Walter Troll

Tumorigenesis in Mouse Skin: Inhibition by Synthetic Inhibitors of Proteases

Three synthetic inhibitors of proteases (tosyl lysine chloromethyl ketone, tosyl phenylalanine chloromethyl ketone, and tosyl arginine methyl ester) inhibit the tumorigenesis initiated in mouse skin by 7,12-dimethylbenz(a)anthracene and promoted by croton oil or its active principle, phorbol ester. These protease inhibitors, when applied directly to mouse skin, inhibit some of the irritant effects of the tumor promoter and are not toxic.

Protease inhibitors antagonize the activation of polymorphonuclear leukocyte oxygen consumption

Abstract We report that the burst of oxygen consumption, as well as the resultant production of O 2 − • and H 2 O 2 , occurring in activated human polymorphonuclear leukocytes is inhibited by various compounds which have in common the ability to antagonize the effects of proteolytic enzymes. This effect of protease inhibitors was observed with a variety of stimuli, both phagocytic and non-phagocytic, used to activate O 2 − • production in human polymorphonuclear leukocytes. Inhibition was also noted in rat polymorphonuclear leukocytes and alveolar macrophages. The results indicate that proteolysis may be involved in activating the burst of oxygen consumption following stimulation of phagocytic cells.

Stimulation of human polymorphonuclear leukocyte superoxide anion radical production by tumor promoters

Comparison was made of the ability of the potent tumor promoter phorbol myristate acetate (PMA), as well as less active PMA analogs and non-phorbol ester tumor promoters, to stimulate superoxide anion radical (O-.2) production by human polymorphonuclear leukocytes (PMN). The rate of O-.2 production was found to correlate with the tumor-promoting activity of the phorbol esters as opposed to their inflammatory activity. Mezerein and telocidin B were slightly better stimulators of O-.2 production than PMA. Acetic acid was inactive. These data are discussed in terms of a possible role for O-.2 and other reactive oxygen species in tumor promotion.

Retinoid inhibition of superoxide anion radical production by human polymorphonuclear leukocytes stimulated with tumor promoters

Abstract All-trans retinol, retinyl acetate and retinoic acid were found to be effective inhibitors of O 2 − • polymorphonuclear leukocytes stimulated with the tumor promoter phorbol myristate acetate. Retinol similarly inhibited cells stimulated with mezerein or teleocidin B. No-effect concentrations of the protease inhibitor antipain potentiated the inhibitory effect of low levels of retinol. Higher concentrations of retinol and antipain resulted in an additive or less than additive inhibitory effect.

Protease inhibitors as cancer chemopreventive agents

Protease inhibitors (PIs), which are widely distributed in plants and animals and have a variety of functions, interfere with cancer development in a number of ways, including suppression of oxygen radicals, oncogenes, and metastases. Epidemiologic evidence supports their prevention of major human c

The effect of epsilon amino caproic acid and other inhibitors of proteolysis upon the response of human peripheral blood lymphocytes to phytohemagglutinin.

Previous work has suggested that intracellular proteolysis may play a role in lymphocyte stimulation. An inhibitor of proteolysis, epsilon amino caproic acid (EACA) was studied for its effect on the lymphocyte response to phytohemagglutinin (PHA). EACA was found to inhibit several parameters of lymphocyte stimulation (e.g. DNA, RNA, and protein synthesis as well as alterations in morphology) This inhibition was not due to diminished cellular viability and did not permanently impair the capacity of the lymphocyte to subsequently respond to PHA. Additionally, there was no evidence that this inhibition was due to other possible effects of EACA, such as alterations in Na(+) - K(+) transport, competitive amino acid deprivation or interference with PHA binding. Moreover, the inhibitors of proteolysis, tosyl arginine methyl ester (TAME), tosyl lysine chloromethyl ketone (TLCK), and tosyl phenyl-alanine chloromethyl ketone (TPCK), were also shown to inhibit lymphocyte stimulation.EACA was most effective when added during the first 24 hr of stimulation. Therefore, these experiments support the hypothesis that proteolysis is an essential step in the early phase of lymphocyte activation.

