On the localization of polyribosomes in the system of chloroplast lamellae

From chloroplasts of 10-day-old pea seedlings exposed to the light for 19 h, two fractions have been isolated. One of them is rich in lamellae of the stroma, and the other is rich in thylakoids and fragments of the grana. These fractions have been obtained after centrifugation of chloroplasts disrupted by osmotic shock in a discontinuous sucrose gradient. The fraction containing thylakoids of grana differs from the fraction of lamellae of the stroma in its higher content of RNA and DNA as related to protein and in the capacity to incorporate intensively ¹⁴C amino acids into proteins. After its treatment with detergents (0.5% sodium deoxycholate and 0.4% Triton X-100) and repeated centrifugation in the discontinuous sucrose gradient it dissociates further into two fractions. During electron microscopic studies one of these fractions displays partially disrupted grana and the other exhibits extensive networks of polyribosomes incompletely liberated from proteins, including the de novo synthesized protein.The similar treatment of the fraction rich in lamellae of the stroma does not result in the liberation of polyribosomes.It is concluded that in this stage of chloroplast development, polyribosomes occurring in the lamellae system are localized in the thylakoids of grana and are not bound to lamellae of the stroma.     

Localization and Organization of the Translational Apparatus in Mitochondrial Membranes of Astasia longa

In isolated mitochondrial membranes of Astasia longa, large and small circular substructures were observed with diameters of 1.30 and 0.35 m and thickness of 0.08 and 0.03 m, respectively. Such substructures were isolated by membrane treatment with proteolytic enzymes (proteinase K, trypsin) or by lipid solubilization with Triton X-100. After the removal of surface protein layer, we uncovered circular polyribosomes with similar diameters as those of original substructures. Polyribosomes were identified on the basis of their morphology, positive staining with uranyl acetate, a capacity for chloramphenicol-sensitive incorporation of ¹⁴C-amino acids into polypeptides, and from their buoyant density as estimated by equilibrium centrifugation in the CsCl density gradient. The conclusion is that, in mitochondrial membranes of A. longa, the translational apparatus is organized similarly to that in the membranes of chloroplasts and cyanobacteria, e.g., large and small circular polyribosomes situated within the membrane ring-shaped substructures are the basics for the formation of the latter.