Dominance status and certain operants in a communal colony of rhesus macaques

This study was designed to test the hypothesis that in some species of primates individual differences in responsiveness to certain situations is related to dominance status. During the first phase of the study, the existence of a linear dominance hierarchy was confirmed by ratings of agonistic interactions. In the second phase, bar-pressing behavior was recorded on a cumulative recorder while the experimenter simultaneously rated, at 30-second intervals, all animals present in the research setting. Results indicated that dominance status was systematically related both to rate of bar-pressing and to duration of response blocks, with the more dominant animals bar-pressing at slower rates for longer blocks of time. The finding that individual differences in rate did not vary with social context suggests that dominance-related differences in responsiveness may be quite stable. Certain dominancerelated trends in the variation of social context in the research setting were also noted.     

The role of microtubules in vessel member differentiation inColeus

Summary The role of microtubules in tracheary element formation in cultured stem segments ofColeus has been investigated through the use of the antimicrotubule drug, colchicine. Colchicine treatment of the cultured stem segments produced a dual effect on xylem differentiation. If applied at the time of stem segment isolation or shortly thereafter, wound vessel member formation is almost completely blocked. However, if colchicine is applied after the third day of culture, it does not inhibit differentiation, but instead large numbers of xylem elements are formed which have highly deformed secondary walls. Both effects are related to colchicine's specific affinity for microtubules. In the first case it is shown that colchicine blocks mitosis, presumably by destroying the spindle apparatus, and thus inhibits divisions which are prerequisite for the initiation of xylem differentiation. While, if colchicine is applied after the necessary preparative divisions have taken place, it destroys specifically the cortical microtubules associated with the developing bands of secondary wall, thus causing aberrant wall deposition.Light and electron microscopic analysis of drug-treated cells reveals that the secondary wall becomes smeared over the surface of the primary wall and does not retain the discrete banded pattern characteristic of secondary thickenings in untreated cells. Examination of colchicine-treated secondary walls in KMnO₄ fixed material shows that in the absence of microtubules the cellulose microfibrils lose their normal parallel orientation and are deposited in swirls and curved configurations, and often lie at sharp angles to the axis of the secondary wall band. Microtubules, thus, appear to play a major role in defining the pattern of secondary wall deposition and in directing the orientation of the cellulose microfibrils of the wall. Factors in addition to microtubules also act in controlling the secondary wall pattern, since we observe that even in the absence of microtubules secondary thickenings of two adjacent xylem elements are deposited directly opposite one another across the common primary wall.     

Chromosome Transfer and Recombinant Formation with Deoxyribonucleic Acid Temperature-Sensitive Strains of Escherichia coli

Haploid recombinant yield is reduced in matings conducted at 42.5 C between deoxyribonucleic acid (DNA) temperature-sensitive [dna⁻(TS)] recipients unable to synthesize DNA at 42.5 C and any of the three major donor types (Hfr, F⁺, F′) of Escherichia coli. No such reduction is observed in matings conducted at 42.5 C when the dna⁻(TS) mutation is in the donor parent. Evidence is presented which indicates that chromosome transfer from donors to recipients unable to replicate DNA at 42.5 C during vegetative growth occurs at normal frequencies when the mating is conducted at 42.5 C. It is concluded that some stage in haploid recombinant formation is adversely affected in dna⁻(TS) recipients mated at the temperature restrictive for DNA synthesis.     

Investigations of the bipartite structure of the white-albino maize mutants

Summary Evidence from the study of alleles and modifier genes of the white-albino mutants and additional selected mutants of maize is presented suggesting that the white-albino loci have a bipartite structure. Experimental results from crossover and mutational studies failed to confirm the bipartite model. Alternative explanations for the simultaneous or independent involvement of seedling and endosperm in mutational events in these mutants are considered.Journal paper No. J-6945 of the Iowa Agriculture and Home Economices Experiment Station, Ames. Project No. 1380.     

