R A Thoft

Increased aggrecan (cartilage proteoglycan) production in the sclera of myopic chicks

A previously characterized chick model of myopia was used to evaluate biochemical changes in the sclera which are associated with ocular enlargement and myopia. Chicks were monocularly occluded for 10 days and the DNA, hydroxyproline, and glycosaminoglycan contents of the sclera were compared between the normal and the myopic eyes. No significant differences could be detected in total DNA or hydroxyproline content. There was, however, a 34% increase in glycosaminoglycans and a 20.7% decrease in cell density within the posterior sclera of myopic eyes. The biosynthesis of scleral proteoglycans was determined by measuring 35SO4 incorporation in the sclera of chicks visually occluded for 5, 10, and 15 days. No differences could be detected in 35SO4 incorporation into the cornea or the anterior sclera. However, 35SO4 incorporation was significantly increased in the posterior sclera of myopic eyes by 64% at Day 5, 39% at Day 10, and 49% at Day 15. When fractionated on Sepharose CL-4B, scleral proteoglycans were resolved into two peaks which were identified by Western blot analysis as aggrecan (cartilage proteoglycan) and decorin. Furthermore, Western blot and dot blot analyses indicated that significantly more aggrecan core protein was present in the sclera of myopic eyes compared with equivalent amounts of sclera from control eyes. These results indicate that increased synthesis and accumulation of aggrecan, which increases the volume of extracellular matrix in the posterior sclera, are responsible for the ocular enlargement observed in this model of myopia.

The multipotential cells of the limbus.

Ample evidence exists that there is a centripetal movement of cells from the periphery of the cornea toward the centre. While conjunctival cells have the capacity to transdifferentiate into corneal epithelial cells, the limbal region appears to act as a barrier between the conjunctival and corneal epithelia, even after large epithelial defects are created.The existence of limbal stem cells is suggested by the apparent role of the limbus in acting as a source of peripheral corneal cells. While specific staining of limbal cells has been reported in the rabbit, there is no positive identification of such stem cells in the human. However, in the human there is negative staining for both a keratin cytoskeleton antigen and a cell surface antigen in the limbal epithelial zone. Efforts positively to identify human limbal stem cells continue, as do efforts to culture and transplant such cells.

Conjunctival epithelial cell hypermitosis and goblet cell hyperplasia in atopic keratoconjunctivitis.

Atopic diseases that include eczema (atopic dermatitis), asthma, and seasonal and perennial rhinoconjunctivitis are common manifestations of abnormal immediate hypersensitivity. Ocular involvement, such as atopic keratoconjunctivitis, characteristically includes conjunctival and corneal inflammation, and in a severe form, conjunctival scarring, symblepharon, corneal epitheliopathy, and visual loss. To examine the conjunctival cellular abnormalities in atopic keratoconjunctivitis, we studied the in vivo differentiation and tissue-culture growth characteristics of conjunctiva from normal subjects and patients with severe atopic keratoconjunctivitis. We examined conjunctival biopsy specimens to determine epithelial mitotic rate and goblet cell frequency, and we studied conjunctival explants to determine the latent period for fibroblast outgrowth and fibroblast doubling time. The mitotic rate for atopic keratoconjunctivitis, 6.7% +/- 2.1% (11 patients), was statistically significantly greater than for normal subjects, 2.0% +/- 0.63% (seven subjects) (P = .05). Also the goblet cell frequency for atopic keratoconjunctivitis, 14.6% +/- 3.4% (11 patients), was statistically significantly greater than for normal subjects, 4.8% +/- 0.92% (seven subjects) (P = .02). The latent period for fibroblast outgrowth and the fibroblast doubling time for atopic keratoconjunctivitis were not statistically significantly different from normal control subjects. Therefore, atopic keratoconjunctivitis was associated with conjunctival epithelial hypermitosis, goblet cell hyperplasia, and normal fibroblast tissue-culture growth. These characteristics may be useful in the diagnosis of atopic keratoconjunctivitis. We previously studied another disease characterized by chronic conjunctival inflammation and scarring, cicatricial pemphigoid, which also demonstrated conjunctival epithelial hypermitosis, but in contrast there was near absence of goblet cells, and the fibroblasts were hyperproliferative. These differences may be used to distinguish atopic keratoconjunctivitis from cicatricial pemphigoid.

