Browsing by Author "Dowdle, Eugene B"

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    Characterization of a plasminogen activator from human melanoma cells cultured in vitro
    (1982) Heussen, Christa; Heussen, Christa; Dowdle, Eugene B
    In this thesis I describe the work that I have done on the isolation and characterization of a plasminogen activator, Mel-PA, that is released by human melanoma cells cultured in vitro. This enzyme was compared to the urinary plasminogen activator, urokinase. The human melanoma cell line, RPMI-7272, (also referred to as the "Bowes" melanoma cell line) released large amounts of Mel-PA into the surrounding medium when cultured under serum-free conditions. A subline of these cells (Bowes II) was developed that was capable of continuous growth in the absence of serum. These cells released only one type of plasminogen activator with a molecular weight of approximately 70 000 daltons. A technique was developed in which plasminogen activators were separated electrophoretically and detected in polyacrylamide gel slabs containing the co-polymerized substrates, plasminogen and gelatin. The technique was compared with the zymographic procedure developed by Granelli-Piperno and Reich (62) using fibrin-plasminogen-agarose underlays. Mel-PA was concentrated and partially purified by affinity chromatography on benzamidine-sepharose. This preparation was used to prepare rabbit antisera to the enzyme. These antibodies inhibited the activity of plasminogen activators released by all melanoma cells but had no effect on urokinase. Antibodies to urokinase had no effect on Mel-PA. A survey of human plasminogen activators and their distribution by immunochemical and electrophoretic techniques showed that tissue extracts and body fluids, with the exception of normal urine, contained mixtures of Mel-PA- and urokinase-type enzymes. Urine of patients with some types of renal disease also contained a Mel-PA type enzyme. A study of the distribution of plasminogen activators in tissues and body fluids obtained from a number of animals showed that all mammals examined had two immunochemically distinct plasminogen activators that corresponded, in their distribution, to the urokinase-like and Mel-PA-like enzymes of man. Antibodies to human Mel-PA cross-reacted with the corresponding enzyme in all mammals tested, whereas antibodies to human urokinase were species specific. The seeds of the South African legume, Erythrina latissima, contain a 20 000 dalton protein that functioned as an inhibitor of Mel-PA, plasmin, and trypsin, but had no effect on urokinase. During its reaction with the enzymes the inhibitor was cleaved by Mel-PA and trypsin but not by urokinase. The susceptible bond was straddled by an intrachain disulphide bridge. The inhibitor bound reversibly to Mel-PA and could therefore be used to develop an affinity reagent for a one-step purification procedure for Mel-PA in melanoma cell harvest fluids. Purified preparations of Mel-PA c0uld be shown to comprise both active enzyme (two chain form) and pro-enzyme (one chain form). The one chain form could be converted to the two-chain form by treatment with plasmin. It could also be shown that fibrinogen and fibrin contained a contaminating protease that was capable of converting pro-Mel-PA to Mel-PA. A comparative study of the kinetic behaviour of Mel-PA and urokinase showed numerous differences between the catalytic activities of these two enzymes. Mel-PA was capable of binding to fibrinogen insolubilized on a plastic surface whereas urokinase did not. The presence of fibrinogen enhanced the plasminogen activating activity of Mel-PA but had no effect on urokinase activity.
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    Characterization of a polypeptide factor that inhibits the growth of a human breast cancer line in vitro
    (1988) Harris, Neil S; Dowdle, Eugene B
    This thesis concerns a melanoma-derived growth regulatory factor that inhibited proliferation of several malignant human cell lines, and, in particular, a line designated UCT-BR-1, which was derived from a human breast cancer metastasis. The work is presented in four chapters. Chapter 1 provides a review of the relevant literature at the time of writing; Chapters 2 and 3 describe the experimental work that was done; and in Chapter 4 I discuss the implications of my results for current and future work in growth factors. Experimental results are presented as Charts (which may be Figures or Tables) and the methods and experimental protocols that I used are described in the Chart legends and not in the main text of the thesis. The Appendix contains details of the tissue culture techniques and descriptions of the cell lines that were used. Sources of the various laboratory materials as well as the methods that were employed for the more routine procedures are also described in the appendix.
