Structure and Physiology of the Organs of Feeding and Digestion in Ostrea edulis

1926 ◽  
Vol 14 (2) ◽  
pp. 295-386 ◽  
Author(s):  
C. M. Yonge
Keyword(s):  
Connective Tissue ◽  
Fine Particles ◽  
Muscular Activity ◽  
Mantle Cavity ◽  
Optimum Temperature ◽  
Ostrea Edulis ◽  
Food Material ◽  
Rate Of Dissolution ◽  
Adult Oyster ◽  
Tissue Cells

The anatomy and histology of the food collecting and alimentary organs of the adult oyster are described.The anatomy of the stomach is investigated with the aid of gelatin casts and attention drawn to the food caecum, the ventral groove, and the two ducts of the digestive diverticula.Cilia and mucus glands are universal throughout the food collecting and alimentary organs.There is evidence that the gastric shield is composed of fused cilia.The histology of the style-sac resembles that described by Mackintosh for Crepidula. There is evidence that secretion of the style takes place in the groove.Phagocytes are everywhere numerous in the blood vessels, connective tissue and epithelia, and free in the gut and mantle cavity.The alimentary organs of the larva are described.The anatomy and histology of these organs in the spat isdescribed, the palps are relatively large and the gills asymmetrical. The style-sac is distinct from the mid-gut.The course of the ciliary currents on the gills and palps is described and the importance of the various selective mechanisms emphasized.Selection appears to be purely quantitative, large particles or mucus masses being rejected and smaller ones accepted.Muscular activity is of great importance in the functioning of both gills and palps. Reversal of cilia has never been seen.Rejected matter is removed from the mantle cavity.Material is sorted in the food caecum in the stomach, larger particles passing into the mid-gut and smaller ones towards the gastric shield and ducts of the digestive diverticula, within the tubules of which there is a constant circulation.The rotation of the style assists in the stirring of matter in the stomach.In the style-sac are cilia, which rotate the style and others which push it into the storuach.In the larva the velum acts as a food collecting organ ; the style lies in an extension of the stomach and rotates rapidly. Material passes freely into the digestive diverticula.In the spat rejective mechanisms are highly developed. The style revolves at a speed of between sixty and seventy revolutions per minute.The tubules of the digestive diverticula are the only place where soluble matter is absorbed, in adult, larvae, or spat.Fine particles are ingested and digested intracellularly in the tubules of the digestive diverticula, the products of digestion carried away by amoebocytes, and useless matter rejected into the lumen.Larger particles are ingested and digested by phagocytes in all parts, the products of digestion being carried to the vesicular connective tissue cells and there stored.Enzymes in the style digest starch and glycogen. The amylase, at pH 5.9, has an optimum temperature of 43'C, and is destroyed atThe optimum medium is pH 5-9. It is inactivated by purification with absolute alcohol or by dialysis, but action is restored on the addition of chlorides or bromides and to a less extent iodides, nitrates, and carbonates, but not with sulphates or fluorides.Sucroclastic enzymes in the digestive diverticula act on starch, glycogen, sucrose, raffinose, maltose, lactose, salicin, and amygdalin, but not on inulin, cellulose, or pentosans.The amylase, at pH 5-5, has an optimum temperature of 44-5, and is destroyed at between 64 and 67. It has an optimum pH of 5-5, and is inactivated after purification or dialysis, action being restored in the presence of chlorides or bromides.There is a weak lipase and protease, the latter has two optima at pH 3-7 and at or above 9-0 ; its action is very slow.The only enzymes free in the stomach are those from the style.There is no evidence of any enzymes free in the gill mucus.There is a powerful complete oxidase system in the style, and a catalase in the digestive diverticula and gonad, and traces in the palps, gills, and muscle.The style is the most acid substance in the gut and the cause of the acidity of the gut.The style is dissolved rapidly in fluid of pH 2-3 and above, but very slowly below that point. It is readily dissolved and reformed in the oyster, its presence depending on the maintenance of the balance between the rate of secretion and the rate of dissolution. Its condition is a valuable indication of the state of metabolism.Glycogen and fat are stored, particularly in the vesicular connective tissue cells, the former furnishing the principal reserve food material.The presence of abundant supplies of microscopic plant life rich in carbohydrates provides ideal food for the oyster, and represents optimum conditions for fattening and reproduction.

scholarly journals THE CELLULAR REACTIONS TO LIPOID FRACTIONS FROM ACID-FAST BACILLI

