A radioautographic study on RNA synthesis in aging mouse spleen after 3H-uridine labeling in vitro.

EM radioautographic study on RNA synthesis in aging mouse spleen was conducted after 3H-uridine labeling in vitro. The localization of radiolabelled precursor was used to determine the site of RNA synthesis. The site of the radiolabelled uridine uptake was localized in the haematopoietic cells, particularly in the lymphoblasts. In the labelled cells, most of the silver grains were localized in the nucleus, specifically in the euchromatin. Few cytoplasmic organelles such as the mitochondria and endoplasmic reticulum were labelled with 3H-uridine. Silver grains were also observed over the nucleoli. The labeling index was expressed as the percentage of labelled cells over the total number of cells counted. The labeling index increased from day one after birth and progressively until the 14th day. Thereafter, the labeling index decreased gradually until the 10th month. A significant difference of p less than 0.05 was noted. In all the EMRAG analyzed, it was observed that the number of silver grains per cell increased proportionally with the labeling index. The result of the quantitation of the changes in RNA synthesis correlated well with the maturational development/aging of the animal.     

The Incorporation of Phenylalanine and Uridine in Tetrahymena: A Pressure Study1

SYNOPSIS. The action of pressure was studied on the incorporation of labelled phenylalanine and uridine, and on the synthesis of water-soluble proteins in heat-synchronized Tetrahymena pyriformis. Incorporation of [¹⁴C] phenylalanine and [³H] uridine into TCA insoluble fractions was markedly decreased in pressuretreated Tetrahymena. Moreover, the incorporation was dependent upon the age of the cells. Water-soluble protein synthesis was unaffected. These results appear consistent with the proposal that pressure-induced division-delays occur by inhibiting the accumulation of “division proteins” which are essential for cell division.     

Radioautographic comparison of RNA synthesis patterns in the epithelial cells of mouse pyloric antrum following 3H-uridine and 3H-orotic acid injections

RNA synthesis was examined in the epithelial cells of the mouse pyloric antrum using radioautography 20 min after injection of either 3H-uridine or 3H-orotic acid. The epithelium of the mouse antrum was known to invaginate into blind tubular units composed of mucous cells arranged from base to top into a gland, an isthmus, and a pit. These were subdivided into segments and, after radioautography, silver grains were counted over cell nuclei in each segment. Following 3H-uridine injection, silver grains were present over all nuclei but were more abundant over those of the isthmus than of the gland or the pit. When nuclei were examined in the electron microscope, nucleoplasmic as well as nucleolar silver grains were more numerous in the isthmus than in the pit or gland. Following 3H-orotic acid injection, silver grains were again present over all nuclei; but maximal incorporation appeared to be in pit cell nuclei where, by electron microscopy, it was mainly assigned to the nucleoplasm. When the incorporation was calculated per whole nucleus, however, it was less in pit cell than in isthmal cell nuclei. Even so, the proportion of label in pit cell nuclei was much greater than after 3H-uridine injection. The interpretation of these findings is based on the fact that isthmal cells are immature, whereas cells migrating from the isthmus to become gland or pit cells show increasing differentiation. The immature cells of the isthmus incorporate both uridine and orotic acid more effectively than do the differentiated cells of pit and gland. Since silver grain counts over nuclei provide an index of the rate of RNA synthesis, this synthesis proceeds more actively in the isthmus than in the pit or gland. This is true of ribosomal RNA synthesis, as shown by nucleolar grain counts, and of other RNA's synthesis, as shown by nucleoplasmic grain counts. It seems, however, that while uridine is involved in the synthesis of all types of RNA, orotic acid is mainly implicated in the synthesis of the heterogeneous RNA from which the messenger RNA arises.     

