Food habits of the giant humphead wrasse,Cheilinus undulatus (Labridae)

Synopsis The giant humphead wrasse (Cheilinus undulatus), an inhabitant of coral reefs, is widely distributed in the tropical Indo-Pacific region. Stomach and intestinal contents of 72 specimens from the Pacific and the Red Sea revealed that this fish feeds primarily on mollusks, fishes, echinoids, and crustaceans.This article is one of several presented at the Second European Ichthyological Congress, Paris, 8-15 September 1976, to be published by Environmental Biology of Fishes.     

Photosynthetic responses of Zostera marina L. (Eelgrass) to in situ manipulations of light intensity

Summary Photosynthetic responses of the temperate seagrass, Zostera marina L., were examined by manipulations of photon flux density in an eelgrass bed in Great Harbor, Woods Hole, MA during August 1981. Sun reflectors and light shading screens were placed at shallow (1.3 m) and deep (5.5 m) stations in the eelgrass bed to increase (+35% to +40%) and decrease (-55%) ambient photon flux densities. The portion of the day that light intensities exceeding the light compensation point for Z. marina (H _comp) and the light saturation point (H _sat) were determined to assess the impact of the reflectors and shades. The H _comp and H _sat periods at the deep station shading screen were most strongly affected; H _comp was reduced by 11% and H _sat was reduced by 52%. Light-saturated photosynthetic rates, dark respiration rates, leaf chlorophyll content, chlorophyll a/b, PSU_{O 2} size, PSU density, leaf area, specific leaf area, leaf turnover times and leaf production rates were determined at the end of three sets of 1- to 2-week experiments. None of the measured parameters were affected by the photon flux density manipulations at the shallow station; however, at the deep station leaf production rates were significantly reduced under the shading screen and chlorophyll a/b ratios were higher at the reflector. These results indicate that adjustment to short-term changes in light regime in Z. marina is largely by leaf production rates. Further, the most dramatic changes in the periods of compensating or saturating photon flux densities had the greatest impact on the measured photosynthetic responses.     

Early Events in Parvovirus Replication: Lack of Integration by Minute Virus of Mice into Host Cell DNA

Viral DNA sequences were not detected in high-molecular-weight host DNA until well after the onset of viral DNA replication.     

Outer membrane protein a and other polypeptides regulate capsular polysaccharide synthesis in E. coli K-12.

Summary capR (lon) mutants of Escherichia coli K-12 are mucoid on minimal agar because they produce large quantities of capsular polysaccharide. When such mutants are transformed to tetracycline resistance by plasmid pMC44, a hybrid plasmid that contains a 2 megadalton (Mdal) endonuclease EcoR1 fragment of E. coli K-12 DNA joined to the cloning vehicle-pSC101, capsular polysaccharide synthesis is inhibited and the transformed colonies exhibit a nonmucoid phenotype. Re-cloning of the 2 Mdal EcoR1 fragment onto plasmid pHA105, a min-colE1 plasmid, yielded plasmid pFM100 which also inhibited capsular polysaccharide synthesis in the capR mutants. A comparison of the polypeptides specified by both plasmids pFM100 and pMC44 in minicells demonstrated that seven polypeptide bands were specified by the 2 Mdal DNA, one of which was previously demonstrated to be outer membrane protein a; also known as 3b or M2 (40 kilodaltons, Kdal). Plasmid mutants no longer repressing capsular polysaccharide synthesis were either unable to specify the 40 K dal outer membrane protein a or were deficient in synthesis of 25 K dal and 14.5 K dal polypeptides specified by the 2 Mdal DNA fragment. Studies with a minicell-producing strain that also contained a capR mutation indicated that the capR gene product regulated processing of at least one normal protein, the precursor of outer membrane protein a.     

Regeneration and autotomy exhibited by the Black Widow spider,Latrodectus variolus walckenaer

Summary Crustaceans, insects and to a lesser degree arachnids have been employed in regeneration studies. Amputation and ligation of the legs was used to determine occurring in a Black Widow spider complied with the developmental gradient model of regeneration. The occurrence of autotomy in this species was also documented. Amputation indicated the most proximal point from which regeneration of the leg could occur was the femoral mid-point. Amputation proximal to that area did not result in leg regeneration. Autotomy following amputation was not observed. Ligation of the legs resulted in autotomy when applied at and proximal to the mid-point of the tibia, increasing in frequency as more proximal segments were ligated. Autotomy always occurred at the trochanter-coxa joint. Autotomized legs did not regenerate. The regeneration observed complied with the developmental gradient model.     

