Pryme I F
Mol Cell Biochem. 1986 Jun;71(1):3-18. doi: 10.1007/BF00219323.
It has become evident during recent years that a wide variety of proteins are synthesized on membrane-bound polysomes, very many of which are not ultimately secreted from the cell. The majority of proteins appear to go through some form of post-translational modification before the final appearance of an 'active' product, and in some cases the polypeptide chain may be modified before the completed protein molecule is released from the ribosome. This then raises the question concerning the possibility of the organization of the rough endoplasmic reticulum into individual domains, or compartments, each of which may have the responsibility of performing definite and well defined functions. During recent years the behaviour of two subfractions of the rough endoplasmic reticulum in a variety of cell types and under a variety of conditions has been studied in order to gain insight into a possible compartmentation of this organelle. Throughout the studies disruption of cells has been performed by nitrogen cavitation. This technique was chosen in order to provide conditions of homogenization which were extremely reproducible since shearing forces, mechanical damage and the effects of local heating were eliminated. Endoplasmic reticulum (ER) membranes isolated from the post-mitochondrial supernatant have been separated into subfractions by centrifugation on discontinuous sucrose gradients. By virtue of their high density imparted by the association of ribosomes, rough ER (RER) membranes penetrate 1.4 M sucrose accumulating above either 2.0 M sucrose (light rough -LR membranes) or a cushion of 2.3 M sucrose (heavy rough -HR membranes). Smooth (S) membranes, which are virtually devoid of ribosomes, collect above 1.4 M sucrose. The HR, LR and S subfractions in MPC-11 cells differ in a number of respects: RNA/protein and RNA/phospholipid ratios, polysome profiles and marker enzymes. When cells were homogenized in buffer containing 25 mM KCl then all three ER subfractions were observed, however, when the buffer contained 100 mM KCl then only the LR and S subfractions were observed in gradients, radioactivity equivalent to that in the HR fraction was not recovered in the other two subfractions. Four times as many light chain immunoglobulin polypeptides were found associated with polysomes of HR membranes compared to LR membranes. The nuclear associated ER (NER), though very active in protein synthesis, was only 20% as active in the synthesis of light chain as the combined LR/HR fraction. Studies with MPC-11 cells showed that the relative amounts of the three ER subfractions were related to the phase of the cell cycle.(ABSTRACT TRUNCATED AT 400 WORDS)
近年来已变得明显的是,多种蛋白质是在膜结合多核糖体上合成的,其中很多最终并未从细胞中分泌出去。大多数蛋白质在“活性”产物最终出现之前似乎都经历了某种形式的翻译后修饰,而且在某些情况下,多肽链可能在完整的蛋白质分子从核糖体释放之前就已被修饰。这就进而引发了一个问题:粗面内质网是否有可能被组织成各个区域或隔室,每个区域或隔室可能负责执行特定且明确的功能。近年来,为了深入了解这种细胞器可能存在的区室化情况,对多种细胞类型在各种条件下粗面内质网的两个亚组分的行为进行了研究。在整个研究过程中,细胞的破碎是通过氮空化来进行的。选择这种技术是为了提供高度可重复的匀浆条件,因为消除了剪切力、机械损伤和局部加热的影响。从线粒体后上清液中分离出的内质网(ER)膜通过在不连续蔗糖梯度上离心被分离成亚组分。由于核糖体的结合赋予了粗面内质网(RER)膜较高的密度,它们会穿透1.4 M蔗糖,聚集在2.0 M蔗糖上方(轻粗面 -LR膜)或2.3 M蔗糖的垫层上方(重粗面 -HR膜)。几乎不含核糖体的滑面(S)膜则聚集在1.4 M蔗糖上方。MPC - 11细胞中的HR、LR和S亚组分在多个方面存在差异:RNA/蛋白质和RNA/磷脂比率、多核糖体图谱以及标记酶。当细胞在含有25 mM KCl的缓冲液中匀浆时,能观察到所有三个内质网亚组分,然而,当缓冲液含有100 mM KCl时,在梯度中仅观察到LR和S亚组分,与HR组分相当的放射性在其他两个亚组分中未被回收。与LR膜相比,发现与HR膜多核糖体相关的轻链免疫球蛋白多肽数量多四倍。核相关内质网(NER)虽然在蛋白质合成方面非常活跃,但在轻链合成方面的活性仅为LR/HR组合组分的20%。对MPC - 11细胞的研究表明,三个内质网亚组分的相对含量与细胞周期阶段有关。(摘要截断于400字)