Intracellular Localization of the Systemic Fungicide Triadimenol in Phytopathogenic Fungi

The intracellular localization of the radioactively labelled fungicide (³H)triadimenol A in the in vitro grown sporidia of Ustilago avenae and in the in vivo cultured powdery mildew (Erysiphe graminis f. sp. hordet) on barley (Hordeum vulgare) is described. The specimens were prepared by low temperature techniques: shock freezing, freeze substitution and embedding in Spurr's low viscosity resin. The localization of the fungicide was achieved by means of conventional electron microscopic autoradiography. The available experimental data allow a first qualitative analysis of the distribution of silver grains on freeze substituted sporidia of U. avenae and the infection structures of Erysiphe graminis f. sp. hordei. Concerning U. avenae the fungicide is detected preferentially over the vacuoles, the cytoplasm, and the cell walls after a six month exposure. The host pathogen system powdery mildew on barley exhibits an accumulation of silver grains in the host cell wall adjacent to the infection site and the papillae whereas decisively fewer grains occur inside the haustoria. Apart from this general localization pattern the haustoria show ultrastructural changes caused by the fungicide treatment: vesiculation and collapse of the sheath membrane as well as a diffuse appearance of the haustorial cytoplasm. Around the haustoria an aggregation of host cytoplasm material is observed.     

Chromatin and histones in mealy bug cell explants: activation and decondensation of facultative heterochromatin by a synthetic polyanion

In spermatogonial cells of the mealy bug, Planococcus citri, at interphase the five maternal chromosomes appear as diffuse euchromatin and the five paternal chromosomes are heterochromatic, genetically inactive, and incorporate tritiated uridine into RNA at a diminished rate. Testes squashes were treated with 2–10 mg/ml of the polyanion, polystyrene sulfonate (PSS). The gonial cell nuclei decondensed and after 15 minutes they became uniformly granular and similar in appearance to wholly euchromatic nuclei. When testis expiants were incubated with PSS (2–10 mg/ml) for from 15 to 120 minutes, all stages of deheterochromatization were recovered. The Feulgen reaction revealed that the uniform granules contained DNA; methyl-green-thionin staining indicated that the nucleolus contained RNA. When tritiated uridine was added after 15 minutes of PSS and then incubation continued, autoradiography revealed incorporation into euchromatin and decondensing heterochromatin. Incorporation of uridine increased with dosage of PSS up to 4 mg/ml. PSS (20 mg/ml) was toxic to the cells: They incorporated no uridine and were badly damaged. RNAase treated controls were also devoid of label.—PSS treated cells showed a negative alkaline-fast-green reaction for histone. In vitro a complex was formed between calf thymus histone and PSS which was soluble only above pH 8.5, but not separable on a Dowex acetate ion exchange column. These findings suggest that, probably by disrupting the structure of the DNA-histone complex, polystyrene sulfonate brings about structural decondensation of heterochromatin and enables it (and euchromatin) to incorporate tritiated uridine into RNA at an increased rate.     

Reversible (G0) and nonreadily reversible (Q) noncycling cells in human peripheral blood

PHA-stimulated human lymphoctes (normal-resting-proliferating) at 0, 24, 48, 72, and 144 h were studied with Acridine Orange (AO) staining. By viable cell sorting, by subsequent subculturing, and by use of biochemical, biophysical, and immunological assays, not only have the G₀ resting and G₁ (cycling) cell cycle phases been objectively characterized, but a separate subpopulation of quiescent cells that are functionally viable and deeply committed to nonproliferation, the Q cells, has been identified. Multiparameter cytofluorimetric analysis, methyl¹⁴C-thymidine incorporation, automated image analysis, and mitogen stimulation studies have shown that the “Q” cell, compared to the “G₀” resting but easily recruitable cell, exhibits quite lower red and green AO emission, possesses 2c to 4c DNA content (rather than only 2c), has a higher average optical density, and is either nonrecruitable or recruitable-with-difficulty in PHA-stimulated lymphocyte cultures.     

