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Journal of Lipid Research, Vol. 47, 1620-1630, August 2006
Copyright © 2006 by American Society for Biochemistry and Molecular Biology

Thematic Review

Thematic review series: Patient-Oriented Research. What we have learned about VLDL and LDL metabolism from human kinetics studies

Klaus G. Parhofer^*,1 and P. Hugh R. Barrett

^* Medical Department II, Grosshadern University, Munich, Germany
Metabolic Research Centre, School of Medicine and Pharmacology, University of Western Australia, Perth, Australia

Published, JLR Papers in Press, May 23, 2006.

¹ To whom correspondence should be addressed. e-mail: klaus.parhofer{at}med.uni-muenchen.de

	ABSTRACT

TOP ABSTRACT INTRODUCTION NORMOLIPIDEMIC SUBJECTS FAMILIAL HYPERCHOLESTEROLEMIA... PATIENTS WITH THE METABOLIC... DYSBETALIPOPROTEINEMIA (TYPE III... HYPOBETALIPOPROTEINEMIA CONCLUSION REFERENCES

 
Lipoprotein metabolism is the result of a complex network of many individual components. Abnormal lipoprotein concentrations can result from changes in the production, conversion, or catabolism of lipoprotein particles. Studies in hypolipoproteinemia and hyperlipoproteinemia have elucidated the processes that control VLDL secretion as well as VLDL and LDL catabolism. Here, we review the current knowledge regarding apolipoprotein B (apoB) metabolism, focusing on selected clinically relevant conditions. In hypobetalipoproteinemia attributable to truncations in apoB, the rate of secretion is closely linked to the length of apoB. On the other hand, in patients with the metabolic syndrome, it appears that substrate, in the form of free fatty acids, coupled to the state of insulin resistance can induce hypersecretion of VLDL-apoB. Studies in patients with familial hypercholesterolemia, familial defective apoB, and mutant forms of proprotein convertase subtilisin/kexin type 9 show that mutations in the LDL receptor, the ligand for the receptor, or an intracellular chaperone for the receptor are the most important determinants in regulating LDL catabolism. This review also demonstrates the variance of results within similar, or even the same, phenotypic conditions. This underscores the sensitivity of metabolic studies to methodological aspects and thus the importance of the inclusion of adequate controls in studies.

Supplementary key words very low density lipoprotein • low density lipoprotein • stable isotope • turnover study

	INTRODUCTION

TOP ABSTRACT INTRODUCTION NORMOLIPIDEMIC SUBJECTS FAMILIAL HYPERCHOLESTEROLEMIA... PATIENTS WITH THE METABOLIC... DYSBETALIPOPROTEINEMIA (TYPE III... HYPOBETALIPOPROTEINEMIA CONCLUSION REFERENCES

 
Disorders of lipoprotein metabolism are usually characterized by static measurements of increased or decreased plasma lipid or apolipoprotein concentrations. In addition, disorders are often characterized by describing the function of specific components of the lipoprotein metabolic system that are defective (i.e., receptor defect, enzyme defect, protein defect, etc.). However, lipoprotein metabolism represents a complex network of many components, and it is important to appreciate that this complexity is far greater than that of the individual components. Abnormal concentrations of lipids and apolipoproteins can result from changes in the production, conversion, or catabolism of lipoprotein particles. Thus, although static measurements and functional assays are important techniques that provide mechanistic clues,in the end, it is necessary to study the true unit of function (the integrated metabolic pathway) to understand the complexity of biochemical networks such as lipoprotein metabolism.

Such biochemical networks can best be studied using tracers, which allow, together with concentration measurements, the quantification of transport rates. With respect to lipoprotein metabolism, tracers can be either radioactive or stable isotopes, and lipoproteins can be labeled either endogenously or exogenously. The advantages and disadvantages of these methodological aspects are discussed elsewhere in detail (1, 2). In brief, radioactive tracers are easier to follow from a methodological point of view, but their use is limited by possible health hazards. With exogenous labeling (i.e., lipoproteins are isolated, labeled, and reinjected), the tracer may not necessarily follow the tracee, whereas endogenous labeling (i.e., a labeled amino acid is incorporated into the apolipoprotein under study) requires more sophisticated methods of analysis.

Advances in gas chromatography-mass spectrometry technology and the availability of inexpensive stable isotopes have resulted in an increasing use of endogenous labeling of apolipoproteins with labeled (stable isotopes) amino acids (1, 3–5). Furthermore, new stable isotope methodologies have been developed to study reverse cholesterol transport, fatty acid turnover, and cholesterol absorption (6–10). Therefore, in recent years, most studies evaluating aspects of human in vivo apolipoprotein B (apoB) metabolism have used amino acids labeled with stable isotopes as endogenously incorporated tracers and have combined this methodology with multicompartmental modeling for the analysis of enrichment data. This contrasts with early studies, which established the basic metabolic pathways using radio-iodinated lipoproteins. Notably, most findings established with radiotracers have later been confirmed using endogenous labeling with stable isotopes.

