Network


Latest external collaboration on country level. Dive into details by clicking on the dots.

Hotspot


Dive into the research topics where Clive R. Pullinger is active.

Publication


Featured researches published by Clive R. Pullinger.


Biochimica et Biophysica Acta | 1985

Effects of hormones and pyruvate on the rates of secretion of very-low-density lipoprotein triacylglycerol and cholesterol by rat hepatocytes.

Clive R. Pullinger; Geoffrey F. Gibbons

The secretion of very-low-density lipoprotein (VLDL) triacylglycerol and cholesterol was determined under various conditions in hepatocytes prepared from rats maintained on a controlled lighting and feeding schedule. The rate of lipogenesis in hepatocytes prepared from rats during the feeding period was 2-3-fold higher than that in cells prepared immediately before the animals had access to food. However, there were no corresponding changes in the rates of secretion of triacylglycerol and cholesterol. Pyruvate alone stimulated triacylglycerol secretion but had no effect on the secretion of cholesterol. Despite its stimulation of lipogenesis, insulin suppressed the secretion of both triacylglycerol and cholesterol. This effect on triacylglycerol secretion was more pronounced when lipogenesis was enhanced in the presence of pyruvate. Thus, insulin may act to alleviate hypertriglyceridaemia, which may arise during periods of increased hepatic lipogenesis. The inhibitory effect of glucagon on cholesterol secretion was much less pronounced than that on the secretion of triacylglycerol. The inhibitory effects of glucagon were reversed by pyruvate on cholesterol secretion differed according to whether glucagon was present or absent. These results suggest that the rate of hepatic VLDL triacylglycerol secretion is not necessarily coupled to the rate of lipogenesis in the liver; nor is there any obligatory coupling between the output of triacylglycerol and cholesterol associated with VLDL.


Biochemical and Biophysical Research Communications | 1976

Lanosterol 14α-demethylase. The metabolism of some potential intermediates by cell-free systems from rat liver

Geoffrey F. Gibbons; Konstantinos A. Mitropoulos; Clive R. Pullinger

Abstract A number of potential intermediates of lanosterol ∗ 14α-demethylation have been synthesized for the first time and labelled with 3 H. A direct comparison of the rates of conversion of each of these materials to cholesterol and 5α-cholest-7-en-3β-ol by a cell-free system from rat liver has been made. Although 5α-lanost-8-en-3β,32-diol and 3β-hydroxy-5α-lanost-8-en-32-al were converted to C 27 sterols at a greater rate than was 5α-lanost-8-en-3β-ol, the apparent K m values were larger than those expected if these compounds were obligatory intermediates. 5α-Lanost-8-en-3β,15α-diol and 5α-lanost-8-en-3β,15β-diol were poorer precursors of cholesterol but each was extensively converted both to a more polar compound and to the corresponding 3β,15-diol diester.


Biochimica et Biophysica Acta | 1982

Effects of oleate and compactin on the metabolism and secretion of cholesterol and cholesteryl ester by rat hepatocytes

Clive R. Pullinger; Geoffrey F. Gibbons

Incubation of rat hepatocytes with oleate for a period of 1 h gave rise to a decrease in the total (esterified plus unesterified) cholesterol associated with very-low-density lipoprotein (VLDL). This effect was no longer apparent after longer incubation periods. The rate of cholesterol biosynthesis decreased during the first hour of incubation in the presence of oleate. After longer incubation periods, however, more cholesterol was synthesised in the presence of oleate than in its absence. The extracellular presence of oleate gave rise to a 2-fold increase in the concentration of cellular cholesteryl ester. Under these conditions cholesteryl ester contributed a larger proportion of the total cholesterol secreted with the VLDL. The cholesteryl ester associated with VLDL was derived predominantly from cholesteryl ester synthesised intracellularly. Inhibition of cholesterol synthesis with compactin did not significantly alter the rate of secretion of VLDL-cholesterol. Newly synthesised non-esterified cholesterol equilibrated with the bulk of pre-existing cellular cholesterol before secretion with the VLDL. This was true irrespective of the rate of endogenous cholesterol synthesis.


