Binding of plasma fibronectin to cell layers of human skin fibroblasts

Human plasma fibronectin bound to confluent cell layers of cultured human-skin fibroblasts in two distinct pools. Initial binding of fibronectin occurred in a deoxycholate-soluble pool (Pool I). Binding in Pool I was reversible and reached a steady state after 3 h. After longer periods of incubation, fibronectin became bound in a deoxycholate-insoluble pool (Pool II). Binding in Pool II was irreversible and proceeded at a linear rate for 30 h. After 30 h of incubation, a significant proportion of fibronectin bound in Pool II was present as disulfide-bonded multimers. HT1080 cells, a human sarcoma cell line, did not bind fibronectin in either pool. Also, isolated cell matrices prepared by deoxycholate extraction did not bind fibronection. Binding of fibronectin in Pool I of normal fibroblasts occurred via specific, saturable receptors. There were 128,000 binding sites per cell, and KDiss was 3.6 X 10(-8) M. Fluorescence microscopic localization of fibronectin bound in Pool I and Pool II was performed using fluorescein-conjugated fibronectin. Fluorescent staining in Pool I was present in a punctate pattern and in short, fine fibrils. Pool II fluorescence was exclusively in coarse, dense fibrils. These data indicate that plasma fibronectin may become incorporated into the tissue extracellular matrix via specific cell-surface receptors.     

The effect of the dimeric and multimeric forms of fibronectin on the adhesion and growth of primary glomerular cells

Primary glomerular cells placed in a chemically defined medium containing Waymouth's medium MB 752/1 supplemented with insulin, transferrin, fibroblast growth factor, nonessential amino acids, sodium pyruvate, and antibiotics showed rapid outgrowth of cells which morphologically resembled well differentiated visceral epithelial cells followed by outgrowth of poorly differentiated cells; morphologic evidence suggests these latter cells are precursor cells of the epithelial cell lineage. Whereas the well differentiated glomerular epithelial cells were never observed to divide by sequential phase microscopic observations, a chemically defined medium was developed for optimal growth of the poorly differentiated cell type. This serum-free medium contained Waymouth's medium MB 752/1 supplemented with insulin, transferrin, selenium, and fibronectin (plus non-essential amino acids, sodium pyruvate, and antibiotics). Using this chemically defined medium, we have compared the effects of dimeric and multimeric fibronectin (high molecular weight disulfide-bonded fibronectin produced by incubation of dimeric fibronectin with 3 M guanidine followed by dialysis against 0.05 M cyclohexylaminopropane sulfonic acid (CAPS) buffer, pH 11) on the adhesion and growth of the poorly differentiated primary glomerular cell type. Dimeric fibronectin (FN) was twice as effective as multimeric FN in promoting glomerular cell adhesion, although both forms of FN promoted cell adhesion better than an uncoated substratum. In contrast, cell growth studies demonstrated that multimeric FN was a more potent growth stimulant than dimeric FN. The differential effects of dimeric and multimeric forms of FN in vitro suggests that these molecules may have different functions in vivo.     

Serum proteins of selected Falconiformes and Strigiformes

Blood samples were collected from ten species of raptors during the Fall 1980 migration in the vicinity of Green Bay, Wisconsin. Serum protein electrophoresis was performed on the samples in order to compare taxa based on biochemical information and relate this to current systematics. Results based on the biochemical information are generally consistent with the current systematic positions of these species within their respective orders.     

Thrombospondin is a slow tight-binding inhibitor of plasmin.

Thrombospondin is a multifunctional glycoprotein of platelet alpha-granules and a variety of growing cells. We demonstrate that thrombospondin is a slow tight-binding inhibitor of plasmin as determined by loss of amidolytic activity, loss of ability to cleave fibrinogen, and decreased lysis zones in fibrin plate assays. Stoichiometric titrations indicate that approximately 1 mol of plasmin interacts with 1 mol of thrombospondin, an unexpected result considering the trimeric nature of thrombospondin. Plasmin in a complex with streptokinase or bound to epsilon-aminocaproic acid is protected from inhibition by thrombospondin, thereby implicating the lysine-binding kringle domains of plasmin in the inhibition process. Thrombospondin also inhibits urokinase plasminogen activator, but more slowly than plasmin, stimulates the amidolytic activity of tissue plasminogen activator, and has no effect on the amidolytic activity of alpha-thrombin or factor Xa. These results, therefore, identify thrombospondin as a new type of serine proteinase inhibitor and potentially important regulator of fibrinolysis.     

