Your search keyword '"Kupila-Ahvenniemi, Sirkka"' showing total 3 results

1. Dependence of the quality and the in vitro translation capacity of pine ribosome assemblies on the isolation procedure.

Author

Kupila-Ahvenniemi, Sirkka, Muhonen, Aija, and Malinen, Paula

Subjects

*GENETIC translation, *SCOTS pine, *RIBOSOMES, *PLANT proteins, *PROTEOLYTIC enzymes, *SCANNING electron microscopy

Abstract

A study of the scanning electron micrographs gave the impression that the largest polymers and aggregates had broken down. Protease K (EC 3.4.21.14) when added to the grinding buffer also destroyed the ability of the ribosomes to maintain protein synthesis in vitro. In this case, the shape of the polysome profiles gave the impression of successful isolation. Clumps of ribosomes, presumably originating from large aggregates, were visible in the scanning electron micrographs. Triton X-100 and 0.25 M NaCl in the grinding buffer extracted chromatin, which affected the results. The material lost during the extraction and purification processes consisted mainly of monosomes and their sub-units. On the basis of the above results it was concluded that the preservation of large polysomes and ribosome aggregates in the isolated ribosome assemblies is necessary if they are to maintain a high translation capacity. The content of the assemblies was best revealed in the scanning electron micrographs. The shape of the polysome profiles did not always correlate with the ability of the isolated ribosomes to synthesize proteins.

Published

1987

2. Use of the scanning electron microscope in the study of isolated ribosomes and polysomes.

Author

Kupila-Ahvenniemi, Sirkka, Peura, Raija, and Häggman, Hely

Subjects

*SCOTS pine, *RIBOSOME structure, *RIBOSOMES, *SCANNING electron microscopes, *ELECTRON microscopy, *NUCLEOPROTEINS

Abstract

A procedure is described by which the ribosome assemblies isolated from the buds of Scots pine (Pinus sylvestris L.) as well as the ribosome and polysome fractions purified by sucrose density gradient centrifagation can be prepared for study by scanning electron microscopy. The technique has also been used to illustrate ribosomes extracted froai leaves and roots of Nicotiana tabacum L., from roots of Tuiipa gesneriana hybr. and from commercial wheat germ. The sample under study is spread on a piece of coverslip', frozen and dried at room temperature. The coverslip, with attached material, is taken through the critical point drying procedure, glued on a specimen retainer aod coated with gold‐palladium. The coverslip serves as a sufficiently stable specimen support to allow the study of ribosomes at magnifications of several hundred thousand. Use of the method makes it possible to study the structure of polysomes, to check the purity of fractioned samples and to investigate differences in the ribosome assembly of the developing plant tissues. [ABSTRACT FROM AUTHOR]

Published

1985

3. Variation in the polysome assembly and incorporation of [3H]-uridine in the cells of pine buds during the cold season.

Author

Häggman, Hely, Hohtola, Anja, and Kupila-Ahvenniemi, Sirkka

Subjects

SCOTS pine, RIBOSOMES, URIDINE, AGING, MESSENGER RNA, PLANT metabolism, PLANT physiology

Abstract

The ribosome assemblies isolated from buds of Scots pine (Pinus sylvestris L.) containing microsporangiate strobili varied both quantitatively and qualitatively in samples collected from October to April. The seasonal fluctuation in the amount of ribosonnes was more evident in the cytosolic fraction than in the smaller membrane‐bound fraction. The profiles obtained after sucrose density gradient centrifugation were of two types. One type was commonly obtained from samples collected late in the autumn and early in the spring, and this type was characterized by a relatively high peak for the large subunits, a low or negligible peak for the dimers, and an even or ascending series of peaks for the polymers. The other type was obtained from samples collected during the winter, and was characterized by small peaks for both subunits, a moderate to large peak for the dimers and a descending series of peaks for the polymers. However, the scanning electron microscope investigations indicated that the winter‐time samples did not lack polysomes and clusters of ribosomes. They did not become visible in the polysome profiles because they pelleted too tightly at the bottom of the centrifuge tubes to be removed with gradient fractionation. The au‐toradiographic analyses suggested that the cells were capable of synthesizing mRNA throughout the winter, whereas rRNA synthesis was arrested. On the basis of the above results, we postulate that the synthesis of the enzyme proteins needed for the maintenance of winter‐time metabolism takes place in the cytosolic ribosome fraction. The possible existence of winter‐time polysome stores is also pointed out. [ABSTRACT FROM AUTHOR]

Published

1985