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一些与蛋白质超声雾化相关的因素。

Some factors associated with the ultrasonic nebulization of proteins.

作者信息

Niven R W, Ip A Y, Mittelman S, Prestrelski S J, Arakawa T

机构信息

Amgen Inc., Thousand Oaks, California 91320, USA.

出版信息

Pharm Res. 1995 Jan;12(1):53-9. doi: 10.1023/a:1016282502954.

Abstract

Ultrasonic nebulization of lactate dehydrogenase (LDH) was investigated using a DeVilbiss "Aerosonic" nebulizer. The enzyme (8ml, 0.025 mg/ml Na2HPO4, pH 7.0) was completely inactivated after 20 minutes of operation. However, the inactivation profile observed during ultrasonic nebulization was different from that previously observed using air-jet nebulization. At least two mechanisms are involved, one associated with heating and the other with aerosol production. By preventing heating of the nebulizer fluid during operation, the denaturation profile was dramatically altered. By additionally including 0.01% w/v Tween 80 or 1% w/v PEG 8000, almost all activity was retained. Similar results were obtained by preventing aerosol production and heating. However, 100% of activity was lost when heating was allowed to occur without aerosol formation. The results demonstrate that cooling in conjunction with a surfactant is one approach that could be used to stabilize proteins to ultrasonic nebulization. However, cooling also significantly reduced solute output from the nebulizer. When operated at 10 degrees C output was negligible. At 50 degrees C the output was 5x greater than that found at room temperature. The median droplet size (micron(s)) was not significantly influenced by the operating temperature of the nebulizer fluid (3.6 +/- 0.4, 21 degrees C; 3.9 +/- 0.2, 50 degrees C, p = NS (n = 6)) although the size distribution was noted to increase at the higher temperature.

摘要

使用德维比斯“Aerosonic”雾化器对乳酸脱氢酶(LDH)进行超声雾化研究。在运行20分钟后,该酶(8毫升,0.025毫克/毫升Na2HPO4,pH 7.0)完全失活。然而,超声雾化过程中观察到的失活情况与之前使用空气喷射雾化时观察到的不同。至少涉及两种机制,一种与加热有关,另一种与气溶胶产生有关。通过在运行过程中防止雾化器液体加热,变性情况发生了显著改变。通过额外添加0.01% w/v吐温80或1% w/v聚乙二醇8000,几乎保留了所有活性。通过防止气溶胶产生和加热也获得了类似结果。然而,当允许加热但不形成气溶胶时,100%的活性丧失。结果表明,结合表面活性剂进行冷却可能是一种用于使蛋白质对超声雾化稳定的方法。然而,冷却也显著降低了雾化器的溶质输出。在10摄氏度运行时输出可忽略不计。在50摄氏度时,输出比室温下高5倍。雾化器液体的运行温度对中位液滴尺寸(微米)没有显著影响(21摄氏度时为3.6±0.4;50摄氏度时为3.9±0.2,p =无显著差异(n = 6)),尽管在较高温度下尺寸分布有所增加。

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