Here, we review the current knowledge of apoB metabolism using selected, clinically important conditions, with special focus on studies using stable isotope methodology. One particular goal is to demonstrate the variance of results (and thus conclusions) within similar, or even the same, phenotypic conditions. This underscores the sensitivity of metabolic studies to methodological aspects and thus the importance of the inclusion of adequate controls in any studies. We also stress that some studies include very few subjects and therefore must be interpreted cautiously.

	NORMOLIPIDEMIC SUBJECTS

TOP ABSTRACT INTRODUCTION NORMOLIPIDEMIC SUBJECTS FAMILIAL HYPERCHOLESTEROLEMIA... PATIENTS WITH THE METABOLIC... DYSBETALIPOPROTEINEMIA (TYPE III... HYPOBETALIPOPROTEINEMIA CONCLUSION REFERENCES

 
VLDL- and LDL-apoB metabolism
The main structural apolipoprotein of VLDL, intermediate density lipoprotein (IDL), and LDL is apoB-100. This apolipoprotein remains with the particle, and the lipid content changes as the particle is metabolized. Early studies demonstrated a precursor-product relationship between VLDL, IDL, and LDL particles. Subsequent studies have shown that VLDL and LDL are kinetically heterogeneous groups of particles and thus should be represented by several compartments in multicompartmental models (3, 11) (Figs. 1 , 2 ). The physiological relevance of the subfractions required from a kinetics analyst's point of view remains to be determined. Furthermore, there is some controversy over whether or not there is a direct input of apoB-100 from the liver into the IDL and LDL fractions. Cell experiments, animal models, and some human studies support the concept that the liver is capable of producing apoB-100-containing lipoproteins of different densities, including LDL particles. However, human tracer data are also compatible with the existence of a fast turning-over VLDL compartment, which can shift newly secreted apoB directly to the LDL fraction (3). Demant and colleagues (12) showed that the dispute cannot be resolved by turnover studies because the rapid appearance of labeled apoB in the LDL fraction, after the bolus of labeled amino acids, may be attributable to either direct secretion or a rapidly turning-over VLDL compartment. Based on cell experiments, most researchers now assume that the liver is capable of secreting apoB-containing particles of different densities and thus include a pathway allowing for the direct production of different VLDL subfractions as well as IDL and LDL. A detailed description of apoB secretion is particularly important because perturbations such as weight loss and pharmacotherapy can change not only total apoB production but also the type of particles secreted: less VLDL-apoB secretion has been associated with more direct LDL secretion (13).

View larger version (13K): [in this window] [in a new window]   Fig. 1. Combined model of VLDL-apolipoprotein B (apoB) and VLDL-triglyceride (TG) metabolism (11). The model incorporates a leucine and a glycerol subsystem, which account for triglyceride and apoB synthesis and secretion. The model was used to quantify VLDL-apoB and VLDL-triglyceride metabolism in normolipidemic subjects and patients with the metabolic syndrome.

View larger version (10K): [in this window] [in a new window]   Fig. 2. Model of LDL subfractions. Rebound analysis of apoB mass after apheresis in different LDL subfractions indicates that small, dense LDLs are derived from larger LDLs and from LDL precursors in familial hypercholesterolemia heterozygotes (50). IDL, intermediate density lipoprotein.

It is of great interest to establish whether VLDL secretion differs in the fasted and fed states and whether dietary composition can affect VLDL secretion. Marsh et al. (15) and Watts, Moroz, and Barrett (14) conclude from their meta-analyses that VLDL-apoB-100 production rate is higher in the fed state (25 vs. 14 mg/kg/day), whereas IDL- and LDL-apoB-100 kinetics parameters appear to be less affected by feeding, although there is considerable variation. This variation may relate to different feeding protocols used by the different groups (continuous feeding vs. bolus, fat load vs. mixed meal, etc.). When interpreting these data, it is important to keep in mind that feeding (as it occurs in real life, when larger meals are ingested in an uncontrolled setting) is difficult to study because of the non-steady-state situation induced by the meal.