Macromolecular synthesis in the livers of aging mice as revealed by electron microscopic radioautography

For the purpose of studying the aging changes of macromolecular synthesis in animal cells, we studied many groups of aging mice during development and aging from fetal day 19 to postnatal newborn, juvenile, young adults, aged and senescent adults up to 12 and month 24 (2 years). They were injected with ³H-thymidine, ³H-uridine or ³H-leucine, precursors for DNA, RNA and proteins, as well as ³H-glucose, ³H-glucosamine, ³⁵S-sulfuric acid, or ³H-glycerol for glucide and lipid precursors, respectively, then sacrificed and the liver tissues were taken out, fixed and processed for light and electron microscopic radioautography. On many radioautograms the localization of silver grains demonstrating DNA, RNA and proteins in hepatocytes in respective aging groups were analyzed qualitatively. The number of silver grains and the number of cell organelles in each cell of each animal in respective aging groups were analyzed quantitatively in relation to the aging of individual animals. The results revealed that the localization of respective precursors as well as the number of silver grains in cell nuclei, cell organelles, changed with the aging of animals. The numbers of labeled nuclei and cell organelles, as well as the numbers of silver grains in nuclei and cell organelles changed due to aging of individual animals. The number of mitochondria, the number of labeled mitochondria and the mitochondrial labeling index labeled with silver grains were counted in each hepatocyte. It was demonstrated that the numbers of mitochondria, the numbers of labeled mitochondria and the labeling indices showing DNA, RNA and protein synthesis at various ages from embryonic day 19 to postnatal newborn day 1, 3, 9, 14, adult month 1, 2 and 6, reaching the maxima, then decreased to senile year 1 to 2, indicating the aging changes. The results indicated that mitochondria in hepatocytes synthesized nucleic acids and proteins independently from the nuclei, but their synthetic activities were affected from the aging of the individual animals.     

Syndecan from embryonic tooth mesenchyme binds tenascin.

Syndecan is a cell surface heparan sulfate-rich proteoglycan found on various epithelial cells but also in some embryonic mesenchymal tissues. We have immunoisolated syndecan from embryonic tooth mesenchyme that appeared as a 250-300-kDa molecule (Kav = 0.3 in Sepharose 4B), containing only heparan sulfate side chains (Mr = 35,000). Northern analysis of whole tooth germs and tooth mesenchymes also revealed high expression of syndecan mRNAs (2.6 and 3.4 kilobases). In the binding assay utilizing nitrocellulose as a solid phase to immobilize matrix molecules, syndecan immunoisolated from tooth mesenchyme revealed binding to tenascin, and this interaction was shown to be mediated via heparan sulfate side chains. In contrast, syndecan from mouse mammary epithelial cells showed only weak interaction with tenascin. We propose that syndecan and tenascin may represent interactions of a cell surface receptor and a matrix ligand involved in mesenchymal cell condensation and differentiation during early organogenesis.     

Combined application of low temperature preparation and electron microscopic autoradiography for the localization of systemic fungicides

Summary The intracellular localization of the sterol-biosynthesis-inhibiting (SBI) fungicide (³H)triadimenol A is investigated in vitro in the fungus Ustilago avenae. For this purpose low temperature preparation techniques (shock freezing, freeze substitution, embedding in Lowicryl HM20) are combined with conventional electron microscopic (EM) autoradiography. In particular the suitability of Lowicryl HM20 embedded specimens for EM autoradiography with regard to the finestructure preservation is shown. For the localization of (³H)triadimenol the filamentous grain development as well as the application of the gold latensification method resulting in the appearance of spherical silver grains is tested. Fungicide sensitive wild type sporidia of U. avenae are compared with fungicide resistant cells of the mutant r8. A quantitative analysis of the autoradiographs of the wild type developed according to the gold latensification process shows a relatively homogeneous distribution of silver grains over the entire cell. On the other hand, the resistant mutant is characterized by an accumulation of silver deposits over the vacuoles as compared with the lower density of grains over the cell walls and cytoplasm. The data are discussed in the context of possible resistance mechanisms against SBI-fungicides.     

