Changes in nuclear localization of An3, a RNA helicase,during oogenesis and embryogenesis in Xenopus laevis

The immunolocalization of An3 protein, an ATP-dependent RNA helicase and a member of the DEAD box family, was compared with the localization of fibrillarin, a protein essential for rRNA processing, and snRNPs, which are involved in mRNA splicing reactions, during oogenesis and embryogenesis in Xenopus laevis. Although An3 protein was detected in the cytoplasm of all stages of oocytes, in most stages An3 protein was also present in the nucleus. Prior to stage I An3 protein was uniformly dispersed throughout the entire germinal vesicle; from stages I to V it was in nucleoli. By stage VI nucleolar labeling with anti An3 disappeared and the protein was no longer present within nuclei. An3 reactivity was also present throughout the nuclei of follicle cells surrounding prestage I to stage VI oocytes. Both cytoplasmic and nuclear An3 staining were present in cells of stages 8 to 35 embryos; however, nuclear staining was punctate and uniformly distributed throughout the nucleoplasm. Fibrillarin was diffusely distributed throughout the entire germinal vesicle prior to stage I, localized exclusively to nucleoli of oocytes between stages I and VI and in nucleoli of stages 12 and 35 embryonic cells. Reactivity for snRNPs (anti-Sm) in germinal vesicles of prestage I oocytes was diffuse, and similar to the distribution of An3 and fibrillarin; in later stage oocytes anti-Sm staining was restricted to a population of granules, much fewer in number and more heterogeneous in size than nucleoli. Anti-Sm activity was apparent in nuclei of embryonic cells of stages 8 to 35 embryos. Although colocalization of the Sm epitope and An3 was not observed in developing oocytes and in embryonic cells, Sm reactive material was frequently found in close association with An3-positive nucleoli (oocytes) and nuclear deposits (embryonic cells). In stage IV and V oocytes treated with actinomycin D (4 μg/ml) to inhibit rRNA synthesis, nucleoli, which continued to possess fibrillarin, lacked An3; staining of follicle cell nuclei for An3 was unchanged. Treatment with 200 μg/ml actinomycin D to block mRNA synthesis, inhibited An3 but not fibrillarin staining in nuclei of prestage I oocytes and follicle cells. The changing patterns of An3 reactivity and the differential effects of actinomycin D on such localizations observed here are consistent with a role for An3 in the processing/production of RNA. © 1996 Wiley-Liss, Inc.     

Histopathogenesis of the Galls Induced by Nothanguina phyllobia in Solanum elaeagnifolium

The histopathogenesis of the foliar galls induced by Nothanguina phyllobia Thorne in Solanum elaeagnilolium Cav. was examined via serial sections prepared from plant shoots at 11 time intervals (0.5-30 days) following inoculation. Nematodes infected the blades and petioles of young leaves surrounding the shoot apex. Hypertrophy and hyperplasia of the palisade, pith, cortical, and vascular parenchyma resulted in the formation of confluent leaf, petiole, and stem galls up to 25 cm³ in volume. Externally, leaf galls were irregular, light-green, convoluted spheroid bulges distending the abaxial surface. Mature galls contained a cavity lined with parenchymogenous nutritive tissue comprising intercellular spaces and actively dividing hypertrophied cells. These cells contained granular cytoplasm, hypertrophied nuclei, and brightly stained large nucleoli. Vascular tissues were not discernibly affected during the early stages of gall development. As gall development progressed, however, vascular elements were often displaced and disoriented. The histopathology of this nematode indicates that N. phyllobia is a highly specialized parasite and, for that reason, is suitable as a biological control agent.     

Tracking nucleolar dynamics with GFP-Nopp140 during Drosophila oogenesis and embryogenesis

