628 research outputs found

    Proteins involved in the Vroman effect during exposure of human blood plasma to glass and polyethylene

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    The amounts of fibrinogen adsorbed to glass from various human blood plasmas have been measured as a function of time. The plasmas were 11 single donor plasmas, pooled plasma, a single donor high molecular weight kininogen (HMWK)-deficient plasma and HMWK-deficient plasma, which had been reconstituted with HMWK. For adsorption times between 1 min and 1 h more fibrinogen adsorbed from HMWK-deficient plasma compared with the amounts of fibrinogen which adsorbed from the other plasmas. This result supports the conclusion of several authors that HMWK is involved in the displacement of fibrinogen, initially adsorbed from normal human plasma to glass. Glass surfaces, pre-exposed to solutions of plasma and subsequently exposed to 1:1 diluted plasma, gives rise to a relatively high adsorption of HMWK which is independent of the plasma concentration of the precoating solution. The results indicate that HMWK from 1:1 diluted plasma is involved in the displacement of proteins from glass surfaces which had been pre-exposed to solutions with a low plasma concentration. Experiments with polyethylene as a substrate reveal that high density lipoprotein (HDL) from 1:1 diluted plasma is involved in the displacement of proteins from polyethylene surfaces which had been pre-exposed to solutions with a low plasma concentration. Moreover, evidence is presented that substantial amounts of albumin and fibrinogen, adsorbed from 1:1000 diluted plasma to glass and polyethylene, are displaced from the surfaces of these materials by proteins from 1:1 diluted plasma different from HMWK and HDL

    Detection of surface-adsorbed (lipo)proteins by means of a two-step enzyme-immunoassay: a study on the Vroman effect

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    In view of reports on the involvement of high-molecular-weight (HMW) kininogen and high-density lipoprotein (HDL) in the Vroman effect, we studied the adsorption of fibrinogen, HMW kininogen, HDL and several other proteins from pooled human plasma and congenitally HMW kininogen-deficient plasma onto glass and low-density polyethylene, both as a function of the plasma concentration and the contact time. Mixtures of purified (lipo)proteins were also included in the study. Protein adsorption was determined by means of a two-step enzyme-immunoassay. Our results support the hypothesis that HMW kininogen is involved in the displacement of fibrinogen, which is almost instantly adsorbed from normal plasma onto glass. On hydrophobic polymers like polyethylene, the low amounts of adsorbed fibrinogen and HMW kininogen from plasma and concentrated plasma solutions may be due to a preferential adsorption of HDL

    The Innovation Threshold

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    In this paper, we propose an economic model to analyse the sales out of new products. This model accounts for the fact that even among firms for which R&D is a permanent activity, a fraction of firms does not have sales of innovative products during a two-year observation period. We propose a model in which the fixed costs of introduction is a major concern in the decision making process. In a structural model we estimate the fixed costs of the market introduction of new products and explain subsequent sales of innovative products. We examine an indicator of innovative output, i.e. sales of products 'new to the firm'. We estimate fixed costs thresholds using data from the Dutch part of the Community Innovation Survey (CIS) from 1998. R&D intensity, competition and market structure have a positive impact on sales of new products. The most important factors to decrease the fixed costs threshold of introduction are product related R&D investments, R&D subsidies and knowledge spillovers.Innovation;Product R&D;Threshold model

    Transitie en toeleveranciers

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    In dit onderzoek hebben de auteurs zich specifiek gericht op het innovatievermogen van de technische toeleverende industrie binnen het glastuinbouwcluster – de kassenbouw, automatisering, klimaatsturing en installatie. Het rapport volgt twee sporen: een observatie van transitieprocessen in de toeleverende industrie, en een reflectie met ondernemers over R&D-strategieën en samenwerking. Het doel van het project was inzicht te verkrijgen in de rol van toeleveranciers in de transitie naar duurzame tuinbouw en de kansen die er voor deze sub-sector liggen in bijdragen aan deze transitie