Effect of insulin at dilution endpoint concentrations on macromolecular synthesis in normal mouse mammary and human breast cancer epithelial cells

Employing defined media conditions, the insulin sensitivities of mouse mammary gland epithelial cells in primary culture and MCF-7 human mammary epithelial cells were determined. Insulin stimulated the rates of [³H]uridine incorporation into RNA and [³H]leucine incorporation into protein in both primary mouse mammary gland epithelial cell cultures and MCF-7 cell cultures at concentrations approximating the dilution endpoint of the hormone (10⁻²¹ M). Insulin stimulated the rate of [³H]thymidine incorporation into DNA in primary mouse mammary gland epithelial cells at the dilution endpoint concentrations. However, MCF-7 cells required insulin concentrations 100–1000-times that necessary in mouse mammary epithelial cultures to elicit an increased rate of [³H]thymidine incorporation into DNA. Evidence is presented which suggests that the increased rates of uptake of [³H]uridine, [³H]thymidine and [³H]leucine into their respective precursor pools is not responsible for the apparent stimulatation of RNA, DNA and protein synthesis.     

Electron microscope autoradiographic study on transcriptional activity of Drosophila melanogaster polytene chromosomes

Incorporation of ³H-uridine into three chromosome regions 21D, 100AB, 7EF showing no puffs was studied by means of EM autoradiography. These regions show rather good coincidence between EM and Bridges' revised maps. The reduction of band number observed in the EM map was mainly at the expense of “doublet” bands. — Theoretical silver grain distributions were calculated on the basis of “universal curves” (Salpeter et al., 1969, J. Cell Biol. v. 41, 1–20) on condition that either bands or interbands are linear sources of radioactivity. From these curves the resolution of EM autoradiography was deduced to be sufficient with regard to the investigated region. — The results show that in addition to the puffs peaks of silver grains occur over the interbands and diffuse bands. The lowest incorporation level is observed over the dense bands. The possibility of utilizing the data obtained for the location of RNA-synthesising regions is discussed.     

Cytochemical properties of interphase chromatin condensed as a result of treatment with caffeine

Treatment of living cultured cells with caffeine (10 mg/ml, 2 h, 37 °C) brings about marked chromatin condensation which results in the appearance of small, distinct chromatin clumps in the majority of interphase nuclei. The changes taking place in the chromatin properties under the action of caffeine are rather similar to those observed in mitotic condensation (an increase in acridine orange and berberine binding and a sharp decrease in [³H]actinomycin D binding in situ; inhibition of [³H]uridine incorporation in vivo) and are reversible from the point of view of the criteria studied (nuclear morphology, ligand binding, [³H]uridine incorporation, culture viability). It is concluded that caffeine treatment can be regarded as a promising approach to the study of events occurring in chromatin condensation.     

Tissue-specificity of hemoglobin synthesis: Localization of heme synthesis in the subepidermal fat body of Chironomus thummi (Diptera)

Possible sites of heme synthesis in the fourth instar of Chironomus thummi were investigated by means of autoradiography of specific isotope incorporation. “Body wall” preparations, which include subepidermal and visceral fat body, oenocytes, muscle, epidermis, and cuticle, were cultured for 1 h in a medium containing tritiated-δ-aminolevulinic acid, a specific precursor to heme biosynthesis. Light-microscopic examination of autoradiographs of sections of the body walls indicates that the subepidermal fat body is the major site of incorporation of the precursor into heme. The visceral fat body shows few silver grains. Oenocytes, as well as muscle and epidermis, are characterized by absence of silver deposits. These findings indicate that the subepidermal fat body of Chironomus is the primary site of heme synthesis, and are discussed in relation to specific hemoglobin synthesis.     

