Your search keyword '"Rich KA"' showing total 4 results

1. Lineage study of degenerating photoreceptor cells in the rd mouse retina.

Author

Blanks JC, Spee C, Barrón E, Rich KA, and Schmidt S

Subjects

Animals, Cell Death, Cell Line, Mice, Mice, Neurologic Mutants anatomy & histology, Photoreceptor Cells pathology, Retinal Degeneration

Abstract

Purpose: A retroviral marker was used to label daughter cells arising from individual neuroblasts in the rd mouse retina, in order to investigate the hypothesis that a clonal relationship exists among degenerating photoreceptor cells., Methods: On the day of birth, a single injection of retrovirus with a lac Z (beta-galactosidase) reporter construct was injected into the retina in the vicinity of the subretinal space. Descendants of single neuroblasts were identified histochemically by examining the retinas at P14 (postnatal day 14). Light and electron microscopic studies were used to identify the retrovirally-induced marker beta-galactosidase using Bluo-gal dye. Double-labeling of degenerating cone cells was accomplished by taking 100 microns vibratome sections of retrovirally-injected eyes and using either FITC-PNA or HRP-PNA to visualize clusters of degenerating cones as well as Bluo-gal labeled clones of photoreceptor cells on the same tissue section., Results: A relatively large number of clones of primarily photoreceptor cells were observed in the peripheral retinas of both normal and rd mice. In a few cases in the rd, photoreceptor cells in a given clone consisted of both PNA- and Bluo-gal-labeled cells as well as of only Bluo-gal-labeled cells., Conclusion: These results suggest that during the period of intense cell death in the rd retina, a single dying photoreceptor cell can be surrounded by photoreceptors (either rods or cones) from the same clone that appear morphologically normal without evidence of degeneration.

Published

1997

2. Aberrant expression of c-Fos accompanies photoreceptor cell death in the rd mouse.

Author

Rich KA, Zhan Y, and Blanks JC

Subjects

Aging physiology, Animals, DNA Fragmentation, Genes, fos, Mice, Mice, Inbred C57BL, Mice, Mutant Strains, Photoreceptor Cells pathology, Proto-Oncogene Proteins c-jun biosynthesis, Reference Values, Retina cytology, Retina pathology, Retinal Degeneration genetics, Retinal Degeneration metabolism, Signal Transduction, Transcription Factor AP-1 biosynthesis, Apoptosis, Photoreceptor Cells physiology, Proto-Oncogene Proteins c-fos biosynthesis, Retina metabolism, Retinal Degeneration pathology

Abstract

Selective degeneration of rod photoreceptor cells in the retinal degenerative (rd) mouse prior to their complete maturation is thought to result from elevated cyclic guanosine monophosphate (cGMP) levels owing to the inherited defect in cGMP-phosphodiesterase. To investigate potential signaling pathways which might lead to apoptotic death of photoreceptors in the rd retina, the expression of immediate-early genes (IEG) of the activating protein-1 transcription factor (AP-1) family was examined. Increasing numbers of apoptotic photoreceptor nuclei were observed in the outer nuclear layer of the rd mouse beginning at postnatal day (P) 10. The peak incidence of apoptotic cells was observed at P13; by P16, almost the entire population of photoreceptors had been lost. Although c-Fos-like immunoreactivity was absent in photoreceptors of normal retinas, we observed that commencing at around P10, increasing numbers of rod photoreceptors in the rd retina exhibited nuclear staining for c-Fos protein. While no change in the distribution patterns of other members of the AP-1 family (c-Jun, JunB, and JunD) was observed in photoreceptors, Müller cell nuclei were transiently immunoreactive for c-Jun on P11. The incidence of c-Fos-positive photoreceptors peaked sharply at P12, 1 day earlier than the peak in apoptosis. Furthermore, the population of c-Fos-positive photoreceptors was distinct from apoptotic photoreceptors exhibiting chromatin condensation. The aberrant expression of c-Fos protein in rod photoreceptors immediately prior to their death in the rd mouse raises the possibility that c-Fos may be directly or indirectly involved in triggering the apoptotic cascade. Furthermore, the additional finding of c-Jun induction in Müller glia suggests that the IEG response to photoreceptor degeneration involves both intra- and intercellular signal transduction pathways.