Glucose Transport in Brucella abortus

Brucella abortus British strain 19 transported glucose with an apparent K(m) of 0.16 mM and an apparent V(max) of 250 nmol per min per mg of N. The only common glucose analogue transported was 2-deoxyglucose (2-DOG), with an apparent K(i) of 0.73 mM. Alpha- or beta-methyl glucosides and 3-O-methylglucose were not transported. Transport was linear for 70 to 90 s, depending on the concentration of substrate used. 2-Deoxyglucose was transported as the free sugar and was not further metabolized once inside the cell. There was no glucose phosphoenolpyruvate phosphotransferase system (PEP-PTS) present, and there were no inhibitors present in Brucella cell-free extract that inhibited the Escherichia coli glucose PEP-PTS. N-Ethylmaleimide (NEM) and p-chloromercuribenzoate (pCMB) completely inhibited transport of glucose and 2-DOG. Glutathione, dithiothreitol, and beta-mercaptoethanol reversed the effects of pCMB but not of NEM. A pH optimum of 7.2 and a temperature optimum of 37 to 45 C were observed for both K(m) and V(max). The glucose transport system appeared to be constitutive for glucose transport in cells grown on fructose, galactose, erythritol, or glucose. The electron transfer inhibitors carbonyl cyanide, m-chlorophenylhydrazone, NaN(3), 2,4-dinitrophenol, and KCN inhibited 2-DOG transport to a greater extent than did the metabolic energy inhibitors NaAsO(4), iodoacetate, KF, and 2-heptyl-4-hydroxyquinoline-N-oxide. Dicyclohexylcarbodiimide, an inhibitor of membrane-bound adenosine triphosphatases, inhibited transport by 100%.     

Effect of mouse genotype on interferon production. I. Lines congenic at theIf-1 locus

The level of circulating Interferon induced in mice by Newcastle disease virus is controlled by a single codominant locus,If-1, with two alleles,If-1 ^l for low andIf-1 ^h for high production. This locus is linked to the histocompatibility locusH-28. Of three C57BL/6By lines congenic for the BALB/cBy allele atH-28, two are carrying the BALB/cBy allele and one, the C57BL/6By allele atIf-1. Thus, mouse strains that are genetically very similar but different in their production of NDV-induced circulating Interferon now are available.A preliminary report of these studies was presented at the ASM meeting at Miami Beach in May 1973.     

Genetic control of the immune response in mice: V. Minor genes involved in the response to H-Y and Ea-1 antigens

Murine responses to both the male specific histocompatibility antigen H-Y and the erythrocyte alloantigen Ea-1 are regulated by genetic factors. In each case a single major gene that controls the immune response has been identified, but additional modifying factors can be demonstrated if appropriate strain combinations are studied. A single gene controlling the response to Ea-1 antigens, which segregates when strains YBR and B10.D2 are crossed, has been shown not to be an allele of theIr-2 locus. A new phenomenon has also been observed in the control of anti-Ea-1 antibody production in that the mating of two responding strains, YBR and HTG, produces an F₁ generation of complete nonresponders. By linkage tests it was shown that the responding strain HTG possesses the nonresponder allele at theIr- 2 locus, so there appear to be recessive genes in the background which are able to overcome the suppressive influence of this allele.     

Evaluation of equilibrium constants by affinity chromatography

Theoretical expressions are derived for affinity chromatography of systems comprising an acceptor A with one binding site for attachment to a functional group X on the column matrix and one site for interaction with a small ligand B that specifically affects its elution. From a general relationship covering all possible interactions between A, B and X simpler expressions are derived for affinity systems in which only two equilibria operate. Methods are suggested whereby these simpler systems may be characterized in terms of the two pertinent equilibrium constants and the concentration of matrix-bound constituent. The means by which the theory may be adapted to affinity chromatography of acceptors with multiple binding sites for ligand is also illustrated. Results of partition experiments on the Sephadex G-100-lysozyme-d-glucose system in acetate-chloride buffer (I=0.17m), pH5.4, are used to demonstrate the feasibility of evaluating quantitatively affinity-chromatography interactions. Values of 30m(-1) and 1.2x10(6)m(-1) are obtained for the equilibrium constants for the reactions of lysozyme with glucose and Sephadex respectively, there being only an occasional binding site in the polysaccharide matrix (approximately 1 in 10(5) glucose residues). In a second experimental study the phytohaemagglutinin from Ricinus communis is subjected to frontal chromatography on Sepharose 4B in the presence of different concentrations of d-galactose, the results illustrating some of the difficulties and limitations that are likely to be encountered in quantitative studies of affinity-chromatographic systems.     

Separation and properties of human brain hexosaminidase C

Hexosaminidase C was separated from human brain supernatant by immunoadsorption of the A and B forms on to a column of immobilized antibody followed by preparative starch-block electrophoresis. There were some differences in the properties of hexosaminidase C preparations after each of these stages, shown by comparison of their heat-inactivation characteristics and filtration through Bio-Gel P-200. The C form prepared by both separation steps had properties which differed markedly from those of the A and B isoenzymes; its molecular weight was much larger, greater than 200000, it had optimum activity between pH6 and 7 and could not be successfully eluted from DEAE-cellulose, even with high salt concentrations, or from Sephadex G-200. These results seem to support the proposal that the C form is under a separate genetic control from the others.