Protein kinase activity in Morris hepatomas

Rat liver protein kinase has been fractionated into five peaks of activity on isoelectrofocusing columns. The major liver peak, which was activated by cAMP, was decreased in two fast growing Morris hepatomas. The second major liver peak, independent of cAMP, was increased in the tumors.     

Phosphofructokinase isozymes of Morris hepatomas

The spin-lattice relaxation rate of solvent protons in suspensions of chloroplast thylakoid membranes undergoes a large transient depression following illumination in white light. This change appears to require the presence of chelatable paramagnetic ions; it is absent in chloroplasts exposed to 1 mm EDTA during the homogenization step of the isolation procedure, but reappears when 50 μm MnCl₂ is added to these suspensions. Conditions that inhibit light-induced R₁ changes are (i) anaerobiosis, (ii) inhibition of plastocyanin function byHg⁺²/CN, and (iii) the presence of superoxide dismutase. These observations suggest that chemical oxidation of nonfunctional Mn (II) by superoxide ion, which is generated under aerobic conditions by autooxidizable acceptors of Photosystem I, is responsible for the phenomenon. This interpretation was confirmed by experiments involving superoxide generation in the dark, using the NADPH-driven diaphorase activity of ferredoxin-NADP-reductase with benzylviologen as an autooxidizable acceptor.     

Vitamin B6 metabolism in Morris hepatomas

The enzymes involved in the metabolism of vitamin B6 were measured in Morris hepatomas and livers of female Buffalo rats fed pyridoxine-sufficient and deficient diets. Pyridoxal phosphate levels in plasmas hepatomas, and livers were also determined. Nontumor-bearing animals were maintained as controls. Regardless of the B6 nutritional status, the concentration of pyridoxal phosphate was lower in the hepatomas than in the livers of the host animals. The apoenzyme levels of ornithine decarboxylase, a pyridoxal phosphate-dependent enzyme, were higher in the hepatomas from animals fed the B6-deficient diet. Liver pyridoxine kinase activity was higher in B6-sufficient animals. In contrast, tumor pyridoxine kinase activity was influenced by B6 intake and was significantly lower than that in host liver. Liver pyridoxine phosphate oxidase activity was not significantly affected by B6 intake or by the presence of tumor. In contrast, hepatomas had little or no pyridoxine phosphate oxidase activity. Pyridoxine phosphate phosphatase activity was elevated in tumors relative to livers. These data indicate that the metabolism of vitamin B6 is markedly different in the hepatomas than in host or control livers and suggest that the tumor is apparently incapable of the complete synthesis of co-enzymatically active pyridoxal phosphate from inactive precursor forms such as pyridoxine.     

Lipid peroxidation in hepatomas of different degrees of deviation

Lipid peroxidation rate in four different hepatomas is quite different and seems to be related to their degree of deviation, low deviation tumours displaying higher peroxidative ability. Moreover, the supernatant of the highly anaplastic Yoshida hepatoma is able to decrease the peroxidation rate in normal liver microsomes. This antioxidant ability is not dependent upon an increased level of glutathione. The concentration of reduced glutathione (GSH) declines strongly during incubation in conditions favouring lipid peroxidation. Unlike normal liver homogenates, this decline of GSH in hepatomas is not due to the transformation of GSH into oxidized glutathione (GSSG) but mostly to the increased activity of the γ-glutamyl-transpeptidase pathway.     

Glucosamine 6-phosphate acetylase in rat ascites hepatomas

The fetal type enzyme pattern of glucosamine 6-phosphate acetylase (glucosamine-phosphate acetyltransferase, EC 2.3.1.4) was present in rat ascites hepatomas. The levels of acid-soluble and protein-bound amino sugars in the hepatomas were determined.     

The activity of the D-T diaphorase in experimental hepatomas

The study of some NAD(P)H dehydrogenating enzymes in one slow- and one fast-growing transplantable hepatoma has shown that the activity of the soluble enzyme D-T diaphorase is increased several-fold when compared with the activity of the control livers. The increase in enzyme activity is similar in both hepatomas, regardless of the rate of growth of the tumors. The activity of the glycerolphosphate, malic and lactic dehydrogenases are decreased in both tumors. The possible functional significance of these changes is discussed in the text.     

DNA content in cells of spontaneous hepatomas in CBA mice

The DNA content was measured in the cells of 37 well-differentiated spontaneous hepatomas from 20 CBA mice aged 18 to 22 months. In all the cases, the DNA distribution pattern was polymodal, with the class of tetraploid cells being predominant. It was independent of the tumor ability to produce AFP. No signs of aneuploidy were noted. The cells of spontaneous hepatomas were characterized by a high level of polyploidy and by a dramatic reduction in the number of binuclear cells as compared with liver cells. A tendency was recorded toward positive correlation between the degree of cellular polyploidy and tumor size. The high level of polyploidy seen in spontaneous hepatomas which is also characteristic of the normal liver is considered to be a sign of tumor maturity.     

