliths contribution for detecting linear acceleration, 4) the effect that altered gravity and aminoglycosides have on the development and adult shape of the crystals, and the evolutionary significance of a changing shape of the crystals from primitive forms (lamprey) to high vertebrate birds and mammals is discussed, 5) functional attributes of the otolithic organs and morphological modifications of the otoliths by physical and chemical insults are presented with an extensive discussion of the most relevant literature published and available to us.

Published
1998

4. Chicken (Gallus domesticus) inner ear afferents

Author

Hara, H, Chen, X, Hartsfield, J. F, Hara, J, Martin, D, and Fermin, C. D

Subjects
Life Sciences (General)
Abstract

Neurons from the vestibular (VG) and the statoacoustic (SAG) ganglion of the chick (Gallus domesticus) were evaluated histologically and morphometrically. Embryos at stages 34 (E8 days), 39 (E13 days) and 44 (E18 days) were sacrificed and temporal bones microdissected. Specimens were embedded in JB-4 methacrylate plastic, and stained with a mixture of 0.2% toluidine blue (TB) and 0.1% basic Fuschin in 25% ethanol or with a mixture of 2% TB and 1% paraphenylenediamine (PDA) for axon and myelin measurement study. Images of the VIIIth nerve were produced by a V150 (R) color imaging system and the contour of 200-300 neuronal bodies (perikarya) was traced directly on a video screen with a mouse in real time. The cross-sectional area of VG perikarya was 67.29 micrometers2 at stage 34 (E8), 128.46 micrometers2 at stage 39 (E13) and 275.85 micrometers2 at stage 44 (E18). The cross-sectional area of SAG perikarya was 62.44 micrometers2 at stage 34 (E8), 102.05 micrometers2 at stage 39 (E13) and 165.02 micrometers2 at stage 44 (E18). A significant cross-sectional area increase of the VG perikarya between stage 39 (E13) and stage 44 (E18) was determined. We randomly measured the cross-sectional area of myelin and axoplasm of hatchling afferent nerves, and found a correspondence between axoplasmic and myelin cross-sectional area in the utricular, saccular and semicircular canal nerve branches of the nerve. The results suggest that the period between stage 34 (E8) and 39 (E13) is a critical period for afferent neuronal development. Physiological and behavioral vestibular properties of developing and maturing hatchlings may change accordingly. The results compliment previous work by other investigators and provide valuable anatomical measures useful to correlate physiological data obtained from stimulation of the whole nerve or its parts.

Published
1998
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7. Color threshold and ratio of S100 beta, MAP5, NF68/200, GABA & GAD. I. Distribution in inner ear afferents

Author

Fermin, C. D, Martin, D. S, and Hara, H

Subjects
Life Sciences (General)
Abstract

Afferents of chick embryos (Gallus domesticus) VIIIth nerve were examined at E3, E6, E9, E13, El7, and hatching (NH) for anti-S100 beta, anti-MAP5, anti-GABA, anti-GAD and anti-NF68/200 stain. Different ages were processed together to determine if the distribution of these antibodies changed during synaptogenesis and myelination. Color thresholding showed that saturation of pixels changed for S100 beta only 5%, for NF68/200 10%, and for MAP5, 10%, between E9-NH. Color ratio of NF68/200 over MAP5 was 1.00 at E13 and 0.25 at E16 and NH. S100 beta, GABA and GAD were co-expressed on nerve endings at the edge of the maculae and center of the cristae, whereas hair cells in the center of the maculae expressed either S100 beta or GABA, but not both. S100 beta/NF68/200 shared antigenic sites on the chalices, but NF68/200 expression was higher than S100 beta in the chalices at hatching. MAP5 was expressed in more neurons than NF68/200 at E11, whereas NF68/200 was more abundant than MAP5 at hatching. The results suggest that: 1) the immunoexpression of these neuronal proteins is modulated concomitantly with the establishment of afferent synapses and myelination; 2) S100 beta may serve a neurotrophic function in the chalices where it is co-expressed with the neurotransmitter GABA and its synthesizing enzyme GAD.

Published
1997

8. Microgravity in the STS-29 space shuttle discovery affected the vestibular system of chick embryos

Author

Fermin, C. D, Martin, D, Jones, T, Vellinger, J, Deuser, M, Hester, P, and Hullinger, R

Subjects
Life Sciences (General)
Abstract

Out of 32 embryos flown (16 @ E2 + 16 @ E9) for 5 days, 16 survived. All sixteen E2 were dead at landing. Eight were opened and eight were incubated at 1.0G. Autopsy showed that 4 E2 survived over 24 hours in space. Eight E14 hatched without anatomical malformations, and 8 E14 were fixed. The height of the macular epithelia was 31 mu m (mean) in control and 26 mu m in flight chicks. The cross-sectional area of macular nuclei of control was 17 mu m(2) for hair cells and 14 mu m(2) in supporting cells. In flight, cross-sectional area was 17 mu m(2) in hair cells and 15 mu m(2) in supporting cells (n=250). The shape factor of cartilage cells (1.0 = perfect circle) between control (mean = 0.70) and flight (mean = 0.72), and the area of cartilaginous cells between controls (mean = 9 mu m(2)) and flight (mean = 9 mu m(2)) did not differ (n=300). The nuclei of support cells were closer to the basement membrane in flight than in control chicks. The immunoreactivity of otoconia with anti keratan, fibronectin or chrondroitin sulfate was not different between flight and control ears. There were more afferent fibers inside the macular epithelia of flight (p<0.05) than control. Three of 8 flight animals had elevated vestibular thresholds (VT), with normal mean response amplitudes and latencies. Modified afferent innervation patterns requiring weeks to compensate are sufficient to elevate VT, and should be investigated further. Other reversible (sublethal) microgravity effects on sensory epithelia (vacuoles, swelling, etc) require quantification.

