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与核糖体结合相关的糙面微粒体膜蛋白。II. 结合的核糖体与结合位点处暴露的特定膜蛋白的交联。

Proteins of rough microsomal membranes related to ribosome binding. II. Cross-linking of bound ribosomes to specific membrane proteins exposed at the binding sites.

作者信息

Kreibich G, Freienstein C M, Pereyra B N, Ulrich B L, Sabatini D D

出版信息

J Cell Biol. 1978 May;77(2):488-506. doi: 10.1083/jcb.77.2.488.

Abstract

Two proteins (ribophorins I and II), which are integral components of rough microsomal membranes and appear to be related to the bound ribosomes, were shown to be exposed on the surface of rat liver rough microsomes (RM) and to be in close proximity to the bound ribosomes. Both proteins were labeled when intact RM were incubated with a lactoperoxidase iodinating system, but only ribophorin I was digested during mild trypsinization of intact RM. Ribophorin II (63,000 daltons) was only proteolyzed when the luminal face of the microsomal vesicles was made accessible to trypsin by the addition of sublytical detergent concentrations. Only 30--40% of the bound ribosomes were released during trypsinization on intact RM, but ribosome release was almost complete in the presence of low detergent concentrations. Very low glutaraldehyde concentrations (0.005--0.02%) led to the preferential cross-linking of large ribosomal subunits of bound ribosomes to the microsomal membranes. This cross-linking prevented the release of subunits caused by puromycin in media of high ionic strength, but not the incorporation of [3H]puromycin into nascent polypeptide chains. SDS-acrylamide gel electrophoresis of cross-linked samples a preferential reduction in the intensity of the bands representing the ribophorins and the formation of aggregates which did not penetrate into the gels. At low methyl-4-mercaptobutyrimidate (MMB) concentrations (0.26 mg/ml) only 30% of the ribosomes were cross-linked to the microsomal membranes, as shown by the puromycin-KCl test, but membranes could still be solubilized with 1% DOC. This allowed the isolation of the ribophorins together with the sedimentable ribosomes, as was shown by electrophoresis of the sediments after disruption of the cross-links by reduction. Experiments with RM which contained only inactive ribosomes showed that the presence of nascent chains was not necessary for the reversible cross-linking of ribosomes to the membranes. These observations suggest that ribophorins are in close proximity to the bound ribosomes, as may be expected from components of the ribosome-binding sites.

摘要

两种蛋白质(核糖体结合糖蛋白I和II)是糙面微粒体膜的组成成分,似乎与结合核糖体有关,已证明它们暴露于大鼠肝脏糙面微粒体(RM)表面,且与结合核糖体紧密相邻。当完整的RM与乳过氧化物酶碘化系统一起孵育时,这两种蛋白质都被标记,但在完整RM的温和胰蛋白酶消化过程中,只有核糖体结合糖蛋白I被消化。只有当通过添加亚裂解浓度的去污剂使微粒体囊泡的腔面可被胰蛋白酶作用时,核糖体结合糖蛋白II(63,000道尔顿)才会被蛋白水解。在完整RM的胰蛋白酶消化过程中,只有30% - 40%的结合核糖体被释放,但在低去污剂浓度存在时,核糖体释放几乎是完全的。极低浓度的戊二醛(0.005% - 0.02%)导致结合核糖体的大亚基优先与微粒体膜交联。这种交联阻止了在高离子强度介质中由嘌呤霉素引起的亚基释放,但不影响[3H]嘌呤霉素掺入新生多肽链。交联样品的SDS - 聚丙烯酰胺凝胶电泳显示,代表核糖体结合糖蛋白的条带强度优先降低,并且形成了不渗透凝胶的聚集体。在低浓度的4 - 巯基丁酸甲酯(MMB)(0.26 mg/ml)时,如嘌呤霉素 - 氯化钾试验所示,只有30%的核糖体与微粒体膜交联,但膜仍可用1%的脱氧胆酸钠溶解。这使得核糖体结合糖蛋白与可沉降的核糖体一起被分离,还原破坏交联后沉淀物的电泳显示了这一点。用只含有无活性核糖体的RM进行的实验表明,新生链的存在对于核糖体与膜的可逆交联不是必需的。这些观察结果表明,核糖体结合糖蛋白与结合核糖体紧密相邻,这正如核糖体结合位点的组成成分所预期的那样。

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