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首页> 外文期刊>Cell transplantation >Cryopreservation of human pancreatic islets from non-heart-beating donors using hydroxyethyl starch and dimethyl sulfoxide as cryoprotectants.
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Cryopreservation of human pancreatic islets from non-heart-beating donors using hydroxyethyl starch and dimethyl sulfoxide as cryoprotectants.

机译:使用羟乙基淀粉和二甲基亚砜作为冷冻保护剂冷冻保存来自非心跳供体的人胰岛。

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摘要

Although widely used, DMSO is toxic for pancreatic islets. We combined hydroxyethyl starch (HES) with DMSO to simplify the procedure of freezing and thawing, and to decrease the toxicity of DMSO. A preclinical study was performed using islets from beagle dogs. After storage for 4 weeks, the islets were thawed and examined. The islet structure was well maintained after thawing. Although the number of the islets decreased to 71.2 +/- 20.1%, the function of the islets was evaluated by static incubation after thawing and showed a 1.80 +/- 0.78 stimulation index. We have introduced this technique for the cryopreservation of human islets from non-heart-beating donors. Twelve cases of human islet cryopreservation were performed. The sample tube of each human cryopreservation was thawed to evaluate the morphology, contamination, and endocrine function. Although fragmentation was observed in five samples (41.6%), the other seven (58.4%) showed a normal structure when evaluated by microscopic and electron microscopic study. The stimulation index (SI) of static incubation deteriorated from 3.37 +/- 3.02 to 1.34 +/- 0.28 after thawing. We divided the thawed islets into two groups: group 1 (n=8), SI > 1.2; group 2 (n=4), SI < 1.2. The group 1 islets showed a higher rate of normal structure (87%) than did group 2 (25%). Moreover, the SI before cryopreservation was 4.01 +/- 3.57 in group 1, which was higher than the SI of 2.11 +/- 0.72 in group 2. Based on the good results from the preclinical study using a large-animal model, this method was introduced for clinical application. Even from the pancreata of non-heart-beating donors, a successful islet cryopreservation was achieved. However, the isolated islets with poor function should not be cryopreserved for transplantation.
机译:尽管已广泛使用,但DMSO对胰岛有毒。我们将羟乙基淀粉(HES)与DMSO结合使用,以简化冷冻和解冻过程,并降低DMSO的毒性。临床前研究是使用比格犬的胰岛进行的。储存4周后,将胰岛融化并检查。解冻后,胰岛结构保持良好。尽管胰岛的数量减少到71.2 +/- 20.1%,但是通过解冻后的静态孵育评估了胰岛的功能,并显示了1.80 +/- 0.78的刺激指数。我们已经引入了这种技术,用于冷冻来自非心跳供体的人类胰岛。进行了十二例人类胰岛冷冻保存。解冻每个人冷冻保存的样品管,以评估其形态,污染和内分泌功能。尽管在五个样品(41.6%)中观察到碎片,但通过显微镜和电子显微镜研究评估时,其他七个(58.4%)显示出正常结构。解冻后,静态孵育的刺激指数(SI)从3.37 +/- 3.02降低至1.34 +/- 0.28。我们将融化的胰岛分为两组:第1组(n = 8),SI> 1.2;第2组(n = 4),SI <1.2。第1组胰岛的正常结构发生率(87%)比第2组(25%)高。此外,冷冻保存之前,第1组的SI为4.01 +/- 3.57,高于第2组的2.11 +/- 0.72。基于使用大动物模型进行的临床前研究的良好结果,该方法被引入临床应用。即使来自非心跳供体的胰腺,胰岛冷冻保存也成功实现了。但是,分离的功能不佳的胰岛不应冷冻保存用于移植。

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