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A surgical cryoprobe for targeted transcorneal freezing and endothelial cell removal

机译:用于靶向经角膜冷冻和内皮细胞去除的手术冷冻探针

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摘要

Purpose. To examine the effects of transcorneal freezing using a new cryoprobe designed for corneal endothelial surgery. Methods. A freezing console employing nitrous oxide as a cryogen was used to cool a series of different cryoprobe tip designs made of silver for high thermal conductivity. In vitro studies were conducted on 426 porcine corneas, followed by preliminary in vivo investigations on three rabbit corneas. Results. The corneal epithelium was destroyed by transcorneal freezing, as expected; however, the epithelial basement membrane remained intact. Reproducible endothelial damage was optimally achieved using a 3.4 mm diameter cryoprobe with a concave tip profile. Stromal edema was seen in the pre-Descemet’s area 24 hrs postfreeze injury, but this had been resolved by 10 days postfreeze. A normal collagen fibril structure was seen 1 month postfreeze, concurrent with endothelial cell repopulation. Conclusions. Transcorneal freezing induces transient posterior stromal edema and some residual deep stromal haze but leaves the epithelial basement membrane intact, which is likely to be important for corneal re-epithelialization. Localized destruction of the endothelial monolayer was achieved in a consistent manner with a 3.4 mm diameter/concave profile cryoprobe and represents a potentially useful approach to remove dysfunctional corneal endothelial cells from corneas with endothelial dysfunction.
机译:目的。为了研究使用为角膜内皮手术设计的新型冷冻探头进行的角膜冷冻效果。方法。使用一氧化二氮作为冷冻剂的冷冻控制台用于冷却由银制成的一系列不同的冷冻探针尖端设计,以实现高导热性。在426个猪角膜上进行了体外研究,然后对3个兔子角膜进行了初步的体内研究。结果。如所预期的,角膜上皮被经角膜冷冻破坏了;然而,上皮基底膜保持完整。使用直径为3.4毫米且尖端为凹形的冷冻探针可最佳地实现可再现的内皮损伤。冷冻后24小时内,在Descemet前区可见间质水肿,但冷冻后10天即可解决。冷冻后1个月,胶原蛋白原纤维结构正常,同时内皮细胞重新聚集。结论。经角膜冷冻诱发短暂的后间质水肿和一些残留的深层间质雾,但使上皮基底膜完好无损,这可能对角膜重新上皮形成很重要。内皮细胞单层的局部破坏是通过直径3.4毫米/凹形的冷冻探头以一致的方式实现的,它代表了一种从具有内皮功能障碍的角膜中去除功能不良的角膜内皮细胞的潜在有用方法。

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