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分离难以捉摸的胰岛。

Isolating the elusive islet.

作者信息

Scharp D W, Downing R, Merrell R C, Greider M

出版信息

Diabetes. 1980;29 Suppl 1:19-30. doi: 10.2337/diab.29.1.s19.

Abstract

The lack of a technique that allows mass isolation of intact, viable human islets is part of the reason that islet transplantation has not become available to the human diabetic. This report outlines the history of islet isolation and presents two new technical modifications that have been developed in the dog. Many of the current problems in islet isolation are presented, including the difficulty in obtaining enough human pancreatic tissue with minimal warm-ischemia time; inadequate distention of the pancreas to provide sufficient disruption for maximal enzymatic reaction to release intact islets; inefficient chopping methods; the use of collagenase of variable composition; different digestion methods for obtaining isolated islets; and inefficient methods for separating and purifying the islets from the ductal, acinar, and fibrous components. The first new modification involves distention of the dog pancreas through the venous system of the gland rather than the ductal system. This results in improved intralobular disruption, which improved the yield of isolated dog islets by permitting more efficient collagenase digestion. The second new modification eliminates the concept of isolating intact islets: the dog pancreas is digested by trypsin to a single-cell preparation that is partially purified by Ficoll gradients; further purification of the endocrine cells results from selective aggregation using rotational culture. This process produces pseudoislets that contain all the islet cell types and can be kept in culture for up to 4 wk, releasing their hormones in response to appropriate stimuli. These modifications may assist in the struggle to isolate the elusive human islet for safe and effective islet transplantation in the diabetic patient.

摘要

缺乏一种能够大量分离完整、有活力的人胰岛的技术,是胰岛移植尚未应用于糖尿病患者的部分原因。本报告概述了胰岛分离的历史,并介绍了在犬类中开发的两项新技术改进。文中阐述了当前胰岛分离中的许多问题,包括难以在最短热缺血时间内获取足够的人胰腺组织;胰腺扩张不足,无法提供足够的破坏以实现最大酶促反应来释放完整胰岛;切碎方法效率低下;使用成分各异的胶原酶;获取分离胰岛的不同消化方法;以及从导管、腺泡和纤维成分中分离和纯化胰岛的低效方法。第一项新改进是通过胰腺的静脉系统而非导管系统对犬胰腺进行扩张。这导致小叶内破坏得到改善,通过允许更有效的胶原酶消化提高了分离犬胰岛的产量。第二项新改进摒弃了分离完整胰岛的概念:将犬胰腺用胰蛋白酶消化成单细胞制剂,通过菲可梯度进行部分纯化;通过旋转培养的选择性聚集实现内分泌细胞的进一步纯化。这个过程产生含有所有胰岛细胞类型的假胰岛,并且可以在培养中保存长达4周,在适当刺激下释放其激素。这些改进可能有助于努力分离难以捉摸的人胰岛,以便在糖尿病患者中进行安全有效的胰岛移植。

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