We expressed two green fluorescent protein (GFP)-tagged Nopp140 isoforms in transgenic Drosophila melanogaster to study nucleolar dynamics during oogenesis and early embryogenesis. Specifically, we wanted to test whether the quiescent oocyte nucleus stored maternal Nopp140 and then to determine precisely when nucleoli formed during embryogenesis. During oogenesis nurse cell nucleoli accumulated GFP-Nopp140 gradually such that posterior nurse cell nucleoli in egg chambers at stage 10 were usually brighter than the more anterior nurse cell nucleoli. Nucleoli within apoptotic nurse cells disassembled in stages 12 and 13, but not all GFP-Nopp140 entered the oocyte through inter-connecting cytoplasmic bridges. Oocytes, on the other hand, lost their nucleoli by stage 3, but GFP-Nopp140 gradually accumulated in oocyte nuclei during stages 8–13. Most oocyte nuclei at stage 10 stored GFP-Nopp140 uniformly, but many stage 10 oocytes accumulated GFP-Nopp140 in presumed endobodies or in multiple smaller spheres. All oocyte nuclei at stages 11-12 were uniformly labeled, and GFP-Nopp140 diffused to the cytoplasm upon nuclear disassembly in stage 13. GFP-Nopp140 reappeared during embryogenesis; initial nucleologenesis occurred in peripheral somatic nuclei during embryonic stage 13, one stage earlier than reported previously. These GFP-Nopp140-containing foci disassembled at the 13th syncytial mitosis, and a second nucleologenesis occurred in early stage 14. The resulting nucleoli occupied nuclear regions closest to the periphery of the embryos. Pole cells contained GFP-Nopp140 during the syncytial embryonic stages, but their nucleologenesis started at gastrulation. This work was supported by the National Science Foundation (grant MCB-0234245). O'Keith Dellafosse was supported by the Louisiana Alliance for Minority Participation (LAMP).     

Effects of Hydroxyurea on the Ultrastructure of Giant Cells in Galls Induced by Meloidogyne javanica

Hydroxyurea (HU) at concentrations of 10 or 20 mg/liter was included in a medium on which excised tomato roots infected with the root-knot nematode Meloidogyne javanica were grown. In the HU, treated roots, giant cells were small and contained large vacuoles. Giant cell nuclei were amoeboidal with relatively small nucleoli in treated roots, compared with giant cells of nontreated galls. In treated-root giant cells, the cytoplasm was diffuse and few organelles such as mitochondria, dictyosomes, and endoplasmic reticulum were detected; also, walls of giant cells were thin with less extensive ingrowths than in nontreated roots. We conclude that HU suppressed normal giant cell formation interfering with its function as a feeding cell.     

Nuclear changes induced by the nematodesXiphinema diversicaudatum andLongidorus elongatus in root-tips of perennial ryegrass,Lolium perenne

Summary The DNA content and size of individual nuclei from galls of perennial ryegrass root-tips induced byX. diversicaudatum andL. elongatus were measured. Feeding byX.diversicaudatum increased the DNA content of the nuclei by varying amounts. No regular doubling pattern of the DNA content was discernible. The DNA values varied up to between 32–64C. Generally the size of the nuclei was not increased, although some were larger than control nuclei. The modified nuclei probably have an altered metabolic function, which increases the food value of the gall to the nematode. Some bi-nucleate cells were also observed, which probably result from mitosis without cytokinesis. A preliminary examination of nuclei from galls induced byL. elongatus revealed similar nuclear changes, but no bi-nucleate cells were found. Editor's note: Awarded the Viviane Maggi prize for the best paper presented by a beginner at the Annual Meeting of the Histochemistry and Cytochemistry Section of the Royal Microscopical Society in April 1981. This paper is a full report of that presentation.     

Histopathogenesis of Galls Induced by Meloidogyne naasi in Wheat Roots

Histopathogenesis of galls induced by Meloidogyne naasi in wheat roots was studied. Large numbers of larvae penetrated wheat root tips within 24 hr; larvae migrated both inter- and intracellularly, causing cortical hypertrophy. Giant cells were formed in the stele around the head of each nematode within 4 to 5 days. Initial pathological alterations in giant cell formation consisted of hypertrophy of protophloem and protoxylem cells, their nuclei and nucleoli. Giant ceils contained 2 to 8 agglomerated multinucleolate nuclei. Synchronous mitotic divisions were first observed 9 days after inoculation. After 21 days, giant cells became highly vacuolate. Observations 40 days after inoculation revealed a complete degeneration of cell contents in many giant cells but their thick walls remained intact. Abnormal xylem completely surrounded the degenerated or partially degenerated giant cells.     

EFFECTS OF BENZAMIDE ON EMBRYONIC DEVELOPMENT OF THE HOUSEFLY

This paper deals with the effects of benzamide, a chromosomal RNA inhibitor, on embryonic development of the housefly Musca domestica nebulo. Eggs exposed to benzamide immediately after oviposition continued to develop until the blastema stage, but further development was arrested. Formation of cell boundaries and nucleoli failed to occur and the nuclei at the posterior pole did not differentiate into pole cells. This suggests that synthesis of new RNA is needed for development beyond the blastema stage. Treatment of eggs at different stages of development showed that as development progressed embryos became less sensitive to the drug. Introduction of benzamide into eggs during the pre-blastema period caused irreversible arrest of development, whereas, treatment during post-blastema stages resulted in reversible inhibition of development. The cortical cytoplasm thus appears to induce a significant change in the cleavage nuclei, which alters their sensitivity to the drug.     