Regulation of lipoprotein receptors on rat hepatomas in vivo

It has been shown previously that the rat hepatoma no. 7288C grown in vivo or in vitro expresses fewer receptors which recognize chylomicron remnants than does normal rat liver, and it was suggested that this may contribute to the deletion of dietary cholesterol-induced regulation of cholesterol synthesis in hepatomas (Barnard, G., Erickson, S. and Cooper, A. (1984) J. Clin. Invest. 74, 173-184). To investigate this further, Buffalo rats bearing hepatomas (HTC no. 7288C) were made hypercholesterolemic by feeding an atherogenic diet and hypocholesterolemic by ethinyl estradiol injections. Under all circumstances, tumor membranes had fewer receptors than liver membranes as measured by specific binding of [125I]chylomicron remnants. Ethinyl estradiol treatment increased the number of lipoprotein receptors 1.7-fold in liver membranes and 1.2-1.6-fold in tumor membranes, but hypercholesterolemia did not produce any significant changes in remnant binding to either liver or hepatoma membranes. Feeding an atherogenic diet induced a 2.4-fold increase in total cholesterol content in the liver, primarily as cholesterol ester; however, there was no change in total, free or ester cholesterol in the hepatomas. Acyl coenzyme A:cholesterol acyltransferase activity was low in this hepatoma line and neither treatment significantly affected its activity. One explanation for the lack of effect of the atherogenic diet on hepatoma cholesterol metabolism in addition to the decreased number of lipoprotein receptors might be the failure of access of lipoproteins to the tumor cell. To assess this, radioiodinated apo E-rich lipoproteins of various sizes were injected intravenously into rats with hepatomas. Their disappearance from the circulation was followed, and the uptake of each lipoprotein into a variety of tissues was determined. Chylomicron remnants were the most avidly removed particles. VLDLH, IDLH and HDLC were removed more slowly and less completely. None of the lipoproteins accumulated substantially in the tumors suggesting a limited access to the hepatoma tissue. Thus, in addition to the observed reduction in lipoprotein receptor number, limited lipoprotein access to the hepatoma tissue may be a significant factor in contributing to the apparent lack of feedback regulation of cholesterol synthesis by hepatoma tissue in vivo.     

Enzymic imbalance in serine metabolism in rat hepatomas.

The renaturation of the tetrameric enzyme phosphoglycerate mutase from baker's yeast after denaturation in guanidinium chloride was studied. Three proteinases (trypsin, chymotrypsin and thermolysin) cause extensive loss of activity of samples taken during the early stages of refolding. As judged by SDS/polyacrylamide-gel electrophoresis, the proteinases cause substantial degradation of the polypeptide chain with no evidence for large quantities of fragments of Mr greater than 6500. These data suggest that the early intermediates in the refolding, especially the folded monomer, possess a number of sites that are susceptible to proteolysis.     

Changes in the glucose-6-phosphatase complex in hepatomas

Hepatomas tend to have a decreased glucose-6-phosphatase activity. We have observed phenotypic stability for this change in Morris hepatomas transplanted in rats. To determine if this decrease is selective for translocase functions or the hydrolase activity associated with glucose-6-phosphatase, we have compared activities in liver and hepatomas with glucose-6-phosphate or mannose-6-phosphate as substrates and with intact or histone-disrupted microsomes. In five out of seven subcutaneously transplanted rat hepatoma lines, the microsomal mannose-6-phosphatase activity was lower than in preparations from liver of normal or tumor-bearing rats. With liver microsomes and with most hepatoma microsomes, preincubation with calf thymus histones caused a greater increase in mannose-6-phosphatase than in glucose-6-phosphatase activity. In studies with liver and hepatoma microsomes there were similar increases in mannose-6-phosphatase activity with total calf thymus histones and arginine-rich histones. A smaller increase was seen with lysine-rich histones. The effect of polylysine was similar to the action of lysine-rich histones. There was only a small effect with protamine at the same concentration (1 mg/ml). Rat liver or hepatoma H1 histones gave only about half the activation seen with core nucleosomal histones. Our data suggested that microsomes of rat hepatomas tend to have decreased translocase and hydrolase functions of glucose-6-phosphatase relative to activities in untransformed liver. (Mol Cell Biochem122: 17–24, 1993)