Published
1996

9. Comparison of DNA fragmentation and color thresholding for objective quantitation of apoptotic cells

Author

Plymale, D. R, Ng Tang, D. S, Fermin, C. D, Lewis, D. E, Martin, D. S, and Garry, R. F

Subjects
Life Sciences (General)
Abstract

Apoptosis is a process of cell death characterized by distinctive morphological changes and fragmentation of cellular DNA. Using video imaging and color thresholding techniques, we objectively quantitated the number of cultured CD4+ T-lymphoblastoid cells (HUT78 cells, RH9 subclone) displaying morphological signs of apoptosis before and after exposure to gamma-irradiation. The numbers of apoptotic cells measured by objective video imaging techniques were compared to numbers of apoptotic cells measured in the same samples by sensitive apoptotic assays that quantitate DNA fragmentation. DNA fragmentation assays gave consistently higher values compared with the video imaging assays that measured morphological changes associated with apoptosis. These results suggest that substantial DNA fragmentation can precede or occur in the absence of the morphological changes which are associated with apoptosis in gamma-irradiated RH9 cells.

Published
1995

10. The glycan keratan sulfate in inner ear crystals

Author

Fermin, C. D, Martin, D. S, Li, Y. T, and Li, S. C

Subjects
Life Sciences (General)
Abstract

The otoconial matrix (OM) of chicks (Gallus domesticus) inner ear was analyzed. Histochemically the OM was reacted with phosphotungstic acid (PTA) and immunohistochemically with the monoclonal antibody antikeratan sulfate (antiKS). The OM was digested with the enzyme endo-beta-galactosidase (E beta Galase) or separated by 1D and 2D gel electrophoresis. PTA which reacts with glycoproteins precipitated the OM, suggesting that the OM contains glycoproteins. A central core in each crystal had no PTA staining, suggesting that the core lacked glycoproteins. Anti KS antibody stained the OM with increased density in older embryos as determined by color thresholding. E beta Galase, which cleaves the lactosamine repeating units in KS, decreased the immunostain by 30% in the OM and by 20% in the cartilage. The OM from the utricle, saccule and macula lagena contained similar molecular weight bands. Five dense bands in the OM were less dense in tissue and blood controls, suggesting that such bands are enriched in the OM. Isoelectric focusing of the OM showed a negatively charged high molecular weight smear not present in blood and faint in tissue controls. The high affinity of the OM for the cationic PTA stain, the strong immunohistochemical reaction of the OM with anti KS antibody and high molecular weight negative smear in 2D gels taken together suggest that: a) the OM contains large amounts of glycoproteins and glycans, one of which is keratan sulfate, because its immuno stain with antiKS antibody was decreased by the enzyme E beta Galase, b) the utricle, saccule and macula lagena may have similar composition, and c) the concentration of KS may increase gradually until complete mineralization of the OM is reached.

Published
1995

11. Expression of S100 beta in sensory and secretory cells of the vertebrate inner ear

Author

Fermin, C. D and Martin, D. S

Subjects
Life Sciences (General)
Abstract

We evaluated anti-S100 beta expression in the chick (Gallus domesticus) inner ear and determined that: 1) the monomer anti-S100 beta is expressed differentially in the vestibular and auditory perikarya; 2) expression of S100 beta in the afferent nerve terminals is time-related to synapse and myelin formation; 3) the expression of the dimer anti-S100 alpha alpha beta beta and monomer anti-S100 beta overlaps in most inner ear cell types. Most S100 alpha alpha beta beta positive cells express S100 beta, but S100 beta positive cells do not always express S100 alpha alpha beta beta. 4) the expression of S100 beta is diffused over the perikaryal cytoplasm and nuclei of the acoustic ganglia but is concentrated over the nuclei of the vestibular perikarya. 6) S100 beta is expressed in secretory cells, and it is co-localized with GABA in sensory cells. 7) Color thresholding objective quantitation indicates that the amount of S100 beta was higher (mean 22, SD +/- 4) at E19 than at E9 (mean 34, SD +/- 3) in afferent axons. 8) Moreover, S100 beta was unchanged between E11-E19 in the perikaryal cytoplasm, but did change over the nuclei. At E9, 74%, and at E21, 5% of vestibular perikarya were positive. The data suggest that S100 beta may be physically associated with neuronal and ionic controlling cells of the vertebrate inner ear, where it could provide a dual ionic and neurotrophic modulatory function.

Published
1995

12. Elliptical-P cells in the avian perilymphatic interface of the Tegmentum vasculosum

Author

Fermin, C. D, Lee, D. H, and Martin, D. S

Subjects
Life Sciences (General)
Abstract

Elliptical cells (E-P) are present at the perilymphatic interface lumen (PIL) of the lagena. The E-P cells often separate from the tegmentum vasculosum (TV) and have touching processes that form a monolayer between the K+ rich perilymph and the Na+ rich endolymph, similar to the mammalian Reissner's membrane. We examined the TV of chicks (Gallus domesticus) and quantitated the expression of anti-S100 alphaalphabetabeta and S100 beta. There was a 30% increase of S100 beta saturation in the light cells facing the PIL when compared to other TV light cells. We show that: (1) the dimer anti- S100 alphaalphabetabeta and the monomer anti-S100 beta are expressed preferentially in the light cells and the E-P cells of TV; (2) expression of S100 beta is higher in light cells facing the PIL than in adjacent cells; (3) the expression of the dimer S100 alphaalphabetabeta and monomer S100 beta overlaps in most inner ear cell types, including the cells of the TV, most S100 alphaalphabetabeta positive cells express S 100 beta, but S100 beta positive cells do not always express S100 alphaalphabetabeta; and (4) the S100 beta expression in light cells, the abundant Na+-K+ ATPase on dark cells of the TV, and previously demonstrated co-localization of S100 beta/GABA in sensory cells suggest that S100 beta could have, in the inner ear, a dual neurotrophic-ionic modulating function.

Published
1995

13. Post-embedding tem signal-to-noise ratio of S-100

Author

Fermin, C. D, Lee, D. H, and Martin, D

Subjects
Life Sciences (General)
Abstract

We assessed the reactivity of purified S-100 antiserum in immuno-electron microscopy by counting the number of gold particles per microns 2 over inner ear tissues embedded in different media. Sections containing predominantly Schwann's cell cytoplasm and nucleus, afferent fiber axoplasm and myelin sheath of chick cochleae were reacted with anti-S-100 IgG, an antibody to a calcium binding protein of neuronal tissues, then labeled with anti-IgG-gold conjugate. This investigation was conducted because previously published procedures, unmodified, did not yield acceptable results. Preparation of all specimens was identical. Only the medium (PolyBed 812, Araldite or Spurr epoxies; and LR White, LR Gold or Lowicryl plastics) was changed. The medium was made the changing variable because antigens available in post-embedding immuno-electron microscopy are decreased by heat, either used and/or released during polymerization of the embedding medium. The results indicate that: (a) none of the embedding media above provided optimal signal-to-noise ratio for all parts of the nerve stained in the same section; (b) aggregation of gold particles over cells was highest in embedding media with high background labeling over areas devoid of tissue (noise); (c) aggregation occurred randomly throughout both cellular and acellular regions; and (d) particles aggregated less and were distributed more evenly in tissues from media yielding good ultrastructural integrity.