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    The desmoplastic response : mechanisms of tumour-induced fibrogenesis
    (1989) Fearns, Colleen; Dowdle, Eugene B
    The main concern of this thesis is with desmoplasia - a process in which excessive connective tissue is deposited in a neoplasm. This is a common phenomenon in neoplasia but one whose mechanisms are poorly understood. To study the process, I used a human malignant melanoma cell line (UCT-Mel 7) that was established in this laboratory and that, when injected into athymic mice, gave rise to tumours that showed a number of interesting features. Firstly, the tumour induced a marked desmoplastic response as evidenced by a high content of hydroxyproline in tumour lysates, intense staining for reticulin in sections of the tumour and infiltration of the tumour by host mesenchymal cells. Secondly, the desmoplasia was associated in UCT-Mel 7-derived tumours with an unusual phasic pattern of growth that was related to the in vitro passage number of the melanoma cells. On occasions, murine tumours developed at the site of inoculation of human tumour cells. I have identified 2 possible mechanisms by which UCT-Mel 7 cells could have induced the desmoplastic response: either the tumour cells could have exerted their effect indirectly, i.e. via macrophages, or they could have stimulated the host's stromal cells directly. UCT-Mel 7 cells were shown to be chemotactic for mouse macrophages and human foreskin fibroblasts were stimulated, in a dose-dependent manner, to synthesize increased amounts of collagen when co-cultured with mouse peritoneal exudate cells. Stimulation could only be effected by direct cell:cell contact; medium conditioned by macrophages was not effective. The amount of stimulation was not dependent on the state of activation of the peritoneal cells nor on the strain of mouse used. Tumour cells were also found to act directly. Co-culture of UCT-Mel 7 cells and fibroblasts resulted in increased collagen synthesis by the fibroblasts. Increased synthesis of the protein was reflected in an increase in the amount of collagen mRNA. UCT-Mel 7 cell stimulated in a dose-dependent manner with an absolute requirement for intimate cell:cell contact with the fibroblasts. DNA synthesis was not required. Dexamethasone, retinoic acid and the tumour promoter, phorbol myristate acetate, had significant primary effects on fibroblast collagen synthesis but did not modify the response to melanoma cells. Indomethacin, however, had a minimal primary effect upon the fibroblasts but significantly augmented the melanoma cell effect. The nature of the stimulatory cell:cell contact is still uncertain. The gap junction inhibitor, α-glycyrrhetinic acid, did not diminish the melanoma cell effect. Preliminary findings suggested that cell-surface proteoglycans may be important. Removal of the proteoglycans with the inhibitor of proteoglycan assembly, 4-methylumbelliferyl-β-D-xyloside, abrogated the melanoma cell:fibroblast interaction. Recombinant basic fibroblast growth factor did. not seem to be involved in the desmoplastic response. It was of incidental interest to note that this compound inhibited fibroblast collagen synthesis in a manner that was augmented by the concomitant addition of heparin. A surprising finding was the production of a potent inhibitor of collagen synthesis by superinduced cells of the mouse macrophage cell line, P388D₁. This inhibitor has not been fully characterised.
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    Diamphotoxin : the arrow poison of the !Kung Bushmen
    (1980) De la Harpe, Jonathan H; Dowdle, Eugene B
    In this thesis I describe a toxic protein, diamphotoxin, that is present in the pupae of the beetle Diamphidia nigro-ornata. This insect is used as an arrow poison by the !Kung Bushmen inhabiting the savannah of eastern Namibia and western Botswana. Preliminary investigations showed that the pupae contained a 3,7 S cationic protein which caused haemolysis and, after intramuscular injection, local paralysis followed by death. By intravenous lethality assay, one 200 mg pupa contained 20 000 mouse lethal doses. Assays for the toxin were developed based upon haemolysis in vitro and lethality in vivo. These assays were used to monitor purification of the toxin. Diamphotoxin was purified by acid extraction in 0,1M glycine-HCl pH 3,0 followed by ammonium sulphate fractionation, chromatography on hydroxyl apatite, phosphocellulose and, finally, on DEAE cellulose. A consistent increase in activity after the hydroxyl apatite chromatography pointed to the removal of an inhibitor during this step. A subsequent severe loss of activity after chromatography on phosphocellulose could neither be explained nor overcome. The phosphocellulose chromatography step yielded three peaks of toxic activity. Immunological studies revealed cross-reactivity but not identity between these three toxin species. The toxin in the first peak to elute from the phosphocellulose column was purified to electrophoretic homogeneity by chromatography on DEAE cellulose. Attempts to purify the toxin in the other two phosphocellulose peaks were not successful. The