1932 ◽  
Vol 56 (6) ◽  
pp. 867-891 ◽  
Author(s):  
Kenneth C. Smithburn ◽  
Florence R. Sabin
Keyword(s):  
Life Cycle ◽  
Connective Tissue ◽  
Comparative Study ◽  
Fine Particles ◽  
Giant Cells ◽  
Epithelioid Cell ◽  
Epithelioid Cells ◽  
Acid Fast Bacilli ◽  
Tissue Cells ◽  
Do So

1. A comparative study has been made of the cellular reactions induced by phosphatides from five strains of acid-fast bacilli. Each of these reactions is characterized principally by epithelioid cells and giant cells. 2. The phosphatides are first phagocytized by young connective tissue cells or monocytes. The lipoid is then dispersed into fine particles with the formation of classical epithelioid cells. 3. A comparison has been made of the reactions induced by heat-killed and defatted tubercle bacilli with those induced by tuberculophosphatide. 4. Further studies have been made to determine whether or not the phosphatide causes sensitization to tuberculin. It does not do so. 5. The life cycle of the epithelioid cell has been observed in all its stages.

Increased matrix gene expression by glucose in rat neural connective tissue cells in culture

Diabetes ◽  
1991 ◽  
Vol 40 (5) ◽  
pp. 605-611 ◽  
Author(s):  
P. Muona ◽  
J. Peltonen ◽  
S. Jaakkola ◽  
J. Uitto
Keyword(s):  
Gene Expression ◽  
Connective Tissue ◽  
Cells In Culture ◽  
Matrix Gene ◽  
Tissue Cells

The Structure, Development, and Operation of the Hinge Ligament of Ostrea edulis

1951 ◽  
Vol s3-92 (18) ◽  
pp. 129-140
Author(s):  
E. R. TRUEMAN
Keyword(s):  
Surface Area ◽  
Outer Layer ◽  
Tensile Strain ◽  
Central Position ◽  
Ostrea Edulis ◽  
Structure Development ◽  
Dorsal Region ◽  
Larval Stages ◽  
Adult Oyster

1. The ligamental structure of Ostrea edulis is briefly described. The ligament is situated between the valves of the shell immediately below the urtibo and may be divided into two main layers, the outer and the inner, the principal features of which appear to correspond with those of other bivalves. The outer layer is divided into anterior and posterior halves by the inner layer, which occupies a central position. 2. The axis (hinge or pivotal axis) about which the valves open is situated in the adult oyster along a line drawn through the outer layer and the upper part of the inner layer. When the valves are closed the ligament above this axis is subjected to a tensile strain andthat portion below to compression, the force s so produced causing the opening of the valves. An attempt has been made t o measure this force in relation to the surface area of the valves and it is found to be approximately 4.5 gm.mm./mm.2 This figure is comparable to those obtained when certain other species of bivalves are used. 3. Th eligament is shown to develop from the simple outer layer of the early larval stages, first by the addition of aninner layer and then by growth of this structure chiefly in a ventral direction. The initial dorsal region of the ligamentsoon degenerates and at the same time the pivotal axis moves ventrally between the valves, thus increasing in length. This method of growth is compared with that of an elongate external ligament and the mechanical implications are suggested.

scholarly journals AUTORADIOGRAPHIC LOCALIZATION OF NEW RNA SYNTHESIS IN HYPERTROPHYING SKELETAL MUSCLE

1973 ◽  
Vol 57 (3) ◽  
pp. 743-759 ◽  
Author(s):  
Charles K. Jablecki ◽  
John E. Heuser ◽  
Seymour Kaufman
Keyword(s):  
Skeletal Muscle ◽  
Connective Tissue ◽  
Rna Synthesis ◽  
Proliferating Cells ◽  
Quantitative Studies ◽  
Physiological Adaptations ◽  
Rat Soleus Muscle ◽  
Tissue Cells ◽  
A Site ◽  
Silver Grains

Work-induced growth of rat soleus muscle is accompanied by an early increase in new RNA synthesis. To determine the cell type(s) responsible for the increased RNA synthesis, we compared light autoradiographs of control and hypertrophying muscles from rats injected with tritiated uridine 12, 24, and 48 h after inducing hypertrophy. There was an increased number of silver grains over autoradiographs of hypertrophied muscle. This increase occurred over connective tissue cells; there was no increase in the number of silver grains over the muscle fibers. Quantitative studies demonstrated that between 70 and 80% of the radioactivity in the muscle that survived fixation and washing was in RNA. Pretreatment of the animals with actinomycin D reduced in parallel both the radioactivity in RNA and the number of silver grains over autoradiographs. Proliferation of the connective tissue in hypertrophying muscle was evident in light micrographs, and electron micrographs identified the proliferating cells as enlarged fibroblasts and macrophages; the connective tissue cells remained after hypertrophy was completed. Thus, proliferating connective tissue cells are the major site of the increase in new RNA synthesis during acute work-induced growth of skeletal muscle. It is suggested that in the analysis of physiological adaptations of muscle, the connective tissue cells deserve consideration as a site of significant molecular activity.