Published
1994
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14. High resolution and image processing of otoconia matrix

Author

Fermin, C. D

Subjects
Life Sciences (General)
Abstract

This study was designed to investigate patterns of fibrils organization in histochemically stained otoconia. Transmission electron microscope and video imaging were used. These data indicate that otoconia of the chick (Gallus domesticus) inner ear may have central cores in vivo. The data also show that the ultrastructural organization of fibrils fixed with aldehydes and histochemical stains follows trajectories that conform to the hexagonal shape of otoconia. These changes in direction may contribute to the formation of a central core. The existence of central cores is important for the in vivo buoyancy of otoconia. Packing of fibrils is tighter after phosphotungstic acid (PTA) stained otoconia than with other histochemical stains, which usually produce looser packing of fibrils and seemingly larger central core. TEM of tilted and untilted material showed that turning of fibrils occurs at the points where the face angles of otoconia form and where central cores exist. Video image processing of the images allowed reconstructing a template which, if assumed to repeat and change trajectories, would fit the pattern of fibrils seen in fixed otoconia. Since it is highly unlikely that aldehyde primary fixation or PTA stain caused such drastic change in the direction of fibrils, the template derived from these results may closely approximate patterns of otoconia fibrils packing in vivo. However, if the above is correct, the perfect crystallographic diffraction pattern of unfixed otoconia do not correspond to patterns of fixed fibrils.

Published
1993
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15. The correlated blanching of synaptic bodies and reduction in afferent firing rates caused by transmitter-depleting agents in the frog semicircular canal

Author

Guth, P, Norris, C, Fermin, C. D, and Pantoja, M

Subjects
Life Sciences (General)
Abstract

Synaptic bodies (SBs) associated with rings of synaptic vesicles and well-defined, pre- and post-synaptic membrane structures are indicators of maturity in most hair cell-afferent nerve junctions. The role of the SBs remains elusive despite several experiments showing that they may be involved in storage of neurotransmitter. Our results demonstrate that SBs of the adult posterior semicircular canal (SCC) cristae hair cells become less electron dense following incubation of the SCC with the transmitter-depleting drug tetrabenazine (TBZ). Objective quantification and comparison of the densities of the SBs in untreated and TBZ-treated frog SCC demonstrated that TBZ significantly decreased the electron density of SBs. This reduction in electron density was accompanied by a reduction in firing rates of afferent fibers innervating the posterior SCC. A second transmitter-depleting drug, guanethidine, previously shown to reduce the electron density of hair cell SBs, also reduced the firing rates of afferent fibers innervating the posterior SCC. In contrast, the electron density of dense granules (DG), similar in size and shape to synaptic bodies (SB) in hair cells, did not change after incubation in TBZ, thus indicating that granules and SBs are not similar in regard to their electron density. The role of SBs in synaptic transmission and the transmitter, if any, stored in the SBs remain unknown. Nonetheless, the association of the lessening of electron density with a reduction in afferent firing rate provides impetus for the further investigation of the SB's role in neurotransmission.

Published
1993
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16. Colour thresholding and objective quantification in bioimaging

Author

Fermin, C. D, Gerber, M. A, and Torre-Bueno, J. R

Subjects
Life Sciences (General)
Abstract

Computer imaging is rapidly becoming an indispensable tool for the quantification of variables in research and medicine. Whilst its use in medicine has largely been limited to qualitative observations, imaging in applied basic sciences, medical research and biotechnology demands objective quantification of the variables in question. In black and white densitometry (0-256 levels of intensity) the separation of subtle differences between closely related hues from stains is sometimes very difficult. True-colour and real-time video microscopy analysis offer choices not previously available with monochrome systems. In this paper we demonstrate the usefulness of colour thresholding, which has so far proven indispensable for proper objective quantification of the products of histochemical reactions and/or subtle differences in tissue and cells. In addition, we provide interested, but untrained readers with basic information that may assist decisions regarding the most suitable set-up for a project under consideration. Data from projects in progress at Tulane are shown to illustrate the advantage of colour thresholding over monochrome densitometry and for objective quantification of subtle colour differences between experimental and control samples.

Published
1992

17. Development of the endolymphatic sac in chick embryos, with reference to the degradation of otoconia

Author

Yoshihara, T, Kaname, H, Narita, N, Ishii, T, Igarashi, M, and Fermin, C. D

Subjects
Life Sciences (General)
Abstract

The endolymphatic sac of chick embryos (from embryonic day 7 to 1-day-old chicks) was studied light- and electron-microscopically. At stage 30-31 (embryonic day 7-7.5), the epithelial cells of the endolymphatic sac were cuboidal to columnar in shape. Microvilli were relatively well developed. The intercellular space was wide. In the endolymphatic space of the endolymphatic sac, varying shapes and sizes of otoconia-like bodies were often observed. Intracytoplasmic phagosomes containing these bodies were rarely found. After stage 37 (embryonic day 11), otoconia-like bodies in the endolymphatic sac decreased in number and size. They were almost the same as the otoconia in the macular organs, ultrastructurally. These findings indicate that the endolymphatic sac of the chick embryos may possess the function of otoconial degradation and removal of calcium from otoconia.

Published
1992

18. Detection of a human intracisternal A-type retroviral particle antigenically related to HIV

Author

Garry, R. F, Fermin, C. D, Hart, D. J, Alexander, S. S, Donehower, L. A, and Luo-Zhang, H

Subjects
Life Sciences (General)
Abstract

Sjogren's syndrome is an autoimmune disease that is characterized by dryness of the mouth and eyes. The loss of salivary and lacrimal gland function is accompanied by lymphocytic infiltration. Because similar symptoms and glandular pathology are observed in certain persons infected with human immunodeficiency virus (HIV), a search was initiated for a possible retroviral etiology in this syndrome. A human intracisternal A-type retroviral particle that is antigenically related to HIV was detected in lymphoblastoid cells exposed to homogenates of salivary tissue from patients with Sjogren's syndrome. Comparison of this retroviral particle to HIV indicates that they are distinguishable by several ultrastructural, physical, and enzymatic criteria.

