The fine structure of ciliated sensory cells in the epidermis of the earthworm Lumbricus terrestris

An ultrastructural study of the earthworm body wall has revealed three types of sensory cells. Two, the multiciliate and uniciliate sensory cells, are found only in the discrete sense organs and their cilia pass vertically through the cuticle. The third type-isolated multiciliate sensory cells-are scattered throughout the epidermis and never grouped together. However, their cilia do not pass through the cuticle, but run horizontally over the outer surface of the epidermal cells. The structure of the sensory cells is described and compared with that of ordinary epidermal cells and the supporting cells found in the sense organs. Their possible physiological roles are discussed.     

The fine structure of atypical ciliated cells in the human gastric epithelium

Gastric mucosa obtained from the body and pyloric portions of the human stomach were observed by light and transmission electron microscopy. Ciliated cells were found in two of 18 subjects examined, one patient with gastric ulcer and the other one with gastric adenocarcinoma. The ciliated cells were found in epithelia at sites away from the main lesions. The tissues containing ciliated cells showed intestinal metaplasia combined with mild chronic gastritis in both cases. The epithelial layer facing the gastric lumen was composed of columnar cells with numerous uniform microvilli and goblet cells. This epithelium extended to the superficial parts of the tubules surrounded by the lamina propria. The deeper portions of the tubules were composed of mucous secretory, endocrine, and rarely ciliated cells. These ciliated cells were provided with numerous cilia the numbers of which varied considerably from cell to cell. This was in contrast to the primary cilium which is usually single. The central part of the apical cell membrane was sometimes concave in the area from where cilia tended to arise. It was also observed that numerous basal bodies as well as mucus-like granules were contained in the same cell. The axonemal pattern was different from that of ordinary cilia and showed 9 + 0 and 8 + 1 patterns. In longitudinal sections it was found that one peripheral doublet was displaced to the center of the axoneme as it left the basal body.     

The fine structure of barley aleurone cells

Summary The ultrastructural morphology of both dry and water-imbibed barley aleurone cells is described. The aleurone cell is characterized by the presence of numerous aleurone grains and spherosomes. In addition, it contains organelles typical of other plant cells including structures similar to microbodies, and rough endoplasmic reticulum characterized by the presence of numerous polyribosomes. It is inferred that the morphological specialization of aleurone cells is related to their biochemical specialization.Work supported by National Science Foundation grant GB5863. The skillful technical assistance of Mrs. Janet Price is gratefully acknowledged.     

The fine structure of cockroach blood cells

Electron-mictoscopic observations of the blood cells (Haemocytes) in the legs of the cockroach Blaberus discoidalis reveal three 'types' of cells distinguishable on the basis of fine structure. One type of cell contains numerous membrane-limited opaque bodies which may be lysosomes. A second type contains abundant digestive vacuoles and appears phagocytic. A third type, frequently encountered in rewlymoulted untanned animals but less often observed in mature adults, contains membrane-limited tubule-containing bodies (TCB) filled with rows of 340 A tubules which are quite different from cytoplasmic microtubules. It is suggested that haemocytes containing TCB may be equivalent to the coagulocytes (cystocytes) of light microscopy which actively participate-in-the process of haemolymph coagulation in Orthoptera. No attempt whatsoever is made at classification. Since considerable overlap in fine structure exists between cell types, it seems probable that the electron-images of fixed cells observed in this study represent several morphological expressions of which an individual cell may be capable during its lifetime.     

The interrelationship of the soluble and membrane-associated folate-binding proteins in human KB cells

Human KB cells produce two immunologically cross-reactive folate-binding proteins: a particulate cell-associated protein which is solubilized by Triton X-100, and a soluble protein which is released into their growth medium. This compartmentation of these two folate-binding proteins provides a convenient system for studies of their biochemical relationship. The two folate-binding proteins behave similarly to the purified particulate and soluble folate-binding proteins of human milk in analysis by radioactive folate binding, Sephacryl S-200 gel filtration profiles, polyacrylamide gel electrophoresis in either Triton X-100 or sodium dodecyl sulfate, and in Triton X-100 binding based on sucrose density gradient ultracentrifugation in H2O and D2O. The two folate-binding proteins were endogenously labeled by pulsing methionine-starved KB cells with [35S]methionine, and each protein was purified to apparent homogeneity by affinity chromatography at different times during the chase with nonradioactive methionine. The time course of the changes in specific activity (moles of [35S]methionine per mole of folate-binding protein) revealed a more rapid initial rate of synthesis and an earlier maximum in specific activity for the cell-associated folate-binding protein than for the soluble folate-binding protein released into the growth medium. Differences in the levels and specific activities of the two folate-binding proteins of cells exposed to cycloheximide compared with simultaneous controls after pulsing with [35S]methionine suggest that, whereas the cell-associated folate-binding protein is probably produced by de novo protein synthesis, the soluble folate-binding protein seems to be produced from a cellular pool of an already synthesized protein. These results combined with the immunologic cross-reactivity of the two folate-binding proteins strongly suggest a precursor-product relationship between them.     