Effect of interventions on VLDL- and LDL-apoB metabolism in normolipidemic subjects
Very few studies have examined the effect of nutrition on apoB metabolism in normolipidemic subjects. Stacpoole et al. (18) reported that in two normolipidemic subjects a high-carbohydrate, low-fat intake shifted the production of small VLDL particles to large VLDL particles. At the same time, the conversion of VLDL to LDL was reduced. The effect of fish oil supplements on VLDL-apoB-100 kinetics was investigated by Bordin et al. (19). Four weeks of feeding fish oil supplements resulted in a decreased production of VLDL-apoB-100 and a decreased triglyceride concentration. Similar findings have been reported in earlier studies using radioactive tracers (20).

Similarly, few studies have examined the effect of lipid-lowering drugs on apoB metabolism in normolipidemic subjects. Watts and colleagues (21) reported that simvastatin decreased the hepatic secretion of VLDL-apoB by 46% without altering VLDL FCR. LDL-apoB metabolism was not determined in this study. Malmendier et al. (22) evaluated the effect of simvastatin on LDL metabolism in normolipidemic subjects using radiolabeled LDL. A significant increase in LDL-apoB FCR was observed, whereas LDL production did not change. There is no study in normolipidemic subjects in which the effect of statin therapy on VLDL-, IDL-, and LDL-apoB metabolism is evaluated simultaneously. Furthermore, no kinetics studies using fibrates or nicotinic acids have been performed in normolipidemic subjects.

	FAMILIAL HYPERCHOLESTEROLEMIA AND FAMILIAL DEFECTIVE APOB

TOP ABSTRACT INTRODUCTION NORMOLIPIDEMIC SUBJECTS FAMILIAL HYPERCHOLESTEROLEMIA... PATIENTS WITH THE METABOLIC... DYSBETALIPOPROTEINEMIA (TYPE III... HYPOBETALIPOPROTEINEMIA CONCLUSION REFERENCES

 
VLDL- and LDL-apoB metabolism in familial hypercholesterolemia
Radiolabeling studies indicated very early that patients with familial hypercholesterolemia (FH) are characterized by a decreased clearance of LDL particles (23), which is in agreement with the underlying LDL receptor defect. Further studies have mainly focused on VLDL and IDL metabolism. Most studies report an abnormal VLDL metabolism. Cummings and colleagues (24) reported an increased secretion of VLDL, in agreement with a study by Tremblay et al. (25), who reported 50% and 100% increases in VLDL-apoB production in heterozygous and homozygous FH, respectively. On the other hand, Fisher and colleagues (26, 27) reported a decreased VLDL-apoB production rate but an increased direct production of IDL and LDL. In addition, these authors reported a dramatically altered conversion rate of VLDL to LDL. In normolipidemic subjects, between 30% and 50% of VLDL-apoB is converted to LDL; this fraction increases to 100% in FH. The discrepancies between different studies with respect to VLDL and IDL metabolism may also relate to the underlying molecular defect, because FH can be caused by a number of different mutations, as reviewed recently (28). Thus, Millar and colleagues (29) showed that receptor-defective FH patients had a total apoB production similar to controls, whereas receptor-negative FH patients had a significantly greater total apoB production than controls. Overall, in FH, the FCR of LDL-apoB (and to a lesser extent VLDL- and IDL-apoB) is decreased. Production rates also seem to be altered, with the majority of studies showing increased VLDL, IDL, and LDL production.

VLDL- and LDL-apoB metabolism in familial defective apoB-100
Several studies have addressed apoB metabolism in familial defective apoB-100 (FDB) (30–33). These studies uniformly indicate that LDL-apoB FCR is decreased to a similar extent as seen in FH. These studies also agree with respect to the production of LDL, which in all studies was found to be lower than in FH. There are, however, some differences concerning VLDL and IDL metabolism. Pietzsch and colleagues (32) reported that large VLDL₁ particles are produced at normal rates but smaller VLDL₂ particles are produced at an increased rate. At the same time, the FCR of IDL-apoB was increased (+76%) and the transfer rate to LDL was decreased, resulting in an overall reduction of LDL production of 39%. These data were confirmed, to a large extent, by Gaffney and colleagues (31) and by Schaefer et al. (33). Zulewski and colleagues (30), on the other hand, also found an increased production of VLDL but a decreased production of IDL and a nonsignificant decrease in IDL FCR. The differences between these studies with respect to VLDL and particularly IDL metabolism probably relate to the fact that the studies by Pietzsch, Gaffney, and Schaefer and colleagues (31–33) were performed in the fasting state, whereas the study by Zulewski et al. (33) was performed in the fed state.Together, these data indicate that the decreased production of LDL-apoB in FDB may originate from an enhanced removal of apoE-containing LDL precursors by LDL receptors, which may be upregulated in response to the decreased flux of LDL-derived cholesterol into hepatocytes.

