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Human Pancreatic Islet Isolation: Part I: Digestion and Collection of Pancreatic Tissue

机译:人胰岛分离:第一部分:胰组织的消化和收集

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Management of Type 1 diabetes is burdensome, both to the individual and society, costing over 100 billion dollars annually. Despite the widespread use of glucose monitoring and new insulin formulations, many individuals still develop devastating secondary complications. Pancreatic islet transplantation can restore near normal glucose control in diabetic patients 1, without the risk of serious hypoglycemic episodes that are associated with intensive insulin therapy. Providing sufficient islet mass is important for successful islet transplantation. However, donor characteristic, organ procurement and preservation affect the isolation outcome 2. At University of Illinois at Chicago (UIC) we have developed a successful isolation protocol with an improved purification gradient 3. The program started in January 2004, and more than 300 isolations were performed up to November 2008. The pancreata were sent in cold preservation solutions (UW, University of Wisconsin or HTK, Histidine-Tryptophan Ketoglutarate) 4-7 to the Cell Isolation Laboratory at UIC for islet isolation. Pancreatic islets were isolated using the UIC method, which is a modified version of the method originally described by Ricordi et al8. Briefly, after cleaning the pancreas from the surrounding tissue, it was perfused with enzyme solution (Serva Collagenase + Neutral Protease or Sigma V enzyme). The distended pancreas was then transferred to the Ricordi digestion chamber, connected to a modified, closed circulation tubing system, and warmed up to 37°C. During the digestion, the chamber was shaken gently. Samples were taken continuously to monitor the digestion progress. Once free islets were detected under the microscope, the digestion was stopped by flushing cold (4°C) RPMI dilution solution (Mediatech, Herndon, VA) into the circulation system to dilute the enzyme. After being collected and washed in M199 media supplemented with human albumin, the tissue was sampled for pre-purification count and incubated with UW solution before purification. Purification process will be described in Part II: Purification and Culture of Human Islets.
机译:1型糖尿病的管理对个人和社会都是沉重的负担,每年花费超过1000亿美元。尽管广泛使用了葡萄糖监测和新的胰岛素制剂,但许多人仍然出现毁灭性的继发性并发症。胰岛移植可以使糖尿病患者1恢复到接近正常的血糖控制,而没有与强化胰岛素治疗相关的严重降糖事件的风险。提供足够的胰岛质量对于成功的胰岛移植很重要。但是,捐赠者的特征,器官的采购和保存会影响分离结果。2.在伊利诺伊大学芝加哥分校(UIC),我们已经开发出了成功的分离方案,纯化梯度得到了改善。3.该计划于2004年1月开始,已进行了300多次分离进行至2008年11月。将胰腺保存在冷藏溶液中(威斯康星大学或威斯康星大学或HTK,组氨酸-色氨酸酮戊二酸)4-7送至UIC的细胞分离实验室进行胰岛分离。使用UIC方法分离胰岛,UIC方法是Ricordi等[8]最初描述的方法的改良版本。简而言之,从周围组织清洁胰腺后,用酶溶液(Serva胶原酶+中性蛋白酶或Sigma V酶)灌注胰腺。然后将膨胀的胰腺转移至Ricordi消化室,连接至改良的封闭式循环管路系统,并加热至37°C。消化过程中,将培养箱轻轻摇动。连续取样以监测消化过程。在显微镜下检测到游离胰岛后,可通过将冷(4°C)RPMI稀释液(Mediatech,Herndon,VA)冲洗到循环系统中以稀释酶来终止消化。收集并在补充了人白蛋白的M199培养基中洗涤后,对组织取样以进行预纯化计数,并在纯化前与UW溶液一起孵育。纯化过程将在第二部分:人类胰岛的纯化和培养中描述。

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