Autoradiographic analysis on agar plates of antigens from subcellular fractions of rat liver slices.

W S MORGAN, P PERLMANN, T HULTIN
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引用次数: 33

Abstract

Slices of rat livers were incubated with 14C amino acids, homogenized, and subjected to differential centrifugation. The microsomes were further extracted with the non-ionic detergent Lubrol W and with EDTA. These extracts and the microsome free "cell sap," freed from the pH 5 precipitable fraction, were subsequently reacted with antisera using agar diffusion techniques. The antisera employed were obtained from rabbits injected with different subcellular fractions of rat liver or with rat serum proteins. When the agar diffusion plates were autoradiographed it was found that some of the precipitates were radioactive while others were not. Control experiments indicated that this labeling was due to the specific incorporation of (14)C amino acids into various rat liver antigens during incubation of the slices rather than to a non-specific adsorption of radioactive material to the immunological precipitates. When the slices were incubated with the isotope for up to 30 minutes, the serum proteins which could be extracted from the microsomes with the detergent were strongly labeled, as were a number of additional microsomal antigens of unknown significance. In contrast, the serum proteins present in the cell sap were only weakly labeled. Most of the typical cell sap proteins, both those precipitable and those soluble at pH 5, seemed to remain unlabeled. No consistently reproducible results were obtained with the EDTA extracts of the ribosomal residues remaining after extraction of the microsomes with the detergent. Incubation of the liver slices for longer periods (up to 120 minutes) led to a strong labeling of the serum proteins in the cell sap as well as to the appearance of labeling in additional cell sap proteins. The results are discussed with regard to the subcellular site of synthesis and the metabolism of the different antigens.

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大鼠肝切片亚细胞抗原琼脂板放射自显影分析。
用14C氨基酸孵育大鼠肝脏切片,匀浆,差速离心。用非离子洗涤剂Lubrol W和EDTA进一步提取微粒体。这些提取物和游离微粒体的“细胞液”,从pH 5可沉淀的部分中释放出来,随后使用琼脂扩散技术与抗血清反应。所采用的抗血清是用不同的大鼠肝脏亚细胞部分或大鼠血清蛋白注射兔获得的。当琼脂扩散板进行自放射线照相时,发现一些沉淀物具有放射性,而另一些则没有。对照实验表明,这种标记是由于(14)C氨基酸在切片孵育期间特异性结合到各种大鼠肝脏抗原中,而不是由于放射性物质对免疫沉淀的非特异性吸附。当切片与同位素孵育长达30分钟时,可以用洗涤剂从微粒体中提取的血清蛋白被强烈标记,许多其他未知意义的微粒体抗原也被标记。相比之下,存在于细胞液中的血清蛋白仅被弱标记。大多数典型的细胞液蛋白,包括可沉淀的和可在pH 5下溶解的,似乎都没有被标记。用洗涤剂提取微粒体后剩余的核糖体残留物的EDTA提取物没有获得一致的可重复性结果。肝切片孵育较长时间(长达120分钟)导致细胞液中血清蛋白的强标记,以及在其他细胞液蛋白中出现标记。结果讨论了亚细胞合成位点和不同抗原的代谢。
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