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经氯胺-T法碘化的蛋白质在胞吞作用后似乎以异常快的速度降解。

Proteins iodinated by the chloramine-T method appear to be degraded at an abnormally rapid rate after endocytosis.

作者信息

Opresko L, Wiley H S, Wallace R A

出版信息

Proc Natl Acad Sci U S A. 1980 Mar;77(3):1556-60. doi: 10.1073/pnas.77.3.1556.

Abstract

Proteins labeled with either (3)H by reductive methylation or (125)I by the chloramine-T method were incubated with Xenopus laevis oocytes; the incorporation and acid precipitability of the proteins were then studied. The uptake rates of both specifically incorporated (vitellogenin) and nonspecifically incorporated proteins (bovine serum albumin and X. laevis serum proteins lacking albumin) were not influenced by the method of labeling. However, (125)I-labeled proteins were apparently degraded at rates far exceeding their (3)H-labeled counterparts, based on the generation of acid-soluble radioactivity. Thus, after a 3-hr incubation, 3-5 times more (125)I-labeled bovine serum albumin and X. laevis serum proteins lacking albumin were degraded than the corresponding (3)H-labeled proteins (95% compared to 30% and 75% compared to 15%, respectively), whereas after a 24-hr incubation, the degradation of (125)I-labeled vitellogenin was 15 times greater than that of [(3)H]vitellogenin labeled in vivo (60% compared to 4%). Moreover, examination of the relative amounts of (3)H- compared to (125)I-labeled bovine serum albumin deposited into the exogenously derived yolk platelet compartment of the oocyte revealed 7 times more acid-precipitable (3)H-labeled protein, indicating that the observed discrepancies were not due to reincorporation of the (3)H-labeled ligands. Passage of dissolved oocytes previously exposed to (125)I-labeled bovine serum albumin (chloramine-T method) over a column of Bio-Gel P-10 revealed some breakdown of bovine serum albumin to intermediate molecular weight components and the presence of a large amount ( approximately 90%) of labeled low molecular weight compounds, which analysis showed to be 72% free iodine. The evolution of either iodotyrosine or free iodine would nevertheless be perceived as protein degradation by most analytical procedures (e.g., acid precipitation or autoradiography). We conclude, therefore, that apparent degradation rates observed for endocytotically incorporated proteins may vary depending on the method used to label the protein and caution should be exercised when interpreting results obtained with labeled, particularly chloramine-T labeled, proteins.

摘要

用还原甲基化法标记有³H或用氯胺-T法标记有¹²⁵I的蛋白质与非洲爪蟾卵母细胞一起孵育;然后研究蛋白质的掺入情况和酸沉淀性。特异性掺入的蛋白质(卵黄生成素)和非特异性掺入的蛋白质(牛血清白蛋白和缺乏白蛋白的非洲爪蟾血清蛋白)的摄取率均不受标记方法的影响。然而,基于酸溶性放射性的产生,¹²⁵I标记的蛋白质的降解速率显然远远超过其³H标记的对应物。因此,孵育3小时后,¹²⁵I标记的牛血清白蛋白和缺乏白蛋白的非洲爪蟾血清蛋白的降解量比相应的³H标记的蛋白质多3至5倍(分别为95%对30%和75%对15%),而孵育24小时后,¹²⁵I标记的卵黄生成素的降解量比体内标记的[³H]卵黄生成素大15倍(60%对4%)。此外,对沉积在卵母细胞外源卵黄小体区室中的³H标记与¹²⁵I标记的牛血清白蛋白的相对量进行检测发现,酸沉淀性³H标记的蛋白质多7倍,这表明观察到的差异并非由于³H标记配体的再掺入。将先前暴露于¹²⁵I标记的牛血清白蛋白(氯胺-T法)的溶解卵母细胞通过Bio-Gel P-10柱,发现牛血清白蛋白有一些降解为中等分子量成分,并且存在大量(约90%)标记的低分子量化合物,分析表明其中72%为游离碘。然而,在大多数分析程序(例如酸沉淀或放射自显影)中,碘酪氨酸或游离碘的释放都会被视为蛋白质降解。因此,我们得出结论,内吞掺入蛋白质的表观降解速率可能因标记蛋白质的方法而异,在解释用标记蛋白质(特别是氯胺-T标记的蛋白质)获得的结果时应谨慎。

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