isolated molecule was confirmed to be the toxin by haemolysis in a blood-agarose underlay after SDS-gel electrophoresis. The molecular weight estimate for the toxin by SDS-gel electrophoresis was 60 700 daltons and by analytical ultracentrifugation 62 100 daltons. The molecule appeared to exist as a single polypeptide chain. The amino acid composition showed a high proportion of hydrophobic amino acids. Isoelectric focussing showed an isoelectric point of pH 9,45. Toxin mediated haemolysis was studied in detail. The haemolytic event could be broken down into two stages. In the first stage toxin bound irreversibly to the cell but, provided no divalent cations were present, no damage to the cell could be detected. The second stage required the presence of free calcium (or certain other divalent cations), with an optimum concentration at 1 mM. The interaction of calcium with the cell-bound toxin resulted in the cell membrane becoming highly permeable to Na⁺ and K⁺ ions. Experiments designed to detect phospholipase or protease activity in toxin solutions gave negative results. Erythrocytes incubated with ¹²⁵I-labelled pure toxin in calcium-free medium retained a quantity of bound toxin which could not be removed by repeated washing. Incubation of erythrocytes with calcium-free toxin resulted in depletion of the activity of the toxin solution. The kinetics of the haemolytic action of the toxin were shown to be stoichiometric rather than catalytic. It was estimated that haemolysis by the toxin required a minimum of approximately 100 molecules per cell. Studies using circular dichroism measurements and the fluorescent probe 8-anilino-1-naphthalene sulphonic acid (ANS) indicated that a conformational change occurred in the toxin upon exposure to calcium. The ANS studies indicated that upon the addition of calcium the toxin molecule became more hydrophobic. It was concluded that the toxin functions as a calcium regulated Na⁺ and K⁺ ionophore in that it binds to the cell membrane and, in the presence of calcium or certain other divalent cations, assumes a conformation which mediates the free passage of Na⁺ and K⁺ ions. The resultant disruption of normal transmembranous ionic concentration gradients leads to cell lysis by loss of osmoregulation and, in the case of excitable membranes, disruption of electrophysiological activity.
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    Immunity in kwashiorkor
    (1980) Beatty, David William; Dowdle, Eugene B
    The adverse effects of malnutrition on the child are diverse and complex. This thesis describes an examination of the effects of severe malnutrition on immune defence mechanisms and in particular on cellular immune function in vitro.
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    Investigations into the complexity and polymorphism of HLA-D loci in South Africa
    (1989) Oudshoorn, Machteld; Dowdle, Eugene B
    The HLA complex is the most polymorphic genetic system known in man. The frequency of the HLA class II antigens have been well studied in Caucasoids but little data is available concerning HLA antigen frequencies in Negroes. In this thesis the class II antigens, excluding HLA-DP, were studied in South African (SA) Negroes (Xhosa), Cape Coloureds ( a group of mixed racial origin) and SA Caucasoids using serological, cellular ( HTC typing) and Southern blot techniques. The results obtained for the SA Negroes were compared with those previously found in Nigerians and American Negroes. Marked differences in HLA distribution occurred between these groups, which in part may be explained by Khoisan admixture in the SA Negroes. In addition, striking frequency differences were observed between the three SA populations. For example, in the Xhosa the HLA-DR1, DR4, DR7, DRw8, DQw2, DQw3, Dw1 and Dw3 specificities were found at a significantly lower frequency, whereas HLA-DR3, DRw6 and Dw' RSH' were found at a significantly higher frequency compared with the SA Caucasoids. The frequency in the Cape Coloureds was intermediate between those of the Xhosa and Caucasoids. In the SA Negroes and Cape Coloureds, several new specificities were detected such as HLA-DRw18, DR2 LUM(CT), DRwl2x6, DRw8x14, Dw' RSH', Dw' JOH' and Dw' BME'. The HLA-DR and DQ haplotypes in significant linkage disequilibrium were similar in the three groups. However, several haplotypes with unusual DR and DQ combinations such as HLA-DRw17,DQw7; DR9, DQw2 and DR4, DQw5 were present in the SA Negroes and Cape Coloured families. Al though some of these unusual haplotypes could be explained in terms of recombination between the common haplotypes, none could be typed using a panel of well defined homozygous typing cells, suggesting that the response observed in mixed lymphocyte culture arises from separate molecular determinants. The data on HLA class II antigen frequencies presented in this thesis is essential for future studies on HLA and disease associations and for establishing population relationships. Knowledge of new HLA class II antigens in the various population groups is also important in renal transplantation as matching for HLA-DR antigens is known to improve graft survival.