Published
1990

20. Elliptical-P Cells in the Avian Perilymphatic Interface of the Tegmentum Vasculosum

Author

Fermin, C. D., Lee, D. H., and Martin, D. S.

Subjects
inner ear, objective quantitation, Elliptical-P cells, Tegmentum vasculosum, chicken, sense organs, video imaging, Biology, S-100β, color thresholding, transmission electron microscopy (TEM)-post-immunolabeling
Abstract

Elliptical cells (E-P) are present at the perilymphatic interface lumen (PIL) of the lagena. The E-P cells often separate from the tegmentum vasculosum (TV) and have touching processes that form a monolayer between the K+ rich perilymph and the Na+ rich endolymph, similar to the mammalian Reissner's membrane. We examined the TV of chicks (Gallus domesticus) and quantitated the expression of anti-S100ααββ and S100β. There was a 30% increase of S100β saturation in the light cells facing the PIL when compared to other TV light cells. We show that: (1) the dimer anti-S100ααββ and the mono-mer anti-S100β are expressed preferentially in the light cells and the E-P cells of TV; (2) expression of S100β is higher in light cells facing the PIL than in adjacent cells; (3) the expression of the dimer S100ααββ and monomer S100β overlaps in most inner ear cell types, including the cells of the TV, most S100ααββ positive cells express S100β, but S100β positive cells do not always express S100ααββ; and (4) the S100β expression in light cells, the abundant Na+-K+ ATPase on dark cells of the TV, and previously demonstrated co-localization of S100β/GABA in sensory cells suggest that S100β could have, in the inner ear, a dual neurotrophic-ionic modulating function.

Published
1995

21. Comparison of DNA Fragmentation and Color Thresholding for Objective Quantitation of Apoptotic Cells

Author

Plymale, D. R., Ng Tang, D. S., Fermin, C. D., Lewis, D. E., Martin, D. S., and Garry, R. F.

Subjects
Apoptosis, DNA fragmentation, γ-irradiation, human-immunodeficiency virus, Biology, color thresholding
Abstract

Apoptosis is a process of cell death characterized by distinctive morphological changes and fragmentation of cellular DNA. Using video imaging and color thresholding techniques, we objectively quantitated the number of cultured CD4 + T-lymphoblastoid cells (HUT78 cells, RH9 subclone) displaying morphological signs of apoptosis before and after exposure to γ-irradiation. The numbers of apoptotic cells measured by objective video imaging techniques were compared to numbers of apoptotic cells measured in the same samples by sensitive apoptotic assays that quantitate DNA fragmentation. DNA fragmentation assays gave consistently higher values compared with the video imaging assays that measured morphological changes associated with apoptosis. These results suggest that substantial DNA frag-mentation can precede or occur in the absence of the morphological changes which are associated with apoptosis in γ-irradiated RH9 cells.

Published
1995

22. Colour thresholding in video imaging

Author

Fermin, C D and Degraw, S

Subjects
Microscopy, Video, Microcomputers, Image Processing, Computer-Assisted, Color, Humans, In Situ Hybridization, Fluorescence, Software, Research Article
Abstract

The basic aspects of video imaging are reviewed as they relate to measurements of histological and anatomical features, with particular emphasis on the advantages and disadvantages of colour and black-and-white imaging modes. In black-and-white imaging, calculations are based on the manipulation of picture elements (pixels) that contain 0-255 levels of information. Black is represented by the absence of light (0) and white by 255 grades of light. In colour imaging, the pixels contain variation of hues for the primary (red, green and blue) and secondary (magenta, yellow, cyan, pink) colours. Manipulation of pixels with colour information is more computer intense than that for black-and-white pixels, because there are over 16 million possible combinations of colour in a system with a 24-bit resolution. The narrow 128 possible grades of separation in black and white often makes distinction between pixels with overlapping intensities difficult. Such difficulty is greatly reduced by colour thresholding of systems that base the representation of colour on a combination of hue-saturation-intensity (HSI) format.

Published
1995

23. Morphogenesis and calcification of the statoconia in the chick (Gallus domesticus) embryo - Implications for future studies

Author

Fermin, C. D and Igarashi, M

Subjects
Life Sciences (General)
Abstract

The morphogenesis of the statoconia in the chick, Gallus domesticus, injected with a carbon anhydrase inhibitor is studied. The preparation of the embryo specimens for analysis is described. The early, middle, and late stages of embryonic development are examined. The data reveal that acetozolamide inhibits statoconia formation in the middle stage of development and the calcification process follows statoconia formation. The spatial relationship between the development of type 1 and type 2 hair cells and the appearance and maturation of the statoconia is investigated.

Published
1985

24. Development of otoconia in the embryonic chick (Gallus domesticus)

Author

Fermin, C. D and Igarashi, M

Subjects
Life Sciences (General)
Abstract

In the chick (Gallus domesticus) embryo, otoconium formation started first over the macula sacculi around the 4th day of incubation, and a day later over the macula utriculi. It was determined that each otoconium formed as a result of the segmentation of the immature otolithic membrane, and that the calcium responsible for otoconium calcification was incorporated into the organic matrix of each otoconium in the form of small electron-dense granules (20-150 nm in. diameter). The presence of calcium in these granules was confirmed by histochemical staining with osmic-potassium pyroantimonate, by EDTA chelation, and by X-ray micronanalysis under the electron microscope.

Published
1985

33. Localization of Na+, K+-ATPase activity in the tegmentum vasculosum of the chick cochlea

Author

Yoshihara, T., Fermin, C. D., and Igarashi, M.

Abstract

We studied the localization of Na+, K+-ATPase activity in the chick cochlea, utilizing a cytochemical method of K+-p-nitrophenylphosphatase (K+-NPPase), and found that the enzyme activity was limited to the dark cells of the tegmentum vasculosum (TV). Our present results indicate that the dark cells of the TV play an essential role in the maintenance of the ionic composition of the cochlear endolymph.