Effects of c-Jun and a negative dominant mutation of c-Jun on differentiation and gene expression in lens epithelial cells

We have used a retroviral vector (RCAS) to overexpress wild-type chicken c-Jun or a deletion mutant of chicken c-Jun (JunΔ7) lacking the DNA binding region to investigate the possible role of c-Jun in lens epithelial cell proliferation and differentiation. Both constructs were efficiently expressed in primary cultures of embryonic chicken lens epithelial cells. Overexpression of c-Jun increased the rate of cell proliferation and greatly delayed the appearance of “lentoid bodies,” structures which contain differentiated cells expressing fiber cell markers. Excess c-Jun expression also significantly decreased the level of β_A3/A1-crystallin mRNA, without affecting αA-crystallin mRNA. In contrast, the mutated protein, JunΔ7, had no effect no proliferation or differentiation but markedly increased the level of αA-crystallin mRNA in proliferating cell cultures. These results suggest that c-Jun or Jun-related proteins may be negative regulators of αA- and β_A3/A1-crystallin genes in proliferating lens cells.     

重金属镉、锌在菹草叶细胞中的超微定位观察

水环境污染中十分突出的是重金属的污染 ,主要来源为流入物、渗漏和大气沉降 (Ｌａｒｃｈｅｒ ,1995 )。由于重金属污染物不但不能被微生物所分解 ,而且能在生物体内富集 ,并通过水生食物链的生物放大作用而对高营养级的生物甚至人类造成危害 ,因此日益引起人们的特别关注。许多研究从超微结构损伤和生理生化的角度研究了重金属对植物的毒害机制。施国新等 (2 0 0 0 )观察了重金属汞、镉污染对水生植物黑藻叶细胞的超微结构损伤。彭鸣等 (1991)研究了重金属镉、铅诱导的玉米超微结构的变化。李荣春 (2 0 0 0 )研究了Ｃｄ、Ｐｂ及其复合污染…     

NUCLEAR ENVELOPE-ASSOCIATED RESUMPTION OF RNA SYNTHESIS IN LATE MITOSIS OF HELA CELLS

The restitution of RNA synthesis in cultures progressing from metaphase into interphase (G₁) has been investigated in synchronized HeLa S₃ cells by using inhibitors of macro-molecular synthesis and the technique of electron microscope autoradiography. The rate of incorporation of radioactive uridine into RNA approached interphase levels in the absence of renewed protein synthesis. In contrast, maintenance of this rate in G₁ was dependent upon renewed protein synthesis. Restoration of synthesis of heterogeneous nuclear RNA occurred under conditions that inhibited production of ribosomal precursor RNA. In autoradiographs of individual cells exposed to radioactive uridine, silver grains were first detected after nuclear envelope reformation at the periphery of the chromosome mass but before chromosomal decondensation. These data are consistent with the following interpretation. Multiple RNA polymerase activities persist through mitosis and are involved in the initiation of RNA synthesis in early telophase at sites on the nuclear envelope.     

QUANTITATIVE AUTORADIOGRAPHIC STUDY OF LABELED RNA IN RABBIT OPTIC NERVE AFTER INTRAOCULAR INJECTION OF [3H]URIDINE

The distribution of labeled RNA in the optic nerve of the rabbit was studied by quantitative ultrastructural autoradiography after the intraocular injection of [³H]uridine. The highest density of silver grains related to [³H]RNA (27–40 grains/100 µm²) was found in glial cell perikarya; a slightly lower density was present in the glial nuclei (19–20 grains/100 µm²). Axons (4–5 grains/100 µm²) and myelin (2–3 grains/100 µm²) had the lowest grain densities. 74–83% of all counted grains were located outside the axons. By comparing the grain density distribution over the axon with that expected in the case of an exclusive labeling of the surrounding myelin and glial cell processes, it was concluded that the axons contained a number of grains representing [³H]RNA significantly higher than that expected to scatter from myelin and glial processes. Most of these grains were concentrated at the periphery of the axon and were not related to axonal mitochondria.