高比活性生物活性单- 125i胰岛素的制备。

Acta physiologica latino americana Pub Date : 1981-01-01
J C Cresto, D P Udrisar, M C Camberos, J C Basabe, P Gómez Acuña, S F de Majo
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引用次数: 0

摘要

猪肉胰岛素用氯胺T技术(磷酸缓冲液0.25 M;pH值7.5;Edta 0.001 m;氯胺T: 0.2625 mg/ml;焦亚硫酸钠2.4 mg/ml),反应体积为50微升,每30秒加入氯胺T两次(1分钟2.1微克),用5微升焦亚硫酸钠停止反应。在制备淀粉凝胶中分离三个部分:F1(受冷胰岛素污染的单125i -胰岛素)、F2(未受冷胰岛素污染的单125i -胰岛素)和F3 (di- 125i -胰岛素)。制备低比活性和高比活性的胰岛素(碘/胰岛素比分别为0.1/1和1/1)用于研究,并通过抗体和肝细胞的剂量反应曲线来评估质量。利用Scatchard’s曲线得到F2的比活性分别为323和382 mCi/mg。F1的比活性随冷胰岛素污染程度的不同而变化。在碘/胰岛素比为1/1或附近地区,观察到F2 B/F比值的降低。无论特异性活性如何,F3的质量、免疫反应性及其B/F比值均不变。通过观察肝细胞的摄取和分离的脂肪细胞的葡萄糖消耗,证实了抗体的行为。综上所述,在制备淀粉凝胶中,以0.1/1的碘/胰岛素比例标记的F2从冷胰岛素中分离出来,从而提高了其比活性(约360 mCi/mg),而不改变其免疫和生物学特性。
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Preparation of biologically active mono-125I-insulin of high specific activity.

Pork insulin was labeled by the chloramine T technique (phosphate buffer 0.25 M; pH 7.5; EDTA 0.001 M; chloramine T: 0.2625 mg/ml; sodium metabisulfite 2.4 mg/ml) in a reaction volume of 50 microliters, adding chloramine T every 30 seconds twice (2.1 micrograms in 1 minute) and halting the reaction with 5 microliters metabisulfite. Three fractions were separated in preparative starch gel: F1 (mono-125I-insulin contaminated with cold insulin), F2 (mono-125I-insulin free from cold insulin), and F3 (di-125I-insulin). Insulins with low and high specific activity (iodine/insulin ratios 0.1/1 and 1/1 respectively) were prepared for study purposes, and quality was assessed by means of dose-response curves with antibodies and with liver cells. Specific activity of F2 as obtained from dose-response curves utilizing Scatchard's plot was 323 and 382 mCi/mg. Specific activity of F1 varied according to the extent of contamination with cold insulin. A reduction in the F2 B/F ratio was observed upon iodination with iodine/insulin ratios of 1/1 or in the neighborhood. The mass and immunoreactivity of F3, as well as its B/F ratios were constant, regardless of specific activity. The behavior with antibodies was ratified upon observations on uptake by liver cells and glucose consumption by isolated fat cells. In conclusion, F2 labeled with 0.1/1 iodine/insulin ratios was separated from cold insulin in preparative starch gel, thus increasing its specific activity (360 mCi/mg approximately) without alteration of its immunologic or biologic properties.

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