Published
1987
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35. Immunohistochemical evaluation of AKT protein activation in canine mast cell tumours.

Author

Rodriguez S, Fadlalla K, Graham T, Tameru B, Fermin CD, and Samuel T

Subjects
Animals, Biomarkers, Tumor metabolism, Dog Diseases metabolism, Dogs, Female, Male, Mast Cells metabolism, Mastocytoma metabolism, Mastocytoma pathology, Neoplasm Staging veterinary, Dog Diseases pathology, Mast Cells pathology, Mastocytoma veterinary, Proto-Oncogene Proteins c-akt biosynthesis
Abstract

The pathogenesis of canine mast cell tumour (MCT) remains unknown. Moreover, therapeutic options are limited and resistance to targeted drugs and recurrences are common, necessitating the identification of additional cellular targets for therapy. In this study we investigated the expression of phosphorylated AKT protein in 25 archival canine MCT samples by immunohistochemistry and examined the correlation between the immunohistochemical scores and histopathological tumour grades. AKT protein was detected in all of the samples and 24 of the 25 samples expressed the phosphorylated form of the protein, albeit with variable intensity. However, when the immunohistochemical scores of weak, intermediate and strong labelling were compared with the histopathological grades I to III, there was no strong correlation. This study suggests that canine MCT cells have activated AKT and indicates the need for further research on the role of the AKT protein and the possibility of targeting the AKT signalling pathway in MCTs., (Copyright © 2011 Elsevier Ltd. All rights reserved.)

Published
2012
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36. Radioprotection in mice following oral delivery of amifostine nanoparticles.

Author

Pamujula S, Kishore V, Rider B, Fermin CD, Graves RA, Agrawal KC, and Mandal TK

Subjects
Administration, Oral, Animals, Bone Marrow Cells radiation effects, Cell Survival radiation effects, Hematopoietic Stem Cells radiation effects, Male, Mice, Amifostine administration & dosage, Nanostructures, Radiation-Protective Agents administration & dosage
Abstract

Purpose: Amifostine (Ethyol) is an approved cytoprotective agent prescribed to reduce certain side-effects in the chemotherapy of ovarian or non-small cell lung cancer, or in radiation treatment of head-and-neck cancer. The usefulness of this drug is further hampered, because it is not effective when given orally. The objective of this part of the project was to evaluate the radioprotective efficacy of orally active amifostine nanoparticles., Materials and Methods: Radioprotective efficacy was evaluated by measuring the ability of the amifostine nanoparticles (equivalent to 500 mg/Kg) to inhibit whole-body gamma irradiation -induced injury in mice. All mice received acute whole-body gamma irradiation from a Cesium-137 source and the radioprotective efficacy of the formulation was determined by measuring 30-day survival at 9 Gy, bone marrow hemopoeitic progenitor cell survival at 9 Gy and 8 Gy, and intestinal crypt cell survival at 11 Gy., Results: Thirty-day survival, hemopoietic progenitor cell survival, as well as the jejunal crypt cell survival were all significantly enhanced when the mice were treated orally with the amifostine nanoparticles 1 h prior to irradiation., Conclusions: These results clearly and unequivocally demonstrate that the amifostine nanoparticles developed in our laboratory provides significant protection from acute whole-body gamma irradiation injury in mice.

Published
2005
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37. Hepatitis C viral proteins affect cell viability and membrane permeability.

Author

Kalkeri G, Khalap N, Akhter S, Garry RF, Fermin CD, and Dash S

Subjects
Apoptosis, Cell Membrane Permeability, Cell Survival, Gene Expression, Green Fluorescent Proteins, Humans, Luminescent Proteins, Transfection, Tumor Cells, Cultured, Viral Proteins biosynthesis, Viral Proteins genetics, Hepatitis C, Viral Proteins pharmacology
Abstract

To determine the effect of hepatitis C virus (HCV) proteins on cell growth, Huh-7 cells were transfected with a full-length HCV cDNA (pMO9.6-T7 Rz) clone and HCV proteins were expressed using a replication-defective adenovirus that encodes the gene for the T7 RNA polymerase. Expression of HCV proteins from this full-length clone resulted in reduction in viability of transfected cells as measured by trypan blue viability assay. For identification and separation of cells expressing hepatitis C virus proteins by fluorescence microscopy and flow cytometry, GFP was cloned in the HCV full-length clone. Cells transfected with the HCV-GFP chimera clone produced high levels of accurately processed structural and nonstructural proteins similar to those of the HCV full-length clone, which could be detected by Western blot analysis. Cells expressing all HCV proteins lost membrane permeability and underwent apoptotic cell death, indicated by the appearance of a sub-G0 peak in cell cycle analysis, DNA fragmentation in a TUNEL assay, and microscopic detection of nuclear condensation. Using double-channel flow analysis we confirmed that high-level expression of HCV proteins affected membrane permeability and cell survival. These results suggest that expression of all structural and nonstructural proteins from HCV cDNA in hepatic cells induces apoptotic cell death, which might be an important event in chronic hepatitis infection in humans., (Copyright 2001 Elsevier Science.)

Published
2001
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38. Hepatitis C virus protein expression induces apoptosis in HepG2 cells.

Author

Kalkeri G, Khalap N, Garry RF, Fermin CD, and Dash S

Subjects
Cell Cycle, Cell Division, Cell Line, Cell Nucleus metabolism, Cell Nucleus ultrastructure, Cell Survival, DNA analysis, DNA Fragmentation, Flow Cytometry, Hepacivirus genetics, Humans, In Situ Nick-End Labeling, Microscopy, Electron, Mutation, RNA, Antisense genetics, RNA, Viral genetics, Thymidine metabolism, Transfection, Tumor Cells, Cultured, Viral Envelope Proteins metabolism, Apoptosis, Hepacivirus pathogenicity, Viral Envelope Proteins genetics
Abstract

The mechanisms of hepatocyte death and the events that lead to a high rate of chronic liver disease in patients infected with hepatitis C virus are not known. We established a HCV replication system in HepG2 cell culture and utilized this model to address the effect of HCV proteins on HepG2 cell growth and viability. After transfection of HepG2 cells with full-length RNA, a truncated RNA, or an antisense RNA, cell proliferation and cell viability were analyzed by thymidine uptake and the trypan blue exclusion method, respectively. Full-length RNA transfected HepG2 cells showed a decrease in cell proliferation and viability compared to cells transfected with HCV truncated RNA and antisense RNA control. A subset of cells expressing HCV proteins underwent apoptosis as documented by morphological studies, ultrastructural analysis, cell cycle analysis by flow cytometry, terminal transferase enzyme mediated end labeling of DNA, and DNA laddering. This study suggests that expression of HCV proteins can lead to cell death by apoptosis, which may be an important event in the pathogenesis of chronic hepatitis C virus infection in humans., (Copyright 2001 Academic Press.)