Ribulose bisphosphate carboxylase: altered genetic expression in tall fescue

A decaploid tall fescue (Festuca arundinacea Schreb) genotype has been found which exhibits net photosynthetic rates of 32 to 41 mg CO₂/dm²·hour as opposed to a mean of 22 mg CO₂/dm²·hour for 10 hexaploid genotypes. The decaploid genotype exhibited a ribulose 1,5-bisphosphate (RuBP) carboxylase specific activity 1.3- to 2-fold higher than typical tall fescue genotypes. Specific activities of photorespiratory enzymes and nitrate reduction enzymes were lower in the decaploid than the hexaploid genotypes. Results suggest that genetic expression of RuBP carboxylase activity may have been altered to increase the net photosynthesis rate in the decaploid genotype.     

The treatment of the hepatorenal syndrome with intra-renal administration of prostaglandin E1

Three patients with the hepatorenal syndrome were treated with prostaglandin E₁ administered through a selective renal arterial catheter. Prostaglandin E₁ was given in progressively increasing doses (2 to 100 ng/kg/min) over a 60-minute period. Control plasma prostaglandin E levels were elevated in all three patients, 0.98, 0.91, and 0.83 ng/ml, respectively. At the end of the infusion, plasma prostaglandin E levels had risen to 10.4, 2.63, and 10.3 ng/ml in the three patients respectively. Plasma renin activity increased during the course of the infusion in two of the patients. The plasma aldosterone concentration did not change during the prostaglandin E₁ infusion. Intrarenal prostaglandin E₁ failed to increase urine volume or urinary sodium concentration in three patients with the hepatorenal syndrome.     

Purification and properties of soybean nodule xanthine dehydrogenase

Xanthine dehydrogenase (EC 1.2.1.37), an essential enzyme for ureide metabolism was purified from the cytosol fraction of soybean nodules. The purified xanthine dehydrogenase was shown to be homogeneous by electrophoresis and a pI of 4.7 was determined by isoelectric focusing. The enzyme had a molecular weight of 285,000 and two subunits of molecular weight 141,000 each. The holoenzyme contained 1.7 (±0.7) mol Mo and 8.1 (±2.0) mol Fe/mol enzyme and the enzyme also contained FMN and is thus a molybdoironflavoprotein. Soybean xanthine dehydrogenase is the second enzyme in plants demonstrated to contain Mo and the first xanthine-oxidizing enzyme reported to contain FMN, rather than FAD as the flavin cofactor.     

Low-Intensity picosecond fluorescence kinetics and excitation dynamics in barley chloroplasts

The fluorescence decays of barley chloroplasts have been measured by single-photon counting with tunable picosecond dye laser excitation. The fluorescence decays of dark-adapted chloroplasts are best fitted to a sum of three exponential lifetime components with lifetimes of 112, 380 and 2214 ps. The relative magnitude of each component is shown to be dependent on the excitation wavelength and collected emission wavelength. The excitation wavelength dependence is correlated with the Photosystem (PS) I and PS II action study of Ried [36] and with the measured pigment distributions in the photosynthetic unit [37,41]. Experiments varying the single excitation pulse intensity from 10⁸ to 10¹² photons/cm² pulse show that our results are not distorted by singlet-singlet annihilation. Unflowed samples where the cloroplasts are under constant illumination show 2-fold increases in quantum yield of fluorescence primarily in the two longer lifetime components. Theoretical calculations of Shipman [31] on an isolated reaction center with a homogeneous antenna are discussed and the principles extended to discussion of the measured barley chloroplast fluorescence decay components in terms of photosynthetic unit light-harvesting array models and earlier experimental work. Our data support a photosynthetic unit model in which 70–90% of the photons absorbed are quenched by either PS I or efficiently quenching PS II in a process where the fluorescence lifetime is 100 ps. The origin of the intermediate 380 ps. component is probably due to excitation transfer to a PS II reaction center in a redox state which quenches less efficiently.     

Cycloheptaamylose as an affinity ligand of cereal alpha amylase. Characteristics and a possible mechanism of the interaction

The characteristics of alpha amylase purification on a column of cycloheptaamylose-substituted, epoxy-activated Sepharose 6B were investigated. The enzyme was recovered in high yield from crude triticale and wheat extracts. Enzyme activity assessed after elution from the column was 132% of that measured prior to chromatography. There was no evidence of beta amylase isozymes in the purified alpha amylase. Neither barley beta amylase nor sweet-potato beta amylase was retained by the column. Cycloheptaamylose did not inhibit triticale or wheat alpha amylase activity, but did inhibit barley beta amylase activity, yielding a K₁ of 4.5mm. Equilibriumdialysis experiments showed that alpha amylase did interact with cycloheptaamylose. The dissociation constant for the enzyme-ligand was 19μm. It was concluded that cycloheptaamylose bound at a non-catalytic site on the alpha amylase molecule.