Published

1997

3. Use of a retroviral vector with an internal opsin promoter to direct gene expression to retinal photoreceptor cells.

Author

Kido M, Rich KA, Yang G, Barrón E, Kohn DB, al-Ubaidi MR, and Blanks JC

Subjects

3T3 Cells metabolism, Animals, Blotting, Northern, Eye Neoplasms metabolism, Gene Expression, Gene Transfer Techniques, Immunoenzyme Techniques, Mice, Mice, Inbred C57BL, Phosphoric Diester Hydrolases genetics, RNA, Messenger biosynthesis, Retina metabolism, Retinoblastoma metabolism, Tumor Cells, Cultured, beta-Galactosidase genetics, Genetic Vectors, Lac Operon genetics, Moloney murine leukemia virus genetics, Phosphoric Diester Hydrolases biosynthesis, Photoreceptor Cells enzymology, Rod Opsins genetics, beta-Galactosidase biosynthesis

Abstract

Purpose: Viral-mediated gene transfer to retina, as well as to other tissues, is evolving rapidly. We have evaluated the potential of a retroviral vector with an internal opsin promoter fragment to direct gene expression to retinal photoreceptor cells., Methods: Two recombinant retroviral vectors were prepared; in each Vector, a 1.4 kb fragment of the mouse opsin promoter was placed downstream from the neoR gene in the Moloney murine leukemia virus-based vector G1Na. The opsin promoter fragment was linked either to the cDNA for mouse rod photoreceptor phosphodiesterase (PDE) beta-subunit or to the bacterial lacZ reporter gene. These vectors were tested for their ability to direct gene expression after transduction of 3T3 and Y79 cells, or of dissociated retinal cell cultures or retinal explants from neonatal mice., Results: As expected, PDE beta-subunit and beta-galactosidase mRNAs were expressed only at low levels in 3T3 fibroblasts and Y79 retinoblastoma cells. Northern blot analysis indicated that expression was derived from the viral long terminal repeat (LTR) promoter. Infection of primary retinal cell cultures or explants from neonatal mice with BAG retrovirus, in which beta-galactosidase is driven by the viral LTR, resulted in expression in many cell types, while the opsin-lacZ vector mediated the expression of the lacZ reporter gene specifically in photoreceptor cells., Conclusions: The internal opsin promoter fragment appears capable of selectively directing gene expression to photoreceptor cells after retroviral-mediated gene transfer. These findings serve as a basis for future studies using the opsin promoter-beta PDE retroviral vector to rescue photoreceptor cells in the rd mutant mouse, in which the beta-PDE gene is mutated resulting in degeneration of photoreceptor cells during the early postnatal period.

Published

1996

4. Effects of Müller cell disruption on mouse photoreceptor cell development.

Author

Rich KA, Figueroa SL, Zhan Y, and Blanks JC

Subjects

Animals, Cell Communication physiology, Cell Movement physiology, Fluorescent Antibody Technique, Glutamate-Ammonia Ligase metabolism, Mice, Mice, Inbred C57BL, Microscopy, Electron, Neuroglia drug effects, Photoreceptor Cells ultrastructure, Retina enzymology, Retina ultrastructure, 2-Aminoadipic Acid pharmacology, Neuroglia physiology, Photoreceptor Cells growth & development

Abstract

Müller cells have been proposed to play an important role in photoreceptor cell development during the final stages of retinal maturation. The effect of disrupting Müller cells during mouse retinal development was investigated using the specific glial cell toxin, DL-alpha-aminoadipic acid (AAA). By giving multiple systemic injections over several days, impairment of Müller cell function was maintained during the period of photoreceptor migration and differentiation. Following three consecutive days of AAA treatment [commencing on post-natal (P) day 3, 5, 7 or 9, and examined at P8-P14], clumps of photoreceptor nuclei were displaced through the inner segments, lying immediately beneath the retinal pigment epithelium (RPE). Apart from the scalloped appearance of the outer retina, the overall lamination pattern of the retina was relatively well preserved. Even when AAA treatment commenced as early as P3, several days prior to the formation of the outer nuclear layer, the majority of photoreceptors migrated to their correct position and formed inner and outer segments. Therefore, the signals for photoreceptor migration are either provided by the Müller cells prior to P3, or, alternatively, are derived from different intrinsic or extrinsic cues. Disruption of Müller cell function was evidenced by decreased glutamine synthetase activity as well as by increased glial fibrillary acidic protein (GFAP) and decreased cellular retinaldehyde-binding protein (CRALBP) immunoreactivity. Immunocytochemistry with an antibody to CD44, which labels the microvilli of Müller cells at the outer limiting membrane, coupled with electron microscopic analysis, demonstrated that the zonulae adherentes between Müller cells and photoreceptors were either irregular or absent in areas adjacent to displaced clumps of photoreceptors. Thus AAA treatment of early post-natal mice results in localized disruption of the contacts between Müller cells and photoreceptors. These pathologic changes persist into adulthood since at P28, while short stretches of photoreceptors appeared relatively normal with fully developed outer segments, periodic clumps of displaced photoreceptor nuclei were still present adjacent to the RPE. In conclusion, Müller cell processes at the outer limiting membrane appear to play a critical role in providing a barrier to aberrant photoreceptor migration into the subretinal space.

Published

1995