Published
2001
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39. Viral induction, transmission and apoptosis among cells infected by a Human Intracisternal A-type retrovirus.

Author

Deas JE, Thompson JJ, Fermin CD, Liu LL, Martin D, Garry RF, and Gallaher WR

Subjects
Electrophoresis, Polyacrylamide Gel, Endogenous Retroviruses ultrastructure, Flow Cytometry, Genes, Intracisternal A-Particle, Humans, Tetradecanoylphorbol Acetate pharmacology, Tumor Cells, Cultured, Apoptosis, Endogenous Retroviruses physiology
Abstract

Sjogren's Syndrome, a systemic autoimmune disease, is characterized by lymphocytic infiltration of the salivary or lacrimal glands, producing xerostomia or xerophthalmia. Although definitive proof of viral etiology has not been established, a cell line containing viral particles termed Human Intracisternal A-type Particles (HIAP) resulted from co-culture with patient lip biopsies. We stimulated these chronically infected cells with phorbol myristate acetate (PMA) in an effort to enhance production of viral particles for further characterization. We report that the virus present in the HIAP cell line can be induced to become lytic when subjected to PMA and that there is a difference in the effects of PMA on H9 and HIAP cell groups, with apparent protection from apoptosis due to PMA being exerted by viral presence. Delayed apoptosis may prolong exposure of the foreign/self complex, thus enhancing an autoimmune response. Polyacrylamide gel electrophoresis (PAGE) revealed the presence of new peptides in pellets of supernatants of PMA-stimulated HIAP cells, with prominent bands at 55 and 43 kDa, and several fainter ones. HIAP infection was transferred by cell-free filtered supernatants from stimulated cells to H9 cells, which became identical to parent HIAP cells by PAGE and fluorescence activated cell sorter.

Published
1999
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40. Role of potassium in human immunodeficiency virus production and cytopathic effects.

Author

Choi B, Gatti PJ, Haislip AM, Fermin CD, and Garry RF

Subjects
CD4-Positive T-Lymphocytes virology, Cell Line, Culture Media, Cytopathogenic Effect, Viral, DNA, Viral biosynthesis, HIV-1 pathogenicity, Humans, Proviruses genetics, T-Lymphocyte Subsets virology, Viral Proteins biosynthesis, HIV-1 physiology, Potassium physiology, Virus Replication
Abstract

Acute infection of CD4+ lymphoid cells by human immunodeficiency virus type 1 (HIV-1) induces an increase in the intracellular concentration of potassium (K+). Media containing reduced or elevated concentrations of K+ were used to investigate the role of this ion in HIV-1 production and cytopathology. Incubation of CD4+ lymphoblastoid cells acutely infected by HIV-1 (strain LAI) in low K+ medium resulted in an approximately 50% decrease in HIV-1 production and markedly diminished HIV-1 induced cytopathic effects (CPE) relative to cells incubated in medium containing a normal K+ concentration (approximately 5 mM). Incubation of HIV-1 infected cells in media containing elevated concentrations of K+ medium. Cells mM) increased HIV-1 production by two- to fivefold over the amount produced in cells incubated in normal K+ medium. Cells incubated in high K+ media also displayed enhanced HIV-1-induced cytopathology. The decrease in HIV-1 production by low K+ medium and increase by high K+ media could be a accounted for by effects on HIV-1 reverse transcription. However, low K+ medium inhibited HIV-1 protein synthesis and high K+ media increased HIV-1 protein synthesis. These results suggest that the HIV-1-induced increase in intracellular is required for efficient viral replication and to induce cytopathology.

Published
1998
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41. Inhibition of HIV type 1 production by hygromycin B.

Author

Gatti PJ, Choi B, Haislip AM, Fermin CD, and Garry RF

Subjects
DNA, Viral biosynthesis, HIV-1 genetics, HIV-1 growth & development, HIV-1 metabolism, Humans, Protein Biosynthesis, Tumor Cells, Cultured, Anti-Bacterial Agents pharmacology, Anti-HIV Agents pharmacology, HIV-1 drug effects, Hygromycin B pharmacology, Protein Synthesis Inhibitors pharmacology
Abstract

HIV infection alters the cellular uptake of ions and other small molecules. This study was designed to determine whether hygromycin B, a low molecular weight (MW 527) aminoglycoside protein synthesis inhibitor that is normally impermeable to mammalian cells at micromolar concentrations, can selectively inhibit HIV expression and cytopathology. CD4+ T lymphoblastoid cells (H9) and peripheral blood mononuclear cells (PBMCs) were infected with HIV-1, then incubated in medium containing various concentrations of hygromycin B. HIV-1-induced formation of multinucleated giant cells and single cell killing were dramatically reduced in the presence of micromolar concentrations of hygromycin B. Hygromycin B also inhibited HIV-1 production in a dose-dependent manner during acute infection. G418, a larger and more hydrophobic aminoglycoside (MW 692), did not display the same selective inhibition of HIV-1 production as hygromycin B. Relative to mock-infected cells, protein synthesis in acutely infected H9 cells was selectively inhibited by hygromycin B. Hygromycin B also reduced HIV production in PBMCs and in H9 cells persistently infected with HIV. PCR analysis demonstrated that hygromycin B did not inhibit HIV-1 reverse transcription. These results demonstrate that HIV-1 infection renders cells more sensitive to hygromycin B than uninfected cells, and provides support for the hypothesis that HIV-1 induces an alteration of plasma membrane permeability. The HIV-modified cell membrane may be a potential target for antiviral intervention and chemotherapy.