The role of the limbus in ocular surface maintenance and repair

Abstract Since Claes Dohlmans original treatise on the corneal epithelium, a great deal has been learned about the biology of that layer. Its maintenance depends in part on centripetal movement of cells from the periphery toward the center. To some degree the supply of these peripheral cells appears to be dependent on the proliferation of cells at the limbus, from so‐called ‘stem cells’. Studies of stem cell replication and differentiation of their progeny will lead undoubtedly to new insights into the the machanisms responsible for many of the chronic abnormalities of the central corneal surface.

Rapid Diagnostec Test for Ocular Adenovirus

A new, direct, enzyme immunoassay test (Adenoclone, Cambridge BioScience, Hopkinton, MA) was evaluated for the rapid diagnosis of ocular adenovirus infections. In 36 culture-proven cases of adenovirus ocular infection, direct Adenoclone testing of conjunctival swabs was positive in 24 of 31 patients (77%) tested within 1 week of onset of symptoms, and in one of five patients (20%) who presented after 1 week (P less than 0.02). Overall sensitivity was 69%, whereas specificity was 100%. The authors conclude that a positive Adenoclone test is reliable in the rapid diagnosis of early adenovirus ocular infections.

Clinical and Subclinical Ophthalmic Findings with Retinol Deficiency

BACKGROUND Patients at risk for retinol deficiency in developed countries include those with hepatic dysfunction and malabsorption states. Symptoms of retinol deficiency may go unrecognized or unreported. METHODS The authors describe 15 patients with hepatic dysfunction, two of whom had procedures that would predispose to malabsorption and were ophthalmologically symptomatic of retinol depletion. The other 13 patients were ophthalmologically asymptomatic liver transplant candidates examined prospectively for subclinical evidence of retinol deficiency. Combined laboratory analysis, Schirmers testing, conjunctival impression cytology, and electroretinography were performed. RESULTS Twelve of 15 patients had serum retinol levels below the lower limit of normal. Aqueous tear production was reduced in 7 of 14 patients. Abnormal conjunctival morphology was noted in 6 of 12 patients. Electroretinograms were abnormal in the two patients who were visually symptomatic and in seven of nine patients who were ophthalmologically asymptomatic. CONCLUSION Subclinical, physiologically significant retinol deficiency may be a frequent and unrecognized problem among patients with hepatic dysfunction.

Unique Parameters in the Healing of Linear Partial Thickness Penetrating Corneal Incisions in Rabbit: Immunohistochemical Evaluation

The healing of penetrating nonperforating linear corneal incisions in rabbit was analysed immunohistochemically. Regeneration of the basement membrane (BM) zone was evaluated by analysing the following components using monoclonal antibodies (MAbs): 1) an antigen designated AgHEBM1 (a 66k Mr polypeptide), 2) type VII collagen which is associated with anchoring fibrils and 3) an antigen designated Ag63/D7 which is associated with the lamina densa and anchoring plaques. Concomitant activity in the regenerating stroma was evaluated by analysing the distribution of 1) fibronectin, 2) keratan sulfate and 3) a fetal antigen, designated AgM12, (an intermediate filament associated protein with a Mr of 130k). Synthesis of the BM zone components was not evident at day 2 postwounding but was seen at day 7, only at the deepest aspects of the wounds. Re-establishment of a continuous BM zone was evident by day 60. The stromal regeneration had started by day 7, at the deepest aspect of the wounds, as judged from the distribution of stromal antigens including the fetal antigen AgM12. The number of activated cells (cells expressing AgM12) had decreased significantly by day 30 and diminished by day 60. Between day 30 and day 180 the thickness of the regenerated tissues had not increased significantly although the stroma had not yet reached its normal thickness. Even after six months, the epithelial plug persisted and the concentration of the sulfated epitopes of keratan sulfates in the regenerated stromal matrix were less than in the surrounding nonwounded regions. The cessation of expression of AgM12, by the cells in regenerating stroma, coincided with the relative decrease in extracellular matrix syntheses. The return of the stromal cells to the quiescent state also coincided with re-establishment of a continuous BM zone between the epithelium and the stroma in the regenerated tissue. These observations suggested that the synthesis, assembly and remodeling of stromal and epithelial extracellular matrices during the healing of penetrating corneal wounds may be influenced by the interactions between activated stromal cells and epithelial cells.