Anticarcinogenic Action of Protease Inhibitors

Protease inhibitors are synthesized in biological systems and play a critical role in controlling a number of diverse physiological functions. They participate in blood clotting and lysis of clots, in growth processes by modulation of proteolytic digestion of proteins and thus availability of amino acids, and in the induction of selective DNA amplification. When incorporated into the diet, protease inhibitors appear to suppress many types of cancer. In vitro, they suppress neoplastic transformation caused by chemical carcinogens, ionizing radiation, and oncogenes. These observations offer the hope that judiciously applied protease inhibitors in small concentrations may prevent a wide range of human cancers. This hope is further supported by epidemiological studies which show that populations consuming relatively large amounts of protease inhibitors have a lower occurrence of cancer. The tasks remaining are to determine the kind and the level of protease inhibitors that are most effective in preventing cancer without also having toxic side effects and to incorporate them into our diet. Perhaps the most encouraging investigations are those using small nontoxic protease inhibitors available in pure form (epsilon-aminocaproic acid, a trypsin plasminogen activator inhibitor, and nicotinamide, a chymotrypsin inhibitor and known vitamin). Both agents have been shown to be preventive agents of cancer in animals and in vitro models. Further studies with natural protease inhibitors may yield even more effective agents which when incorporated into our diet will prevent the development of many types of cancer.

Sensitive proteolytic enzyme assay using differential solubilities of radioactive substrates and products in biphasic systems

Abstract A continuous assay for proteolytic enzymes capable of measuring 1 nanogram of crystalline trypsin, using tritium-labeled methyl esters of arginine and lysine, is described. Two novel applications of this method have been: (1) the determination of tissue and nuclear proteoesterases and (2) a differential method for the determination of thrombin where plasmin and other trypsin-like enzymes are inhibited by lysine methyl ester.

A hydrogen peroxide block to polyspermy in the sea urchin Arbacia punctulata

Abstract Fertilization by more than one sperm in sea urchins inevitably leads to uneven division and death of the embryo. We provide evidence for a block against this polyspermy involving the hydrogen peroxide release by the egg during fertilization that is triggered by entry of the successful sperm. Polyspermy in 100% of fertilized eggs was demonstrated when catalase was added to destroy hydrogen peroxide immediately after fertilization. Soybean trypsin inhibitor, another polyspermic agent, is shown to prevent the formation of hydrogen peroxide in the fertilized egg. This suggests that the protease released from egg cortical granules during fertilization plays a role in the hydrogen peroxide generating system.

Effects of sodium arsenite on the survival of UV-irradiated Escherichia Coli: INHIBITION OF A rec A-Dependent function

Epidemiological studies and clinical observation suggesting potential hazards of arsenic compounds in increasing the incidence of cancer have been in complete contradiction with experimental findings in animals. Because of the predominance of skin cancers in the epidemiological reports, we decided to investigate the possibility that arsenic compounds might interfere with DNA repair. Using Escherichia coli as a test system, we show that this is indeed the case. Sodium arsenite, at concentrations of 0.1 mM and higher, decreases the survival of ultraviolet-irradiated E. coli WP2, a strain which possesses the full complement of repair genes. The effect of the arsenite increases with increasing ultraviolet dose. Similar results were obtained with the excision repair deficient strains WWP2 (uvrA) and WP6 (polA). Sodium arsenite had no effect on the survival of a recA mutant, WP10. Survival of ultraviolet-irradiated WP5 (exrA) was enhanced by sodium ardenite, the effect being greatest at low ultraviolet doses. It is postulated that arsenite inhibits a recA-dependent step in DNA repair. To account for the increased survival of the exrA mutant, we suggest that in the absence of the exr+ gene, the arsenite-sensitive recA-dependent function is deleterious. The ability of arsenite to inhibit DNA repair may account for the clinical and epidemiological reports linking arsenicals with an increased incidence of cancer.