VLDL- and LDL-apoB metabolism in proprotein convertase subtilisin/kexin type 9 mutations
In recent years, mutations in the proprotein convertase subtilisin/kexin type 9 (PCSK9) gene have also been reported as possible causes of hypercholesterolemia. Overexpression of PCSK9 in the livers of mice results in a marked reduction in LDL receptors in this organ (34–37) and an inhibition of LDL clearance in mice and cultured cells (36). Thus, an increased LDL-apoB FCR would be the expected primary abnormality in kinetics studies. However, Ouguerram and colleagues (38) reported that PCSK9 mutations dramatically increase the production of apoB-100 compared with controls or FH patients with an LDL receptor mutation. These patients also showed a decrease in VLDL and IDL conversion and a decreased LDL FCR (–30%) that was still higher than that observed in LDL receptor-mutated FH. These findings again highlight the close functional relationship between apoB secretion and LDL catabolism (39). Interestingly, several nonsense mutations of PCSK9 result in hypobetalipoproteinemia (40), which is associated with longevity (41). Although no kinetics studies have been performed in these subjects, one could imagine that these forms of hypolipoproteinemia are characterized by both low production of VLDL-apoB and increased catabolism of LDL.

Effect of interventions on VLDL- and LDL-apoB metabolism in FH or FDB
Given the impact of statin therapy on LDL concentrations in patients with FH or FDB, it is surprising that few studies have examined the effect of these drugs on apoB metabolism in such patients. Most studies were performed using radiolabeled lipoproteins as tracers. In 1983, Bilheimer and colleagues (42) demonstrated that mevinolin (lovastatin) and colestipol decreased LDL-cholesterol by 27% in patients with heterozygous FH. This modest decrease in LDL-cholesterol was associated with a 37% increase in LDL-apoB FCR, whereas LDL production did not change. Later, the same group reported that the same combination (mevinolin and colestipol) decreased LDL-cholesterol by 52%, increased LDL FCR by 40%, and decreased production by 26% (43). Thus, in heterozygous FH patients, statins primarily affect LDL FCR, whereas production is only decreased with higher doses, resulting in more pronounced LDL reduction. In children with homozygous FH, lovastatin did not affect the plasma concentration or metabolism of LDL, but it decreased VLDL production by 74% (44). In more recent studies performed using stable isotope methodology in six heterozygous FH patients, simvastatin decreased VLDL-apoB production by 83% with no significant effect on VLDL FCR (45). IDL and LDL kinetics were not studied. However, in another study with mild hypercholesterolemia, it was shown that pravastatin significantly increased LDL FCR by 24% with no significant effect on production (46). In a further study, Winkler and colleagues (47) demonstrated that lifibrol increased LDL-apoB FCR by 75% and increased LDL-apoB production by 33% without affecting VLDL or IDL kinetics.

A number of studies have evaluated the effect of LDL apheresis on kinetics parameters in FH patients. Regular LDL apheresis (weekly reduction of LDL-cholesterol concentration by 60%) did not affect VLDL-, IDL-, or LDL-apoB kinetics parameters. ApoB metabolism was studied with stable isotopes before the first apheresis and then again after 3–6 months of weekly apheresis. Both studies revealed the same kinetics parameters (48). However, when apoB metabolism before and immediately after LDL apheresis was compared, it was shown that VLDL-to-LDL conversion decreased temporarily from 76% to 51%. Furthermore, the tracer data indicated that in some patients LDL-apoB FCR increased transiently by 50% after apheresis (49).

Because LDL apheresis has little effect on endogenous apoB metabolism, it can also be used as a tool to study certain aspects of apoB metabolism. After apheresis, the concentration of apoB in LDL subfractions was analyzed. The resulting rebound curves were used to determine whether small, dense LDL particles are the metabolic product of LDL precursors or of larger LDL particles. In statin-treated heterozygous FH patients, small, dense LDL appeared to originate from both sources (50) (Fig. 2). Whether this is also true in other forms of hyperlipoproteinemia remains to be determined. This study also demonstrates that non-steady-state kinetics can be used to determine metabolic parameters in the absence of a tracer (51), although additional assumptions with respect to modeling are required (51a).