The fine structure of the cells of the mouse peritoneum

Summary The cells of the peritoneum of the mouse have been examined with the electron microscope both by studying the gastro-splenic omentum and by washing the cells out of the peritoneal cavity. They comprise mesothelial cells, mast cells, lymphocytes and macrophages. The mesothelial cells were probably nearly all degenerate. The mast cells released granules which were phagocytosed by the other cells. The lymphocytes were either classical small lymphocytes, or rather larger cells similar to previously described immunoblasts. The macrophages varied considerably in size. Some were probably derived from the covering cells of the milk spots. They contained varying numbers of dense bodies, with the structure of lysosomes. A series of appearances was seen which suggested that these were synthesized in the granular endoplasmic reticulum. A gradation of structure was seen between lymphocytes and small macrophages.The gastro-splenic omentum consisted of two layers of mesothelium, in places fenestrated. The milk spots which were scattered throughout this structure were covered by cells similar to macrophages, and had a core of lymphoid cells in which ran a small blood vessel. The most notable difference between the mesothelial cells and the macrophages was the presence of many small caveolae at the surface of the mesothelial cells, and of larger vacuoles and indentations at the surface of the macrophages. Acknowledgements. I am grateful to Professor R. Barer for much advice and criticism, to Dr. G. A. Meek for guidance on electron microscopy, and to Miss M. Tune and Mr. M. Turton for photographic assistance.This work was supported by a grant from the Medical Research Council and by grants to the Department from the S.R.C., Nuffield Foundation and Unilever Limited.     

Changes in the fine structure of the human testicular interstitial cells after treatment with human gonadotrophins

Summary Study of the fine structure of the human interstitial cells after prolonged stimulation with human gonadotrophin reveals a striking increase in the quantity of the agranular endoplasmic reticulum. This is accompanied by an increase in the number of mitochondria which exhibit more extensive cristae, collections of intramitochondrial lipid and aggregations of electron-dense granular deposits. A rise is also evident in the number of lipofuscin pigment deposits and granular membrane-bounded bodies, both of which exhibit acid phosphatase activity. These changes after gonadotrophic stimulation are discussed in relation to steroid biosynthesis.In the pretreatment biopsies of these patients aged between 25–35 years, some interstitial cells contain intranuclear crystals which exhibit a hexagonal structure. The relationship of these intranuclear crystals to the cytoplasmic crystals of Reinke is discussed.The author is indebted to Dr. J. W. Johnstone and Dr. A. Long for the human material used in this study. Thanks are also due to Dr. H. P. Taft for helpful suggestions in the management of these patients, to Professor B. Hudson for the estimations of plasma testosterone and to Dr. J. B. Brown for the supply of human pituitary gonadotrophin and the estimations of urinary oestrogens. The technical help of Mr. T. Mezciems and the photographic assistance of Mr. J. S. Simmons F. R. P. S. and Miss S. Flett is gratefully acknowledged.     

The fine structure of the kinetochore in meiotic cells of Tradescantia

Summary Observations on Tradescantia cells in the second meiotic division revealed distinct regions in meiotic chromosomes. These areas 1) consistently stain less dense than the chromosomes themselves, 2) have direct connections with the chromosomes at certain points, and 3) serve as focal points for spindle tubules during meiosis. These lighter staining regions are similar in character to kinetochores (centromeres) found in animal cells.

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Zusammenfassung Es wurde beobachtet, daß bestimmte Regionen der Chromosomen von Tradescantia zu der zweiten meiotischen Teilung 1. durchgängig sich weniger stark färben als die Chromosomen selbst, 2. daß sie an gewissen Punkten direkte Verbindungen mit den Chromosomen haben, und 3. daß sie während der Meiosis als Sammelpunkte für Spindeltubuli dienen. Diese schwächer gefärbten Stellen werden als Kinetochoren (Centromeren) interpretiert.

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This work was supported by grant GB-3330 from the National Science Foundation to Dr. Wayne Ferris, and the training grants GM 00441 and DE 00184 from the National Institutes of Health.