Cross-linking of a major fibroblast surface-associated glycoprotein (fibronectin) catalyzed by blood coagulation factor XIII

The surface proteins of cultured human skin fibroblasts were iodinated and then exposed to one or more of the following blood coagulation proteins: thrombin, fibrinogen, and factor XIII (plasma protransglutaminase). Radiolabeled polypeptides were analyzed by polyacrylamide gel electrophoresis in the presence of sodium dodecylsulfate. After exposure to physiological concentrations of activated factor XIII (XIII_a), the band of radioactivity corresponding to the major labeled surface protein (fibronectin, molecular weight = 2.2 × 10⁵ daltons) was cross-linked to a very high molecular weight complex. The cross-linking reaction was inhibited by fibrin (which is known to bind the catalytic subunit of XIII_a). Cross-linking of labeled cell surface fibronectin to fibrin could not be demonstrated. The fibrillar pattern of surface fibronectin appeared unaffected by cross-linking when studied by immunofluorescence. Cross-linking of cell surface fibronectin by XIII_a requires highly specific enzyme-substrate and protein-protein interactions, and may be an important physiological reaction.     

Thrombin stimulates the production and release of a major surface-associated glycoprotein (fibronectin) in cultures of human fibroblasts

Exposure of cultured human skin fibroblasts to thrombin in serum-free medium had several effects on fibronectin, a major cell surface-associated glycoprotein. Pericellular fibronectin fibrils, visualized by immunofluorescence, were lost after exposure for 4–20 h to thrombin (1–8 U/ml). Loss of fibronectin fibrils did not occur if thrombin was inhibited by phenylmethyl-sulfonyl fluoride (PMSF), N-α-tosyl-1-lysyl chloromethane (TosLysCH₂Cl), alpha-1-antithrombin, alpha-2-macroglobulin, or hirudin. Cell surface fibronectin, labeled by lactoperoxidase-catalysed iodination, and newly synthesized fibronectin, metabolically labeled with [³H]mannose, were lost after exposure for 20 h to thrombin. Within 60 min, increased concentrations of fibronectin were detected by radioimmunoassay in media of thrombin-treated cultures. Thrombin increased several-fold the total amount of fibronectin accumulating in cultures over a 20 h period by increasing the amount of fibronectin secreted or shed into the medium. Fetal calf serum, which contained inhibitors of thrombin and hence only low levels of thrombin activity (<0.05 U/ml), also stimulated fibronectin production but did not cause loss of pericellular fibronectin fibrils. Thrombin or serum, under the same experimental conditions, stimulated proliferation of human fibroblasts [46]. The effects of thrombin on fibronectin may be important in wound healing and tissue repair.     

Immunocytochemical localization of fibronectin (LETS proteins) on the surface of L6 myoblasts: light and electron microscopic studies.

Fibronectin (LETS protein) is a major cell surface glycoprotein component of a variety of nontransformed, substrate-attached cells in culture. Its presence has been related to increased adhesive properties. Using the peroxidase-antiperoxidase method to localize antibodies to fibronectin, we have observed that the distribution of fibronectin on L6 myoblasts varies with the density of the culture and the differentiative state of the cells. Low density, undifferentiated cultures of L6 myoblasts have a sparse accumulation of fibronectin; the antibody-antigen reaction indicates its presence on cell membranes, especially where several cells are in proximity. Undifferentiated cells in high density cultures have two forms of fibronectin localization-a diffuse staining on the membrane and a dense staining on an extracellular filamentous matrix. This matrix is composed of filaments ranging from 20–25 nm in diameter which occur singly or coalesce to form bundles. The filaments in this matrix are also observed to have dense globules scattered along their length. These filaments, which are at least in part composed of fibronectin, also react with concanavalin A, as do certain plasma membrane components. In contrast to the observations seen in undifferentiated cells, differentiated cells or myotubes have a diffuse membrane staining with antifibronectin antibodies, and the filamentous form is usually absent.     

Birth seasonally among peasant cultivators: The interrelationship of workload,diet, and fertility

The monthly distribution of live births was analyzed over a 51-year period, 1926–1976, for a rural Taiwan fishing community. Unlike previous studies of birth seasonality, monthly distributions of births did not deviate from what would be expected by chance. This new case is shown to be consistent with the suggestion, developed by Pasternak during a study of birth seasonality in two Taiwan farming communities, that for peasant cultivators the annual cycle of production exerts a more decisive influence on birth seasonality than time of marriage or attributes of temperature, rainfall, or workload. An hypothesis that links the productive cycle to conceptions through the intervening variable of diet is presented and successfully tested using several sets of data on monthly births. A direct effect of nutrition on human fertility, suggested by recent studies of reproductive performance under conditions of nutritional stress, may largely explain seasonality of conceptions and births in populations that experience significant seasonal variation in diet.The Cross Harbor data presented in this paper were collected as part of an ongoing investigation of the comparative demography and social structure of fishing, farming, and market town communities located within a particular Chinese regional system. The support of the National Science Foundation during the period of fieldwork is gratefully acknowledged. I wish to thank G. William Skinner, William H. Durham, Greg Acciaioli, Steven Sangren, Chuang Miao-huei, Harumi Befu, and Philip L. Ritter for their comments on earlier drafts of the present article. I owe a special debt of gratitude to Burton Pasternak (City University of New York), who intellectually inspired and personally encouraged the writing of this paper.