Pathogenicity and Histopathology of Rotylenchulus reniformis Infecting Cantaloup

Rotylenchulus reniformis was pathogenic to cantaloup (Cucumis melo ''Perlita'') under greenhouse conditions. These findings confirm field symptoms of cantaloup infected with R. reniformis. Histopathological studies show that the nematode penetrates the cortex perpendicular to the vascular system and comes to rest with the head against the endodermis in young roots. Feeding stimulated the pericycle to either side of the endodermal feeding cell and caused cell hypertrophy with enlargement of the nucleoli and granular thickening of the cytoplasm. In older roots where the endodermis had collapsed, the nematode fed directly into the pericycle and caused similar symptoms. Nematode development was more rapid at 27 C than at 21 C.     

Nucleolar size in parallel with ribosomal RNA synthesis at diapause termination in the eggs of Bombyx mori

The eggs of Bombyx mori, both in diapause and nondiapause, were subjected to cytological examination of nucleoli and measurement of RNA precursor incorporation (2 hours) into ribosomal RNA. In diapause eggs, the nucleoli were very small and the rate of ribosomal RNA synthesis was the lowest of the samples tested. Most cells in diapause possessed nuclei with one nucleolus. In contrast, the eggs activated from diapause by long chilling attained the largest size of nucleoli and the highest rate of ribosomal RNA synthesis. A significant proportion of the cell nuclei still had only one nucleolus at this stage. Three days after activation, the eggs exhibited intermediate levels in both the size of nucleoli and the rate of ribosomal RNA synthesis. At this stage, about half of the egg cell nuclei had two nucleoli.This paper is dedicated with respect and admiration to Professor D.F. Poulson, who has made many significant contributions on the genetics, embryology and cytology of Drosophila as well as other Insecta, in commemoration of his retirement     

Observations on the Mode of Parasitism and Histopathology of Meloidodera floridensis and Verutus volvingentis (Heteroderidae)

Some aspects of the host-parasite relationships of two heteroderid nematodes are described. Meloidodera floridensis induced formation of single uninucleate giant cells in the stelar parenchyma tissue of sand pine (Pinus clausa) roots. Wrinkling and yellowing of the cuticle were associated with maturation of the adult female (cystoid stage). The mode of parasitism of different life stages of Verutus volvingentis on buttonweed (Diodia virginiana) is described. The nematode caused extensive necrosis during penetration and the formation of a large feeding site consisting of nonhypertrophied parenchyma cells with enlarged nuclei and thickened cell walls in the cortex. Walls between cells within the feeding site degenerated, resulting in the formation of a syncytium. Two citrus rootstocks, rough lemon (Citrus lirnon) and trifoliate orange (Poncirus trifoliata), were not hosts of V. volvingentis.     

锌胁迫下水车前叶细胞自由基过氧化损伤与超微结构变化之间关系的研究

主要研究了模拟锌污染对水车前叶细胞的自由基过氧化损伤和超微结构的变化,并对二者之间的关系作了初步探讨。随锌胁迫程度的增大,叶绿素含量、SOD（超氧化物歧化酶）活性和可溶性蛋白含量呈下降趋势;而POD（过氧化物酶）和CAT（过氧化氢酶）活性则先升后降;MDA（丙二醛）含量上升。超微结构的变化也呈现加重趋势,低浓度处理的变化为细胞核变形、叶绿体膨胀、类囊体排列紊乱;严重的超微结构的损伤是核仁散开、染色质凝集,细胞核几乎成为空核和核膜破裂,核质散出;线粒体脊突膨胀和部分溶解;叶绿体膜断裂、消失和部分类囊体溶解和散到细胞质中。实验结果表明,锌胁迫下叶细胞超微结构的变化 反映了内膜系统遭到严重伤害,这可能是自由基过氧化损伤的结果。     

An autoradiographic and cytophotometric study of oogenesis in a pulmonate snail,Planorbarius corneus