scholarly journals THE COMPARATIVE RESISTANCE OF BACTERIA AND HUMAN TISSUE CELLS TO CERTAIN COMMON ANTISEPTICS

1916 ◽  
Vol 24 (6) ◽  
pp. 683-688 ◽  
Author(s):  
Robert A. Lambert
Keyword(s):  
Hydrogen Peroxide ◽  
Staphylococcus Aureus ◽  
Connective Tissue ◽  
Human Tissue ◽  
Tissue Cultures ◽  
Mercuric Iodide ◽  
Living Body ◽  
Tissue Cells ◽  
The One ◽  
The Ideal

The comparative resistance of bacteria and human tissue cells to antiseptics and other chemicals may be easily tested by tissue cultures under conditions which approximate those found in the living body. A comparative study shows that while human cells (connective tissue and wandering cells) are highly resistant to many antiseptics, they are in general more easily killed than bacteria (Staphylococcus aureus). Of the antiseptics tested, which include mercuric chloride, iodine, potassium mercuric iodide, phenol, tricresol, hydrogen peroxide, hypochlorites (Dakin's solution), argyrol, and alcohol, the one which approaches most closely the ideal disinfectant is iodine, which kills bacteria in strengths that do not seriously injure connective tissue cells or wandering cells.

THE APODEME COMPLEX OF THE FEMORAL CHORDOTONAL ORGAN IN THE METATHORACIC LEG OF THE LOCUST SCHISTOCERCA GREGARIA

1992 ◽  
Vol 163 (1) ◽  
pp. 345-358 ◽  
Author(s):  
P. M.J. SHELTON ◽  
R. O. STEPHEN ◽  
J. J.A. SCOTT ◽  
A. R. TINDALL
Keyword(s):  
Extracellular Matrix ◽  
Connective Tissue ◽  
Direct Observation ◽  
Schistocerca Gregaria ◽  
Chordotonal Organ ◽  
Acid Fuchsin ◽  
Joint Angles ◽  
Direct Continuation ◽  
Loop Shape ◽  
Tissue Cells

The mechanical connections of the metathoracic femoral chordotonal organ (mtFCO) with its insertion at the femoro-tibial joint are described. The apodeme complex is shown to consist of a distal cuticular rod that is replaced proximally by dorsal and ventral ligaments. The dorsal ligament is a direct continuation of the distal rod but proximally it is replaced by ligamentous cells. The ventral ligament has no cuticular core and consists of ligamentous cells throughout its length. The ligaments are composed of bundles of connective tissue cells that are each enclosed in an extracellular matrix containing acid-fuchsin-staining fibrils. Internally the cells are packed with microtubules. During extension and flexion of the joint, the two ligaments move differentially. During passive extension of the tibia, the ventral ligament remains taut but the dorsal one buckles to form a slack loop. Direct observation of living preparations shows that the loop is first detectable during extension of the tibia at joint angles greater than about 51°. During flexion, the loop gradually tightens and disappears. It has completely disappeared at joint angles of less than about 36°. Changes in loop shape were demonstrable using preparations in which the tibia was moved sinusoidally ±10° about a mean femoro-tibial angle of 90° and photographs were taken using phase-locked illumination. Other details of the apodeme complex are described and the significance of the findings is discussed in relation to mtFCO function.

A Note on the Habits and Nutrition of Solemya parkinsoni (Protobranchia: Bivalvia)

1961 ◽  
Vol s3-102 (57) ◽  
pp. 15-21
Author(s):  
G. OWEN
Keyword(s):  
Organic Material ◽  
Alimentary Canal ◽  
Spring Tide ◽  
Muscular Activity ◽  
Mantle Cavity ◽  
Animal Burrows ◽  
Water Spring

Adult specimens of Solemya parkinsoni Smith, embedded in mud at a depth of 50 cm or more, were collected near low water (spring tide). The animal burrows with the anterior end downwards and does not maintain an opening to the surface. An inhalant current is drawn into the mantle cavity anteriorly on each side of the foot, while an exhalant current leaves by the single, posteriorly situated aperture. This is probably a respiratory current, bottom material entering the mantle cavity as a result of the muscular activity of the mantle and foot. The course of the alimentary canal is described, and the problem of feeding and nutrition correlated with the extreme reduction of the gut exhibited by S.parkinsoni discussed. It is suggested that an initial breakdown of organic material may take place in the mantle cavity.

Sign in / Sign up

Export Citation Format

Share Document