    The Innovation Threshold

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    Dependence of endothelial cell growth on substrate-bound fibronectin

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    A better understanding of the mechanism of adhesion, spreading and proliferation of human endothelial cells (HEC) on polymeric surfaces may lead to the development of vascular prostheses which allow the formation of an endothelial lining on the luminal surface. In the present investigation the interaction of HEC with polyethylene precoated with monoclonal antibodies directed against HEC membrane antigens and against extracellular matrix compounds was studied. F(ab¿)2 fragments of a monoclonal antibody, directed against an endothelial cell membrane antigen, and F(ab')2 fragments of a monoclonal antibody, directed against cellular fibronectin, were also included in this study. Preadsorption of these antibodies and F(ab')2 fragments, including mixtures of antibodies and mixtures of F(ab')2 fragments, resulted in cell adhesion and spreading as well as moderate cell proliferation (or no proliferation) for several days. However, a good proliferation of HEC was only observed on polyethylene precoated with fibronectin or CLB-HEC-FN-140 (directed against fibronectin). These results strongly suggest that fibronectin, bound to a solid substrate, provides a biochemical signal necessary for the proliferation of HEC. The initial proliferation of HEC on other preadsorbed antibodies or F(ab')2 fragments may be explained by the fact that suspended HEC, used for cell seeding, still possess cell membrane-bound fibronectin

    The role of cellular fibronectin in the interaction of human endothelial cells with polymers

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    During in-vitro adhesion, spreading and proliferation of human endothelial cells (HEC) on tissue culture polystyrene (TCPS), cellular fibronectin is deposited onto the surface of TCPS in spite of the fact that relatively large amounts of proteins have been adsorbed from the serum-containing culture medium to this surface. Evidence is presented that serum proteins, adsorbed to the TCPS surface, are displaced by cellular fibronectin. In addition, the interaction of HEC with polyethylene, precoated with monoclonal antibodies directed against HEC membrane antigens and against extracellular matrix compounds, was studied. F(ab')2 fragments of two monoclonal antibodies were also included in this study. Preadsorption of these antibodies and F(ab')2 fragments resulted in cell adhesion and spreading as well as moderate cell proliferation (or no proliferation) for several days. A good cell proliferation of HEC was only observed on polyethylene precoated with fibronectin or an antibody directed against fibronectin. The results indicate that the direct or indirect deposition of fibronectin is a prerequisite for the proliferation of HEC. It is suggested that fibronectin, bound to a solid substrate, provides a biochemical signal necessary for the proliferation of HEC

    Опорно-анкерне кріплення гірничих виробок вугільних шахт України

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    В статье анализируется опыт применения анкерной крепи горных выработок в горно- геологических условиях угольных шахт Украины. Представлены результаты практического применения.In the article experience of applications of roof bolting of mine workings in geological conditions of Ukrainian coal mines is analyzed. Results of a practical intrusion are presented

    Interleukin 7 as interleukin 9 drives phytohemagglutinin-activated T cells through several cell cycles; no synergism between interleukin 7, interleukin 9 and interleukin 4

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    The effects of the interlenkins IL-7 and IL-9 on cell cycle progression were investigated by conventional [3H]thymidine incorporation and by the bivariate BrdU/Hoechst technique. 8oth IL· 7 and IL-9 drive phytohemagglutinin-activated T cells through more than one cell cycle, but IL-7 wasmorepotent on cell cycle progression than IL-9. Neither synergistic nor inhibitory effects were seen between various combinations of the lymphokines IL-7, IL-9 and IL-4 compared to each lymphokine alone. When T cells are activated with phytohemagglutinin for 3 days, all or most IL-4 responsive cells respond to IL-7 as weil, whereas only a part of IL-7 responders are IL-4 responders. In contrast, when T cells are activated with phytohemagglutinin for 7 days, the quantitative data of the cell cycle distribution soggest that the population of IL-7 responders is at least an overlapping, if not a real subset of the population of the IL-4 responders
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