	PATIENTS WITH THE METABOLIC SYNDROME AND/OR TYPE 2 DIABETES

TOP ABSTRACT INTRODUCTION NORMOLIPIDEMIC SUBJECTS FAMILIAL HYPERCHOLESTEROLEMIA... PATIENTS WITH THE METABOLIC... DYSBETALIPOPROTEINEMIA (TYPE III... HYPOBETALIPOPROTEINEMIA CONCLUSION REFERENCES

 
VLDL- and LDL-apoB metabolism
ApoB metabolism in the metabolic syndrome and related disorders was recently reviewed by Chan, Barrett, and Watts (52). Individuals with insulin resistance have increased secretion rates of VLDL-apoB and triglycerides. The FCRs of VLDL-apoB and VLDL-triglycerides as well as of LDL-apoB are reduced compared with lean individuals (53–56). Visceral fat (57), hepatic fat (58), insulin resistance (59), and plasma adiponectin (60) seem to be the primary regulators of abnormal apoB and triglyceride kinetics in this condition. An increased amount of peritoneal fat results in an alteration of portal free fatty acid flux (61), an altered pattern of adipocytokines (62), and a disturbed ratio of proinflammatory to anti-inflammatory processes (63). It is currently unknown how these factors (FFA, adipocytokines, inflammation) affect each other, but they seem to be intimately linked. Although each factor may increase VLDL secretion by itself, it is the altered flow of free fatty acids that probably has the greatest impact on driving hepatic VLDL overproduction.

Although initial studies indicated an overall overproduction of VLDL particles, recent studies indicate a more complex abnormality. Adiels and colleagues (11, 54) developed a multicompartmental model that allows the kinetics of triglyceride and apoB-100 in different VLDL factions to be assessed simultaneously (Fig. 1). They found a significant positive correlation between triglyceride and apoB production in VLDL₁ and VLDL₂. Insulin resistance and type 2 diabetes were associated with excess hepatic production of VLDL₁ but not VLDL₂ particles. The direct secretion of VLDL₂-apoB and triglycerides was comparable in insulin-resistant and insulin-sensitive subjects, consistent with previous studies (11, 54, 64), indicating that VLDL₁ and VLDL₂ production are independently regulated. The overproduction of VLDL₁ particles may result in a number of subsequent metabolic abnormalities, such as abnormal postprandial lipoprotein metabolism, the generation of small, dense LDL particles, and the increased catabolism of HDL particles (65).

An increased concentration of VLDL₁ results in an increased exchange of triglycerides for cholesteryl ester in HDL particles. This process, which is mediated by cholesteryl ester transfer protein, results in the formation of short-lived triglyceride-rich HDL particles and explains why hypertriglyceridemia is associated with low HDL-cholesterol. A similar process is probably responsible for the formation of small, dense LDL particles, although the formation of small, dense LDL may be the result of a more complex interaction.

Effect of interventions on VLDL- and LDL-apoB metabolism in patients with the metabolic syndrome and/or type 2 diabetes mellitus
The effect of nutritional interventions on apoB metabolism in patients with the metabolic syndrome or type 2 diabetes mellitus was recently reviewed by Barrett and Watts (66). Riches et al. (67) demonstrated that weight reduction decreases hepatic apoB secretion and increases LDL catabolism, although in another study reduction of abdominal fat resulted in a decreased rate of VLDL-triglyceride secretion that was not accompanied by decreased VLDL-apoB secretion (68). In another study in hypertriglyceridemic, obese patients, weight reduction induced complex changes in VLDL and LDL metabolism (13). VLDL secretion and LDL FCR were decreased, whereas LDL production remained unchanged. However, weight reduction was associated with changes in the source of LDL-apoB. Before weight loss, 73% of LDL was derived from VLDL and 27% from direct secretion, whereas after weight loss, only 47% originated from VLDL and 53% was secreted directly.

Fish oil supplements decrease VLDL-apoB secretion, do not alter VLDL-apoB FCR, and increase VLDL- to LDL-apoB conversion, accounting for the absence of any effect on plasma LDL-apoB (69). Plant sterols decrease the hepatic secretion of VLDL-apoB in hypercholesterolemic diabetics resulting from a reduced hepatic cholesteryl ester pool. Somewhat surprisingly, LDL-apoB catabolism was not changed by sitostanol in this condition (70). The effect of plant sterols or stanols on apoB kinetics in subjects with the metabolic syndrome has yet to be tested.

The effects of statins and other lipid-lowering drugs on apoB metabolism in patients with the metabolic syndrome were recently reviewed by Chan, Barrett, and Watts (52). A large body of evidence suggests that statins significantly increase the catabolism of all apoB-100-containing lipoproteins, such as VLDL, IDL, and LDL. With respect to VLDL-apoB secretion, the results are less consistent, with some studies showing no effect on apoB secretion (71–74) and others demonstrating a decrease in VLDL secretion during lovastatin or simvastatin therapy (75, 76). A recently published study further questions whether statin therapy can indeed affect VLDL-triglyceride secretion (77). In this study, the triglyceride-lowering effect of statins was solely attributable to increased triglyceride clearance.