Summary The spatial and temporal patterns of macromolecular syntheses in oocytes and somatic auxiliary cells of the snail Planorbarius corneus have been investigated by autoradiography and cytophotometry. Oogenesis has been divided into three stages, comprising early meiosis up to diplotene (stage I), previtellogenetic growth phase (stage II), and vitellogenesis (stage III). No DNA synthesis was found in any oocyte stage. In stage-I oocytes, only nucleoli were found labelled with ³H-uridine. Oocyte nuclei of stage II and III actively synthesize RNA in nucleoli and chromosomes. The most intense incorporation of uridine in chromatin probably occurs during the previtellogenesis — vitellogenesis transition period during which cytological findings suggest well developed lampbrush chromosomes. RNA synthesis in amphinucleoli of stage-III oocytes is restricted to basophilic nucleolar parts, whereas acidophilic parts (protein bodies) neither synthesize nor store RNA. During vitellogenesis oocytes incorporate amino acids into yolk platelet proteins. Radioactive proteins are found in yolk platelet precursors 5 h after injection of the tracer and in yolk platelets 3 h thereafter. The labelling pattern suggests that oocytes synthesize certain hitherto unidentified yolk components. No evidence for the participation of follicle cells in synthesis and transport of vitellogenic proteins has been obtained from autoradiography. Cytological findings suggest an important role for these cells in oogenesis. They are highly active in RNA and protein synthesis. Cellular differentiation is accompanied by polyploidization of the nuclei which attain a highest DNA content of 256 c. Polyploidization probably occurs in incremental steps as indicated by complete endomitotic chromosomal cycles. Autoradiographs show that, during vitellogenesis, oocytes do not incorporate significant amounts of glucose, and only certain follicle cells were labelled with glucose, probably indicating the synthesis of glycogen.     

锌胁迫下水车前叶细胞自由基过氧化损伤与超微结构变化之间关系的研究

主要研究了模拟锌污染对水车前叶细胞的自由基过氧化损伤和超微结构的变化,并对二者之间的关系作了初步探讨,随锌胁迫程度的增大,叶绿素含量,SOD（超氧化物歧化酶）活性和可溶性蛋白含量呈下降趋势;而POD（过氧化物酶）和CAT（过氧化氢酶）活性则先升后降;MDA（丙二醛）含量上升,超微结构的变化也呈现加重趋势,低浓度处理的变化为细胞核变形,叶绿体膨胀,类囊体排列紊乱,严重的超微结构的损伤是核仁散开,染色质凝集,细胞核几乎成为空核和核膜破裂,核质散出;线粒体脊突膨胀和部分溶解;叶绿体膜断裂,消失和部分类囊体溶解和散到细胞质中,实验结果表明,锌胁迫下叶细胞超微结构的变化反映了内膜系统遭到严重伤害,这可能是自由基过氧化损伤的结果。     

Effect of low temperatures on the level of nucleic acids and protein in the nuclei of early bird embryos (cytophometric study)]

The content of DNA and protein in the nuclei was determined cytophotometrically as well as DNA and RNA in nucleoli of chicken embryos of different gastrullation stages after 3 days of storage at +6 degrees, +2 degrees and - 2 degrees C. It was established that the response of embryos to cold at the cell level became apparent in inhibiting the protein synthesizing system (under effects of suboptimal and extreme temperature). inhibiting the migration processes of nuclear RNA into the nucleoplasm and nuclear proteins into the cytoplasm and a certain alteration in the nucleus ploidy (under extreme conditions). The reaction of each stage under study and different cellular layers of the same differentiation stage were shown to have certain specificity.     

THE FINE STRUCTURE OF THE NUCLEOLUS IN MITOTIC DIVISIONS OF CHINESE HAMSTER CELLS IN VITRO

The nucleolus of Chinese hamster tissue culture cells (strain Dede) was studied in each stage of mitosis with the electron microscope. Mitotic cells were selectively removed from the cultures with 0.2 per cent trypsin and fixed in either osmium tetroxide or glutaraldehyde followed by osmium tetroxide. The cells were embedded in both prepolymerized methacrylate and Epon 812. Thin sections of interphase nucleoli revealed two consistent components; dense 150-A granules and fine fibrils which measured 50 A or less in diameter. During prophase, distinct zones which were observed in some interphase nucleoli (i.e. nucleolonema and pars amorpha) were lost and the nucleoli were observed to disperse into smaller masses. By late prophase or prometaphase, the nucleoli appeared as loosely wound, predominantly fibrous structures with widely dispersed granules. Such structures persisted throughout mitosis either free in the cytoplasm or associated with the chromosomes. At telophase, those nucleolar bodies associated with the chromosomes became included in the daughter nuclei, resumed their compact granular appearance, and reorganized into an interphase-type structure.     