Biochemical and Biophysical Research Communications | 1981

A biphasic effect of exogenous oleate on the rate of cholesterol biosynthesis by rat hepatocytes

Clive R. Pullinger; Geoffrey F. Gibbons

Abstract Short-term (0–1 h) incubations of rat hepatocytes with oleate (2 mM) resulted in a decrease in the rate of cholesterol synthesis compared to controls incubated in the absence of fatty acid. However, during this period the activity of hydroxy-methylglutaryl coenzyme A (HMG-CoA) reductase was higher in the oleate-incubated cells. After longer incubation periods in the presence of oleate there was a higher rate of cholesterol synthesis than in the corresponding non-oleate controls and HMG-CoA reductase activity remained elevated. This biphasic effect provides an explanation for previous contradictory reports concerning the effect of exogenous fatty acids on the rate of cholesterol synthesis in liver. The present studies also suggest that in some physiological situations, the rate of cholesterol synthesis is determined by substrate supply rather than by HMG-CoA reductase activity.


Biochimica et Biophysica Acta | 1980

Metabolism of hydroxy sterols by rat liver

Geoffrey F. Gibbons; Clive R. Pullinger; T.A. Baillie; R.A. Clare

5 alpha-[16-3H]lanost-8-ene-3 beta,15 alpha-diol and 5 alpha-[16-3H]lanost-8-ene-3 beta,15 beta-diol were both extensively metabolised by rat liver enzymes in vitro. Quantitatively, the most important product in both cases was a more polar compound, tentatively identified as a 5 alpha-lanost-8-enetriol. In addition, 5 alpha-[16-3H]lanost-8-ene-3 beta,15 beta-diol gave rise to the corresponding 3 beta,15beta-diol diester, whilst with 5 alpha-[16-3H]lanost-8-ene-3 beta,15 alpha-diol only the 3 beta-hydroxyl group was esterified. The enzymes involved may normally be responsible for metabolising spontaneously produced non-enzymic oxidation products of dietary or cellular cholesterol. High concentrations of 5 alpha-[16-3H]lanost-8-ene-3 beta,15 beta-diol stimulated ester formation. With both substrates, carbon monoxide inhibited formation of the polar sterol metabolite but stimulated ester formation. Under all conditions, cholesterol was a relatively minor metabolic product of either of the 5 alpha-lanost-8-ene-3 beta,15-diols.


Archives of Biochemistry and Biophysics | 1985

Diurnal changes in the rate of cholesterogenesis in hepatocytes from fed and starved rats: effects of precursors and pancreatic hormones in vitro.

Olafur G. Björnsson; Clive R. Pullinger; Geoffrey F. Gibbons

The activity of 3-hydroxy-3-methylglutaryl coenzyme A reductase (HMG-CoA reductase) varied with a diurnal periodicity in hepatocytes prepared at different times from rats accustomed to a controlled feeding and lighting schedule. The rates of sterol synthesis varied in a similar manner but the maximum rate was not synchronous with maximum HMG-CoA reductase activity. The diurnal increase in HMG-CoA reductase activity and sterol synthesis rate started before food was offered to donor animals. Neither insulin nor glucagon had any effect on the diurnal pattern of hepatic sterol synthesis in vitro. Pyruvate inhibited sterol synthesis in hepatocytes prepared during the feeding period but had no effect at other times of day. When food was withheld from donor animals at the beginning of the normal feeding period both HMG-CoA reductase activity and the rate of sterol synthesis rapidly decreased. During this period neither insulin nor lipogenic substrates, alone or in combination, were able to restore the rates of sterol synthesis to normal values. In hepatocytes prepared from animals starved for a longer period (43 h) the decrease in the activity of HMG-CoA reductase was much less than that in the rate of sterol synthesis. In contrast to hepatocytes from fed or short-term-starved animals, the rate of sterol synthesis in these hepatocytes could be increased by glucose or pyruvate.


Biochemical Journal | 1983

The role of substrate supply in the regulation of cholesterol biosynthesis in rat hepatocytes

Clive R. Pullinger; Geoffrey F. Gibbons


Biochemical Journal | 1979

Utilization of endogenous and exogenous sources of substrate for cholesterol biosynthesis by isolated hepatocytes.

Geoffrey F. Gibbons; Clive R. Pullinger


Biochemical Society Transactions | 1978

Cholesterol biosynthesis in hepatocytes.

Geoffrey F. Gibbons; Clive R. Pullinger


Biochemical Society Transactions | 1977

The use of cholesterol oxidase in an improved method for measurement of the true rate of cholesterol biosynthesis [proceedings].

Geoffrey F. Gibbons; Clive R. Pullinger

Collaboration


Dive into the Clive R. Pullinger's collaboration.

Top Co-Authors

Avatar
Top Co-Authors

Avatar
Top Co-Authors

Avatar
Top Co-Authors

Avatar

R.A. Clare

Medical Research Council

View shared research outputs
Top Co-Authors

Avatar

T.A. Baillie

Medical Research Council

View shared research outputs
Researchain Logo
Decentralizing Knowledge