Thus, in patients with the metabolic syndrome, the effect of statins on apoB metabolism seems to be more complex than in FH, in which statins primarily increase LDL FCR and decrease production, but only at higher doses. A recently published review (78) indicates that the effect of statins is dependent upon the lipoprotein phenotype before treatment. In patients with low LDL FCR at baseline, statins increase the FCRs of all apoB-containing lipoproteins, whereas in patients with normal LDL FCR, statins primarily decrease apoB production. In the metabolic syndrome, however, in which the state of insulin resistance and increased fatty acid flux drive VLDL-apoB secretion, statins increase rates of catabolism but do not appear to reduce VLDL secretion, even at high doses (79).

Statins also affect the metabolism of triglyceride-rich lipoproteins, presumably via LDL receptor-independent mechanisms. Atorvastatin reduces apoC-III concentrations (80), which may result in increased LPL activity, allowing more VLDL-apoB to be converted to LDL, thus minimizing the effect on LDL-apoB concentration. A similar mechanism has been proposed to account for the effect of statins on postprandial lipoprotein metabolism (81).

Peroxisome proliferator-activated receptor agonists, such as fibrates, primarily increase the catabolism of VLDL-, IDL-, and LDL-apoB, whereas they seem to have little effect on the hepatic secretion of lipoproteins (79), although earlier studies performed with exogenously radiolabeled lipoproteins indicated that fibrates increase the FCRs of VLDL and IDL but decrease LDL FCR in hypertriglyceridemia (82). This discrepancy may relate to different fibrates and to differences in patient groups. Because fibrates are agonists for a nuclear receptor and thus affect a master regulator, the observed effects on apoB metabolism may depend more on the underlying condition than in the statins. This may also explain why the effect of fibrates appears broader than the rather specific effect of statins on LDL concentration via the regulation of HMG-CoA reductase and hence the LDL receptor. In diabetic patients, fibrates result in a more pronounced shift in LDL subtype distribution compared with statins (83).

The dyslipidemia in diabetic patients is the result of both insulin resistance and hyperglycemia. Therefore, it is not surprising that the lipid profile during pioglitazone therapy is more favorable than during sulfonylurea treatment, despite achieving similar levels of glucose control (84). Because insulin resistance is characterized by an overproduction of VLDL₁, it could be expected that the beneficial effect of pioglitazone on lipids is primarily the result of decreased VLDL secretion. In a recent study, Nagashima and colleagues (85) evaluated the effect of pioglitazone on the kinetics of VLDL-, IDL-, and LDL-apoB as well as on VLDL-triglycerides. Surprisingly, they found that pioglitazone treatment reduced VLDL-triglyceride concentration primarily by increasing the lipolytic removal of VLDL-triglycerides without affecting VLDL-triglyceride and -apoB production. Conversion of VLDL to LDL was unaffected as well. It is unclear why weight reduction and pioglitazone therapy, both of which decrease insulin resistance, supposedly have such different effects on apoB metabolism. This is particularly disturbing because the effect on triglyceride concentration and LDL subtype distribution is similar.

There are no studies evaluating the effect of nicotinic acid or ezetimibe on apoB metabolism in the metabolic syndrome or type 2 diabetes, although both drugs were shown to have effects on lipid concentrations in such patients.

In a recently published study, the effect of the cholesteryl ester transfer protein inhibitor torcetrapib on apoB metabolism was evaluated (86). Although there is no evidence that the subjects studied were insulin-resistant, they exhibited characteristics of the metabolic syndrome (low HDL-cholesterol, high VLDL-apoB production). In this study, torcetrapib reduced VLDL-, IDL-, and LDL-apoB-100 levels primarily by increasing the rate of clearance. In contrast, when torcetrapib was added to atorvastatin, it enhanced the clearance of VLDL particles, whereas the effects on IDL- and LDL-apoB concentration were primarily mediated by reduced production (86).

	DYSBETALIPOPROTEINEMIA (TYPE III HYPERLIPIDEMIA)

TOP ABSTRACT INTRODUCTION NORMOLIPIDEMIC SUBJECTS FAMILIAL HYPERCHOLESTEROLEMIA... PATIENTS WITH THE METABOLIC... DYSBETALIPOPROTEINEMIA (TYPE III... HYPOBETALIPOPROTEINEMIA CONCLUSION REFERENCES

 
Dysbetalipoproteinemia, which is usually characterized by homozygosity of apoE2, is characterized by a delayed catabolism of apoB-100- and apoB-48-containing lipoproteins with little conversion to IDL and LDL (87). Turner and colleagues (88) showed that the production of IDL is increased in dysbetalipoproteinemia and that the time for conversion of IDL- to LDL-apoB is delayed 5-fold. More recent studies focusing on chylomicron metabolism have shown that dysbetalipoproteinemia is associated with delayed chylomicron metabolism (89, 90).