Ultrastructure of tapetal cell ontogeny inBeta

Summary Tapetal cell development and degeneration in anthers ofBeta vulgaris L. were studied with the electron microscope. Tapetal cells become differentiated from sporogenous cells early in anther ontogeny. The tapetal nuclei divide mitotically; binucleate tapetal cells contain relatively little endoplasmic reticulum and otherwise resemble meristematic cells of higher plants. There follows an increase in endoplasmic reticulum and by the time the sporogenous tissue has entered meiotic prophase, the tapetal cells have differentiated the usual characteristics of secretory cells. Degenerative changes begin to appear in tapetal cells after meiosis of the sporogenous tissue. Such changes include loss of inner tangential and anticlinal walls, degeneration of tapetal nuclear envelopes, disruption of the plasmalemma, and changes in the cytoplasmic organelles. Coated tubules are associated with tapetal nucleoli during degenerative stages and the tubules persist after tapetal nuclei have degenerated. Tapetal cell cytoplasm disappears completely by the stage of microspore mitosis.     

Histological Comparisons of Fergusobia/Fergusonina-Induced Galls on Different Myrtaceous Hosts

The putative mutualism between different host-specific Fergusobia nematodes and Fergusonina flies is manifested in a variety of gall types involving shoot or inflorescence buds, individual flower buds, stems, or young leaves in the plant family Myrtaceae. Different types of galls in the early-to-middle stages of development, with host-specific species of Fergusobia/Fergusonina, were collected from Australian members of the subfamily Leptospermoideae (six species of Eucalyptus, two species of Corymbia, and seven species of broad-leaved Melaleuca). Galls were sectioned and histologically examined to assess morphological changes induced by nematode/fly mutualism. The different gall forms were characterized into four broad categories: (i) individual flower bud, (ii) terminal and axial bud, (iii) ''basal rosette'' stem, and (iv) flat leaf. Gall morphology in all four types appeared to result from species-specific selection of the oviposition site and timing and number of eggs deposited in a particular plant host. In all cases, early parasitism by Fergusobia/Fergusonina involved several layers of uninucleate, hypertrophied cells lining the lumen of each locule (gall chamber where each fly larva and accompanying nematodes develop). Hypertrophied cells in galls were larger than normal epidermal cells, and each had an enlarged nucleus, nucleolus, and granular cytoplasm that resembled shoot bud gall cells induced by nematodes in the Anguinidae.     

Biological Relationship of Rotyleinchulus borealis on Several Plant Cultivars

The embryogenic development of Rolylenchulus borealis, at 24-26 C, was completed on corn, in 12-15 days, and the life-cycle of the nematode from egg to egg required 35-40 days at 20-25 C. Juveniles remained in the soil as preinfective stages for 17-19 days before becoming adults. Only immature vermiform and swollen egg-laying females were found attached to corn roots. Eggs were laid in a gelatinous matrix on the root surface; the number of eggs per egg mass was 45 ± 28 on corn roots. Bean, green pea, potato, sorghum, and sweet potato were also found to be hosts of R. borealis. The nematode established a permanent feeding site on corn root in an endodermal cell that became hypertrophied. Pericyclic cells close to the feeding site showed granular cytoplasm and nuclei with hypertrophied nucleoli. A cell wall ingrowth was also noted around the area of stylet penetration into the endodermal cell.     

REFORMATION OF NUCLEOLUS-LIKE BODIES IN THE ABSENCE OF POSTMITOTIC RNA SYNTHESIS

The dependence of nucleolar reformation on RNA synthesis that resumes in late anaphase or early telophase has been investigated in synchronously dividing Amoeba proteus. RNA synthesis was completely inhibited throughout all stages of mitosis and the early hours of interphase with high concentrations of actinomycin D. In such cells, nucleolus-like bodies that bind azure B and pyronin were apparent in the reformed nuclei. The bodies appear as dense, fibrous masses with loosely associated, finely fibrillar material. There are no characteristic granular regions in the reformed structures. It is suggested that the bodies probably represent mainly nucleolar protein and residual RNA which can bring about the reorganization of nucleoli in the absence of postmitotic RNA synthesis.