Published
1998
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42. A synthetic peptide corresponding to the carboxy terminus of human immunodeficiency virus type 1 transmembrane glycoprotein induces alterations in the ionic permeability of Xenopus laevis oocytes.

Author

Comardelle AM, Norris CH, Plymale DR, Gatti PJ, Choi B, Fermin CD, Haislip AM, Tencza SB, Mietzner TA, Montelaro RC, and Garry RF

Subjects
Animals, Ion Transport, Oocytes cytology, Oocytes metabolism, Patch-Clamp Techniques, Xenopus laevis, Cell Membrane Permeability drug effects, HIV Envelope Protein gp41 chemistry, Oocytes drug effects, Peptide Fragments pharmacology
Abstract

The carboxy-terminal 29 amino acids of the human immunodeficiency virus type 1 transmembrane glycoprotein (HIV-1 TM) are referred to as lentivirus lytic peptide 1 (LLP-1). Synthetic peptides corresponding to LLP-1 have been shown to induce cytolysis and to alter the permeability of cultured cells to various small molecules. To address the mechanisms by which LLP-1 induces cytolysis and membrane permeability changes, various concentrations of LLP-1 were incubated with Xenopus laevis oocytes, and two-electrode, voltage-clamp recording measurements were performed. LLP-1 at concentrations of 75 nM and above induced dramatic alterations in the resting membrane potential and ionic permeability of Xenopus oocytes. These concentrations of LLP-1 appeared to induce a major disruption of plasma membrane electrophysiological integrity. In contrast, concentrations of LLP-1 of 20-50 nM induced changes in membrane ionic permeability that mimic changes induced by compounds, such as the bee venom peptide melittin, that are known to form channel-like structures in biological membranes at sublytic concentrations. An analog of LLP-1 with greatly reduced cytolytic activity failed to alter the electrophysiological properties of Xenopus oocytes. Thus, by altering plasma membrane ionic permeability, the carboxy terminus of TM may contribute to cytolysis of HIV-1-infected CD4+ cells.

Published
1997
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43. Tumor-host interaction: analysis of cytokines, growth factors, and tumor-infiltrating lymphocytes in ovarian carcinomas.

Author

Merogi AJ, Marrogi AJ, Ramesh R, Robinson WR, Fermin CD, and Freeman SM

Subjects
Adenocarcinoma immunology, Adenocarcinoma secondary, Adult, Aged, Colonic Neoplasms immunology, Colonic Neoplasms pathology, DNA Primers, Esophageal Neoplasms immunology, Esophageal Neoplasms pathology, Fallopian Tube Neoplasms immunology, Fallopian Tube Neoplasms pathology, Female, Granulocyte-Macrophage Colony-Stimulating Factor metabolism, Humans, Immunohistochemistry, Interferon-gamma metabolism, Interleukins metabolism, Lymphocytes, Tumor-Infiltrating metabolism, Middle Aged, Ovarian Neoplasms metabolism, Ovarian Neoplasms pathology, RNA analysis, Transforming Growth Factor beta metabolism, Tumor Necrosis Factor-alpha metabolism, Cytokines metabolism, Lymphocytes, Tumor-Infiltrating immunology, Ovarian Neoplasms immunology
Abstract

The host-tumor interaction may play an important role in determining tumor progress. Recent studies have shown that this interaction can be influenced by the release of soluble factors by tumor cells and tumor-infiltrating lymphocytes (TIL). The aim of our study is to characterize the nature of cytokines and growth factors and their relationship to the cellular infiltrates in 16 patients with ovarian cancer using reverse transcriptase-polymerase chain reaction (RT-PCR) and immunohistochemistry. Total RNA from 20 malignant and 10 benign specimens were used to assay for expression of 12 cytokines. Additionally, monoclonal antibodies (MAbs) were used to detect T cells, CD4+ helper and CD8+ cytotoxic/suppressor T-cell subtypes, B cells, and macrophages. Our results showed the expression of transforming growth factor-beta1 (TGF-beta1), interleukin-10 (IL-10), and granulocyte-macrophage colony-stimulating factor (GM-CSF) in 19, 17, and 10 malignant specimens, P < .001, .001, and .05, respectively. Other cytokines such as interferon-gamma (IFN-gamma), tumor necrosis factor-alpha (TNF-alpha), TNF-beta/LT, IL-2, and IL-6 were expressed in a few cases, and IL-1alpha and IL-4 expression were not detected. The benign samples did not express IL-10, but GM-CSF, TGF-beta1, and IL-8 were expressed in one, one, and four specimens, respectively. Interestingly, in four cases in which samples from the primary and relapse tumors were available for analysis, the tumors in relapse showed a significant increase for TGF-beta1 (P < .05) and a decreased trend in IL-10 mRNA levels. The source of these factors was tumor cells as detected immunohistochemically. This combined alteration of TGF-beta1 and IL-10 was associated with a significant reduction in number of TIL in general, and CD8+ and macrophages in particular (P = .036 and .049, respectively). Our findings suggest the important role of certain soluble factors in the complex process of tumor progression. Furthermore, understanding the tumor-host relationship and the factors influencing the interaction may be helpful in developing effective and innovative treatment methods.

Published
1997
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44. Antibodies against retroviral proteins and nuclear antigens in a subset of idiopathic CD4+ T lymphocytopenia patients.

Author

Garry RF, Fermin CD, Kohler PF, Markert ML, and Luo H

Subjects
Adult, Antigens, Nuclear, CD4-Positive T-Lymphocytes immunology, Coculture Techniques, Cytopathogenic Effect, Viral, Humans, Immunoblotting, Male, T-Lymphocytopenia, Idiopathic CD4-Positive blood, T-Lymphocytopenia, Idiopathic CD4-Positive virology, Virion immunology, Antibodies, Antinuclear blood, Antibodies, Viral blood, Autoantigens immunology, Nuclear Proteins immunology, Retroviridae Proteins immunology, T-Lymphocytopenia, Idiopathic CD4-Positive immunology
Abstract

Idiopathic CD4+ T lymphocytopenia (ICL) is an immunodeficiency syndrome characterized by severe depletion of CD4+ T lymphocytes, but in which human immunodeficiency virus cannot be detected. Peripheral blood mononuclear cells (BPMCs) from an ICL patient were cocultured with HUT78 T-lymphoblastoid cells, and an acute cytopathic effect and formation of multinucleated cells were observed. A human intracisternal A-type retroviral particle designated HIAP-II was detected in cells surviving the acute cytopathic effect. Eight of 13 ICL patients in a blinded screen of a serological panel provided by the National Centers for Disease Control and Prevention (CDC) had serum antibodies that specifically reacted with HIAP-II associated proteins by Western immunoblotting. None of 19 control sera in the panel that were unreactive with HIV Gag proteins produced a positive result on HIAP-II immunoblots. Comparable results were obtained in a blinded screen of a second CDC serological panel. Sera from 8 of 14 ICL patients in the second serological panel were positive for antinuclear autoantibodies (ANAs) commonly observed in patients with systemic autoimmune diseases. These results suggest the possible involvement of an A-type retrovirus or autoimmunity in development of ICL in a subset of patients.