In the study by Turner et al. (88), gemfibrozil therapy reduced VLDL and IDL production in dysbetalipoproteinemia. A more recent study in patients with coexisting dysbetalipoproteinemia and heterozygous FH (91) demonstrated that VLDL and IDL FCRs were decreased, whereas LDL FCR was increased, compared with FH heterozygotes and normolipidemic control subjects. Furthermore, fenofibrate treatment increased VLDL and IDL FCRs but also increased LDL production.

	HYPOBETALIPOPROTEINEMIA

TOP ABSTRACT INTRODUCTION NORMOLIPIDEMIC SUBJECTS FAMILIAL HYPERCHOLESTEROLEMIA... PATIENTS WITH THE METABOLIC... DYSBETALIPOPROTEINEMIA (TYPE III... HYPOBETALIPOPROTEINEMIA CONCLUSION REFERENCES

 
Hypobetalipoproteinemia is characterized by low concentrations of LDL-cholesterol and apoB (92, 93). Familial hypobetalipoproteinemia is primarily caused by mutations in the apoB gene. Almost 60 different mutations have been described that interfere with the translation of the full-length apoB. Many of these mutations cause the production of truncated apoB. Hooper, van Bockxmeer, and Burnett (94) recently reviewed this field.

The metabolism of several truncated apoBs has been studied using stable isotope technique (Table 2 ). These studies have provided important information on the structure-function relationships of normal apoB. Both decreased production rates and increased clearance rates are responsible for the low plasma concentrations of apoB. Truncations that retain the LDL receptor binding domain, such as apoB-89, apoB-87, and apoB-75, have increased FCRs (95–97). On the other hand, truncated forms of apoB are also secreted at lower rates. VLDL-apoB secretion was reduced by 1.4% for each 1% of apoB truncated (98). Truncated apoBs smaller than apoB-30 are not detectable in plasma; thus, this appears to be the minimum length of apoB that is required for microsomal triglyceride transfer protein (MTP)-dependent lipoprotein assembly. In vitro data indicate that the lipid content of secreted apoB-containing lipoproteins is decreased as apoB is shortened (99).

Some forms of hypobetalipoproteinemia are not attributable to truncated forms of apoB. Latour and colleagues (101) performed a stable isotope study in such a kindred and observed 2- to 3-fold increases in VLDL- and LDL-apoB-100 FCRs. The underlying mechanisms are unclear and remain to be elucidated (93).

	CONCLUSION

TOP ABSTRACT INTRODUCTION NORMOLIPIDEMIC SUBJECTS FAMILIAL HYPERCHOLESTEROLEMIA... PATIENTS WITH THE METABOLIC... DYSBETALIPOPROTEINEMIA (TYPE III... HYPOBETALIPOPROTEINEMIA CONCLUSION REFERENCES

 
Human lipoprotein kinetics studies provide insight into the factors that control the secretion and catabolism of apoB-containing lipoproteins. Studies in hypolipoproteinemia and hyperlipoproteinemia have elucidated the processes that control VLDL secretion as well as VLDL and LDL catabolism. In hypobetalipoproteinemia attributable to a truncation in apoB, the rate of secretion is closely linked to the length of apoB. On the other hand, in patients with the metabolic syndrome, it appears that substrate, in the form of free fatty acids, coupled to the state of insulin resistance can induce the hypersecretion of VLDL-apoB. Studies in patients with FH, FDB, and PCSK9 mutations show that these mutations are the most important determinants in regulating LDL catabolism.

The overall importance of these studies relates to our need to understand the factors that link abnormalities of lipoprotein metabolism with an increased risk of atherosclerotic disease. Although apoB metabolism is a central component of lipoprotein metabolism, it is only one component. Therefore, apoB metabolism must be seen in context together with postprandial lipoprotein metabolism and reverse cholesterol transport. Although such interactions are of great interest and relevance, few kinetics data are available to date. Future studies should focus on the interaction between different pathways of lipoprotein metabolism and how lipoprotein metabolism is linked to protein and carbohydrate metabolism at the whole body level.

This review also demonstrates that metabolic studies may provide contradictory data even under similar or identical conditions. This further highlights the sensitivity of the methodology used for kinetics studies and underscores the need to design studies carefully and include appropriate controls.

	ACKNOWLEDGMENTS

 
This work was supported by grants from the National Health and Medical Research Council of Australia (NHMRC) and the National Institutes of Health (Grant NIBIB P41 EB-00195). P.H.R.B. is a senior research fellow of the NHMRC.

Manuscript received April 24, 2006 and in revised form May 22, 2006.

