Journal Contents

Am Jour Ophthalmol
Br J Ophthalmol
Can J Ophthalmol
J Cat Ref Surg
Cornea
Curr Eye Res
Eur J Ophthalmol
Eye
J Glaucoma
JAMA Ophthalmol
Graefes Ophthalmol
Indian J Ophthalmol
Int Ophthalmol Clin
Invest Ophth Vis Sci
Jpn J Ophthalmol
JPOS
Korean J Ophthal
J Neuroophthalmol
Ophthalmic Epidemiol
Ophthalmic Genet
Ophthal Plast Rec Surg
Ophthalmic Res
Ophthalmologica
Ophthalmology
Retina
Surv Ophthalmol
Ophthalmology Review Journal
Volume 4 Established 1995

Retina and Vitreous



Establishment and characterization of a retinal Muller cell line.
Sarthy VP; Crabb JW; French RP; Kennedy BN; Dutt K Brodjian SJ
Invest Ophthalmol Vis Sci 1998 Jan;39(1):212-6

PURPOSE: Primary cultures of Muller cells have proven useful in cell biologic, developmental, and electrophysiological studies of Muller cells. However, the limited lifetime of the primary cultures and contamination from non-neural cells have restricted the utility of these cultures. The aim of this study was to obtain an immortalized cell line that exhibits characteristics of Muller cells.

METHODS: Primary Muller cell cultures were prepared from retinas of rats exposed to 2 weeks of constant light. Cells were immortalized by transfection with simian virus 40. Single clones were obtained by repeatedly passaging cells using cloning wells. Immunocytochemical and immunoblotting studies were carried out with glial fibrillary acidic protein (GFAP)-specific and cellular retinaldehyde-binding protein (CRALBP)-specific antibodies. Transient transfections with CRALBP-luciferase constructs were performed by electroporation.

RESULTS: Oncogene transformation resulted in the establishment of a permanent cell line that could be readily propagated. Immunocytochemical and immunoblotting studies demonstrated that the Muller cell line, rMC-1, expressed both GFAP, a marker for reactive gliosis in Muller cells, and CRALBP, a marker for Muller cells in the adult retina. Transient transfection assays showed that promoter-proximal sequences of the CRALBP gene were able to stimulate reporter gene expression in rMC-1.

CONCLUSIONS: Viral oncogene transformation has been successfully used to isolate a permanent cell line that expresses Muller cell phenotype. The rMC-1 cells continue to express both induced and basal markers found in primary Muller cell cultures as well as in the retina. The availability of rMC-1 should facilitate gene expression studies in Muller cells and improve our understanding of Muller cell-neuron interactions.


Authors' abstarc, IOVS
Northwestern University Medical School,
Chicago, Illinois

[ ORJ-Subject ] [ ORJ-Date ] [ IO Home ] [ Retina ]



Retina and Vitreous



Acute retinal necrosis late in the second trimester
Shiraki K; Kanaoka Y; Miki T; Henmi K; Ataka S Moriwaki M
Am J Ophthalmol 1998 Jan;125(1):103-4

PURPOSE: To report treatment of a patient with acute retinal necrosis during pregnancy.

METHODS: A 24-year-old woman in her twenty-third week of gestation was diagnosed with acute retinal necrosis. A combination of acyclovir and interferon therapy was started at 25 weeks. Pars plana vitrectomy was performed during the 26th week of gestation.

RESULTS: The necrotizing retina became gliotic within 3 weeks of surgery. The patient's visual acuity improved to LE, 20/40. A healthy baby was delivered at 39 weeks of gestation.

CONCLUSION: Combination therapy of acyclovir and interferon followed by surgery partially restored the patient's vision without affecting fetal development.


Authors' abstract, AJO
Osaka City University Medical School,
Osaka, Japan

[ ORJ-Subject ] [ ORJ-Date ] [ IO Home ] [ Retina ]



Footer