首页> 外文期刊>Peritoneal dialysis international: Journal of the International Society for Peritoneal Dialysis >Temperature: the single most important factor for degradation of glucose fluids during storage.
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Temperature: the single most important factor for degradation of glucose fluids during storage.

机译:温度:储存期间葡萄糖液降解的最重要的单一因素。

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OBJECTIVE: Bioincompatible glucose degradation products (GDPs) develop during heat sterilization of peritoneal dialysis (PD) fluids. However, degradation may also take place during storage. Consequently, storage may add to the bioincompatibility caused by heat sterilization. The aim of the present study was to investigate how different factors such as the sterilization procedure, pH, glucose concentration, and temperature influence GDP production during storage. DESIGN: Degradation in glucose solutions was followed by pH and UV absorbance at 228 nm and 284 nm over 2 years of storage. Different sterilization times, storage temperatures, pH, and glucose concentrations were included in the study. Peritoneal dialysis fluids were also used in the experiment. Bioincompatibility was estimated through inhibition of cell growth in L-929 fibroblasts, and GDPs through UV absorption and liquid chromatography. RESULTS: The most important factor determining the rate of GDP production during storage was temperature. The GDPs created by heat sterilization promoted further degradation of glucose during subsequent storage. A pH of around 3.2 protected glucose from degradation during both heat sterilization and storage. At a storage temperature of 20 degrees C and a pH of 3.2, degradation was almost negligible. Heat sterilization produced considerable amounts of GDPs absorbing at 228 nm. During initial storage, these 228 nm-absorbing GDPs almost disappeared. After reaching a nadir, absorbance at 228 nm again started to increase. Contrary to this, absorbance at 284 nm [caused mainly by 5-hydroxymethyl-2-furaldehyde (5-HMF)] increased during the whole storage period. After 2 years at 40 degrees C, the concentrations of GDPs produced during storage were of the same magnitude as those caused by heat sterilization. Inhibition of cell growth of L-929 fibroblasts correlated well with the part of the absorbance at 228 nm not caused by 5-HMF in glucose solutions that were heat sterilized under a wide range of conditions. This part of228 nm absorbance (denoted 228corr) was caused almost entirely by 3,4-dideoxyglucosone-3-ene (3,4-DGE). CONCLUSIONS: Temperature is the single most important factor for glucose degradation during storage. The concentrations of bioincompatible GDPs produced may, under improper conditions, be as high as those produced during sterilization. High concentrations of glucose and low pH protect glucose from being degraded during both sterilization and storage. A good estimate of 3,4-DGE concentration in the fluids can be obtained correcting the UV absorbance at 228 nm for the influence from 5-HMF (and, when appropriate, for lactate). The 228corr may thus be used as a simple quality control for the fluids.
机译:目的:在腹膜透析液(PD)的热灭菌过程中会产生生物不相容的葡萄糖降解产物(GDPs)。但是,在存储过程中也可能发生降解。因此,储存可能增加由热灭菌引起的生物相容性。本研究的目的是研究不同的因素,例如灭菌程序,pH,葡萄糖浓度和温度如何影响存储过程中的GDP。设计:在葡萄糖溶液中降解后,在保存2年后会在228 nm和284 nm处进行pH和UV吸收。研究中包括不同的灭菌时间,储存温度,pH和葡萄糖浓度。腹膜透析液也用于实验中。通过抑制L-929成纤维细胞中的细胞生长来评估生物不相容性,并通过紫外线吸收和液相色谱来评估GDP。结果:决定存储期间GDP增长率的最重要因素是温度。通过热灭菌产生的GDP促进了后续存储过程中葡萄糖的进一步降解。大约3.2的pH值可防止葡萄糖在加热灭菌和储存过程中降解。在20摄氏度的存储温度和3.2的pH值下,降解几乎可以忽略不计。加热灭菌产生了大量的228 nm吸收的GDP。在初始存储期间,这些228 nm吸收的GDP几乎消失了。达到最低点后,在228 nm处的吸光度再次开始增加。与此相反,在整个存储期间,在284 nm处的吸光度[主要由5-羟甲基-2-呋喃醛(5-HMF)引起]增大。在40摄氏度下放置2年后,存储过程中产生的GDP浓度与热灭菌引起的浓度相同。 L-929成纤维细胞的细胞生长抑制与228 nm处的吸光度不是由5-HMF引起的,在广泛的条件下进行了热灭菌的葡萄糖溶液中的相关性很好。 228 nm吸光度的这一部分(表示为228corr)几乎完全由3,4-dideoxyglucosone-3-ene(3,4-DGE)引起。结论:温度是储存期间葡萄糖降解的最重要的单一因素。在不适当的条件下,产生的与生物不相容的GDP浓度可能与灭菌过程中产生的浓度不一样。高浓度的葡萄糖和低pH值可防止葡萄糖在灭菌和存储过程中降解。可以得到流体中3,4-DGE浓度的良好估算值,以校正5-HMF(以及在适当时适用于乳酸)的影响,校正228 nm处的UV吸光度。 228corr因此可以用作流体的简单质量控制。

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