Published
1996
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45. Reduction of human immunodeficiency virus production and cytopathic effects by inhibitors of the Na+/K+/2Cl- cotransporter.

Author

Voss TG, Gatti PJ, Fermin CD, and Garry RF

Subjects
CD4-Positive T-Lymphocytes cytology, CD4-Positive T-Lymphocytes drug effects, CD4-Positive T-Lymphocytes virology, Cell Death, Cell Line, Cytopathogenic Effect, Viral drug effects, HIV Core Protein p24 metabolism, HIV-1 growth & development, HIV-1 metabolism, Humans, Potassium metabolism, Sodium metabolism, Sodium-Potassium-Chloride Symporters, Antiviral Agents pharmacology, Carrier Proteins antagonists & inhibitors, Furosemide pharmacology, HIV-1 drug effects, Membrane Proteins antagonists & inhibitors
Abstract

Infection of CD4+ T-lymphoblastoid cells by cytopathic strains of HIV-1 results in an increase in cell volume that leads to lysis and cell death. The increase in volume is attributable in part to an HIV-induced increase in intracellular monovalent ion concentrations mediated by the plasma membrane-associated Na+/K+/2 Cl- cotransporter. Loop diuretics, which inhibit cotransporter activity, blocked HIV-induced HIV production and cytopathic effects at physiologically employed concentrations.

Published
1996
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46. Colour thresholding in video imaging.

Author

Fermin CD and Degraw S

Subjects
Humans, In Situ Hybridization, Fluorescence, Microcomputers, Software, Color, Image Processing, Computer-Assisted, Microscopy, Video
Abstract

The basic aspects of video imaging are reviewed as they relate to measurements of histological and anatomical features, with particular emphasis on the advantages and disadvantages of colour and black-and-white imaging modes. In black-and-white imaging, calculations are based on the manipulation of picture elements (pixels) that contain 0-255 levels of information. Black is represented by the absence of light (0) and white by 255 grades of light. In colour imaging, the pixels contain variation of hues for the primary (red, green and blue) and secondary (magenta, yellow, cyan, pink) colours. Manipulation of pixels with colour information is more computer intense than that for black-and-white pixels, because there are over 16 million possible combinations of colour in a system with a 24-bit resolution. The narrow 128 possible grades of separation in black and white often makes distinction between pixels with overlapping intensities difficult. Such difficulty is greatly reduced by colour thresholding of systems that base the representation of colour on a combination of hue-saturation-intensity (HSI) format.

Published
1995

47. Viral burden in AIDS.

Author

Garry RF and Fermin CD

Subjects
Acquired Immunodeficiency Syndrome drug therapy, CD4-Positive T-Lymphocytes microbiology, Cell Death, HIV physiology, Humans, Immune System physiology, Nucleosides therapeutic use, Acquired Immunodeficiency Syndrome microbiology
Published
1993
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48. [Possible involvement of a recently discovered human retrovirus in idiopathic immunologic disorders, including Sjögren syndrome (autoimmune exocrinopathy)].

Author

Fermin CD and Garry RF

Subjects
Autoimmune Diseases immunology, Humans, Inclusion Bodies, Viral ultrastructure, Microscopy, Electron, Retroviridae Infections immunology, Salivary Glands microbiology, Sjogren's Syndrome immunology, Vacuoles ultrastructure, Virulence, Autoimmune Diseases microbiology, Retroviridae pathogenicity, Retroviridae Infections microbiology, Sjogren's Syndrome microbiology
Abstract

Recent studies have suggested that newly-discovered human retroviruses may contribute to the pathogenesis of several immunological diseases. We linked a human intracisternal A-type retroviral particle (HIAP) to systemic autoimmune diseases, such as Sjögren's Syndrome. A-type retroviruses are envelope-deficient, a property that may contribute to their pathobiology and epidemiology. Potential mechanisms by which a defective retrovirus could induce immune dysfunctions are discussed.

Published
1993

49. Membrane alterations linked to early interactions of HIV with the cell surface.

Author

Fermin CD and Garry RF

Subjects
CD4-Positive T-Lymphocytes metabolism, Cell Membrane metabolism, Cells, Cultured, HIV-1 growth & development, Humans, Intracellular Membranes metabolism, Intracellular Membranes ultrastructure, Membrane Fusion, Vacuoles metabolism, Vacuoles ultrastructure, Virus Replication, CD4-Positive T-Lymphocytes ultrastructure, Cell Membrane ultrastructure, HIV Infections pathology, HIV-1 ultrastructure
Abstract

Ultrastructural studies suggest that cell surface alterations occur early during the course of HIV-1 infection of CD4+T-lymphoblastoid cells. Attachment and penetration of HIV resulted in formation of membrane discontinuities and pores and "ballooning." Distention of the endoplasmic reticulum occurred in some cells within the first hour after HIV infection, and this correlated with the numbers of virions bound at the cell surface. These results suggest that HIV virion components may directly damage the cell membrane.

Published
1992
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50. Early damage to granulocytes during storage.

Author

Humbert JR, Fermin CD, and Winsor EL

Subjects
Cell Membrane ultrastructure, Cell Survival, Cytoplasmic Granules ultrastructure, Free Radicals, Granulocytes ultrastructure, Humans, Microscopy, Electron, Neutrophils physiology, Neutrophils ultrastructure, Oxidation-Reduction, Time Factors, Vacuoles ultrastructure, Blood Preservation, Granulocytes physiology
Published
1991

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