Forward Light Scattering of the Vitreous Gel After Enzymatic Aging: An In Vitro Model to Study Vitreous Opacification.

Purpose: Symptomatic vitreous opacifications, so-called floaters, are difficult to objectively assess majorly limiting the possibility of in vitro studies. Forward light scattering was found previously to be increased in eyes with symptomatic floaters. Using an objective setup to measure forward light scattering, we studied the effects of enzymatically digesting the components of the vitreous body on straylight to develop an in vitro model of vitreous opacifications. Methods: Fifty-seven porcine vitreous bodies were digested using hyaluronidase, collagenase, trypsin, and bromelain, as well as using a combination of hyaluronidase + collagenase and hyaluronidase + bromelain. A modified C-Quant setup was used to objectively assess forward light scattering. Results: Depletion of hyaluronic acid majorly increased vitreous straylight (mean increase 34.4 deg2/sr; P = 0.01), whereas primarily digesting the vitreous gel with collagenase or trypsin did not significantly affect straylight. When collagenase or bromelain is applied in hyaluronic acid depleted vitreous gels, the increase in forward light scattering is reversed partially. Conclusions: The age-related loss of hyaluronic acid primarily drives the increase in vitreous gel straylight induced by conglomerates of collagen. This process can be reversed partially by digesting collagen. This in vitro model allows the objective quantification and statistical comparison of straylight burden caused by vitreous opacities and, thus, can serve as a first testing ground for pharmacological therapies, as demonstrated with bromelain.

A Novel Tendon Injury Model, Induced by Collagenase Administration Combined with a Thermo-Responsive Hydrogel in Rats, Reproduces the Pathogenesis of Human Degenerative Tendinopathy.

Patellar tendinopathy is a common clinical problem, but its underlying pathophysiology remains poorly understood, primarily due to the absence of a representative experimental model. The most widely used method to generate such a model is collagenase injection, although this method possesses limitations. We developed an optimized rat model of patellar tendinopathy via the ultrasound-guided injection of collagenase mixed with a thermo-responsive Pluronic hydrogel into the patellar tendon of sixty male Wistar rats. All analyses were carried out at 3, 7, 14, 30, and 60 days post-injury. We confirmed that our rat model reproduced the pathophysiology observed in human patients through analyses of ultrasonography, histology, immunofluorescence, and biomechanical parameters. Tendons that were injured by the injection of the collagenase-Pluronic mixture exhibited a significant increase in the cross-sectional area (p < 0.01), a high degree of tissue disorganization and hypercellularity, significantly strong neovascularization (p < 0.01), important changes in the levels of types I and III collagen expression, and the organization and presence of intra-tendinous calcifications. Decreases in the maximum rupture force and stiffness were also observed. These results demonstrate that our model replicates the key features observed in human patellar tendinopathy. Collagenase is evenly distributed, as the Pluronic hydrogel prevents its leakage and thus, damage to surrounding tissues. Therefore, this model is valuable for testing new treatments for patellar tendinopathy.

Comparative analysis of preparation of human hepatocytes by the ethylenediamine tetraacetic acid and collagenase technique

PURPOSE: To compare the viability of human hepatocytes dissociated by the ethylenediaminetetraacetic acid and collagenase techniques. METHODS: Hepatocytes were prepared by dissociation of liver fragments obtained from hepatectomies performed for therapeutic purposes at the Service of Digestive Tract Surgery, Federal University of Triângulo Mineiro. RESULTS: During the first 4 days of the experiment, 70 percent of the cells presented birefringent membranes and were not stained with 2 percent erythrosine, and were therefore considered to be viable. During the first 3 days, hepatocyte viability was on average 71 percent in the EDTA group and 76 percent in the collagenase group, with no significant difference between groups. No significant difference was observed between groups at any time. The secretion of albumin by the cultured hepatocytes was preserved up to the seventh day. Mean albumin secretion during the first 3 days was 50 æg/ml in the two groups and a reduction of albumin production was observed from the fourth to the seventh day. Again, no significant difference was observed between groups at any time. CONCLUSION: Cell viability and preservation of albumin secretion by hepatocytes are similar for the EDTA and collagenase techniques.

OBJETIVO: Comparar a viabilidade dos hepatócitos humanos dissociados pelas técnicas do ácido etilenodiaminotetracético e da colagenase. MÉTODOS: Hepatócitos foram preparados pela dissociação de fragmentos de fígado, provenientes de hepatectomias realizadas com o objetivo terapêutico no Serviço de Cirurgia do Aparelho Digestivo da Universidade Federal do Triângulo Mineiro. RESULTADOS: Detectou-se que nos quatro primeiros dias de experimento 70 por cento das células estavam com suas membranas biorrefringentes e não se coravam pela eritrosina a 2 por cento portanto foram consideradas viáveis. Observou-se que nos três primeiros dias a viabilidade dos hepatócitos foi em média 71 por cento no grupo EDTA e 76 por cento na colagenase, diferença esta sem significado estatístico entre os grupos. Em nenhum momento, detectou-se diferença estatística entre os grupos. Com relação a preservação da secreção de albumina pelos hepatócitos em cultura observou-se que foi mantida até o sétimo dia. Da mesma forma, notou-se que nos três primeiros dias a média de secreção de albumina de ambos os grupos foi de 50 ìg/dl e que após o quarto dia verificou-se redução da produção até o sétimo dia. Também não foi observado diferença significativa em nenhum momento entre os grupos. CONCLUSÃO: A viabilidade celular e a preservação da função de secretar albumina pelos hepatócitos são semelhantes pelas técnica do EDTA e da colagenase.

Aspectos morfológicos do processo de cicatrizaçäo em ratos albinos sob a açäo da colagenase / Morphologic features of cicatrization in august rats with the use of colagenase

Fez-se um estudo histológico sobre o uso da enzima colagena-se (clostrídio-peptidase A) associada a antibiótico (cloranfenicol), quando aplicada à pele de ratos, após a retirada de fragmento. A morfologia do tecido de reparação mostrou bons resultados após o uso dessa enzima. Os autores discutem as vantagens da utilização de enzimas na eliminação de áreas necróticas, acelerando a reparação de áreas lesadas.