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    The penetration protease of the cercariae of Schistosoma mansoni
    (1980) Heussen, Christa; Dowdle, Eugene B
    This thesis is concerned with a study of the proteases released by the cercariae of Schistosoma mansoni while penetrating mammalian skin. The proteases present in secretions collected from the preacetabular glands of cercariae were shown to be active against ¹²⁵I-labelled fibrin but not against undenatured ³H-collagen. A sensitive solid phase radioenzyme assay, with ¹²⁵I-fibrin as the substrate, was used to show that the cercarial protease could be totally inhibited by serine protease inhibitors such as diisopropylfluorophosphate or phenylmethylsulfonyl fluoride, but not by the sulfhydryl reagents iodoacetamide or p-chloromercuribenzoate. Typical trypsin inhibitors such as soy bean trypsin inhibitor, trasylol or benzamidine inhibited the enzyme to a lesser degree. The active-site labels, TLCK, TPCK and AcAAAACK of trypsin, chymotrypsin and elastase respectively had no effect. Calcium and magnesium stimulated protease activity at concentrations below 0,5 mM, but inhibited at higher concentrations, whereas EDTA had no effect. The pH optimum of the protease lay between pH 9,0 and 9,5. From these studies, I have concluded that the major cercarial penetration protease is an alkaline serine protease with trypsin-like specificity, but not acting via the same mechanism. A technique was developed for examining cercarial proteases in polyacrylamide gels containing SDS and copolymerized gelatin substrate. Bands of proteolytic activity could be detected by negative staining. This method was used to show that cercarial secretions contained one major protease with a molecular weight of 35 000 and that crude enzyme preparations are readily contaminated with bacterial proteases. Partial purification of the major cercarial protease was achieved by cation exchange chromatography.
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    Proteolytic mechanisms involved in the metastasis of human melanoma cells
    (1994) Fletcher, Jean Margaret; Dowdle, Eugene B
    The metastatic process requires that tumour cells are capable of traversing various micro-environmental barriers, such as the basement membrane. There are various proteolytic mechanisms which could contribute to the process, plasminogen activation by tissue plasminogen activator (tPA) and urokinase plasminogen activator (uPA) is one such mechanism. Extensive reports in the literature (reviewed in the introduction) indicate that most tumour cells synthesize uPA and that it is this enzyme, particularly when receptor-bound, which plays a role in invasion. UCT-Mel 3 is a human malignant melanoma cell line which was established in our laboratory, and has been shown to be highly metastatic in the nude mouse. This cell line is typical of many melanomas in that it synthesizes only tPA and not uPA. In part 1 of this thesis I further investigated the plasminogen activator production by these cells (at the level of mRNA as well as activity) as well as expression of plasminogen activator inhibitor PAl-1 and receptors for tPA and uPA (uPAR). UCT-Mel 3 cells expressed uPAR although uPA was not detected. I also examined cells cultured from two metastatic deposits. Interestingly, the metastatic cells produced PAl-1 which was undetected in the parent cells. After confirming that UCT-Mel 3 do not express detectable levels of uPA, I attempted (in part 2) to determine whether tPA could play a comparable role to that of uPA in the invasive process. My strategy was to inhibit the expression of tPA via two different methods, namely the use of antisense RNA and ribozyme. I then hoped to isolate clones producing no tPA, which would have been injected into nude mice in order to assay for metastasis. Unfortunately, neither of these methods proved to be successful in abrogating tPA expression. I was thus unable to achieve the ultimate aim of the project. However, during the course of the study a number of unforeseen problems arose. Firstly, the clonal variation within the cell population, and secondly, my inability to obtain antisense transfectants. I have speculated that a possible reason for the latter may be that the cells are in fact unable to grow in the absence of tPA.