	REFERENCES

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1. Burnett, J. R., and P. H. Barrett. 2002. Apolipoprotein B metabolism: tracer kinetics, models, and metabolic studies. Crit. Rev. Clin. Lab. Sci. 39: 89–137.[Medline]

2. Barrett, P. H. R., and D. M. Foster. 1996. Design and analysis of lipid tracer kinetic studies. Curr. Opin. Lipidol. 7: 143–148.[Medline]

3. Parhofer, K. G., P. Hugh, R. Barrett, D. M. Bier, and G. Schonfeld. 1991. Determination of kinetic parameters of apolipoprotein B metabolism using amino acids labeled with stable isotopes. J. Lipid Res. 32: 1311–1323.[Abstract]

4. Patterson, B. W. 2002. Methods for measuring lipid metabolism in vivo. Curr. Opin. Clin. Nutr. Metab. Care. 5: 475–479.[CrossRef][Medline]

5. Packard, C. J., T. Demant, J. P. Stewart, D. Bedford, M. J. Caslake, G. Schwertfeger, A. Bedynek, J. Shepherd, and D. Seidel. 2000. Apolipoprotein B metabolism and the distribution of VLDL and LDL subfractions. J. Lipid Res. 41: 305–318.[Abstract/Free Full Text]

6. Ouguerram, K., M. Krempf, C. Maugeais, P. Maugere, D. Darmaun, and T. Magot. 2002. A new labeling approach using stable isotopes to study in vivo plasma cholesterol metabolism in humans. Metabolism. 51: 5–11.[Medline]

7. Chetiveaux, M., K. Ouguerram, Y. Zair, P. Maugere, I. Falconi, H. Nazih, and M. Krempf. 2004. New model for kinetic studies of HDL metabolism in humans. Eur. J. Clin. Invest. 34: 262–267.[CrossRef][Medline]

8. Bosner, M. S., L. G. Lange, W. F. Stenson, and R. E. Ostlund, Jr. 1999. Percent cholesterol absorption in normal women and men quantified with dual stable isotopic tracers and negative ion mass spectrometry. J. Lipid Res. 40: 302–308.[Abstract/Free Full Text]

9. Barrows, B. R., M. T. Timlin, and E. J. Parks. 2005. Spillover of dietary fatty acids and use of serum nonesterified fatty acids for the synthesis of VLDL-triacylglycerol under two different feeding regimens. Diabetes. 54: 2668–2673.[Abstract/Free Full Text]

10. Hellerstein, M. K. 2003. In vivo measurement of fluxes through metabolic pathways: the missing link in functional genomics and pharmaceutical research. Annu. Rev. Nutr. 23: 379–402.[CrossRef][Medline]

11. Adiels, M., C. Packard, M. J. Caslake, P. Stewart, A. Soro, J. Westerbacka, B. Wennberg, S. O. Olofsson, M. R. Taskinen, and J. Boren. 2005. A new combined multicompartmental model for apolipoprotein B-100 and triglyceride metabolism in VLDL subfractions. J. Lipid Res. 46: 58–67.[Abstract/Free Full Text]

12. Demant, T., C. J. Packard, H. Demmelmair, P. Stewart, A. Bedynek, D. Bedford, D. Seidel, and J. Shepherd. 1996. Sensitive methods to study human apolipoprotein B metabolism using stable isotope-labeled amino acids. Am. J. Physiol. 270: E1022–E1036.

13. Ginsberg, H. N., N. A. Le, and J. C. Gibson. 1985. Regulation of the production and catabolism of plasma low density lipoproteins in hypertriglyceridemic subjects. Effect of weight loss. J. Clin. Invest. 75: 614–623.[Medline]

14. Watts, G. F., P. Moroz, and P. H. Barrett. 2000. Kinetics of very-low-density lipoprotein apolipoprotein B-100 in normolipidemic subjects: pooled analysis of stable-isotope studies. Metabolism. 49: 1204–1210.[CrossRef][Medline]

15. Marsh, J. B., F. K. Welty, A. H. Lichtenstein, S. Lamon-Fava, and E. J. Schaefer. 2002. Apolipoprotein B metabolism in humans: studies with stable isotope-labeled amino acid precursors. Atherosclerosis. 162: 227–244.[CrossRef][Medline]

16. Walsh, B. W., I. Schiff, B. Rosner, L. Greenberg, V. Ravnikar, and F. M. Sacks. 1991. Effects of postmenopausal estrogen replacement on the concentrations and metabolism of plasma lipoproteins. N. Engl. J. Med. 325: 1196–1204.[Abstract]

17. Welty, F. K., A. H. Lichtenstein, P. H. Barrett, G. G. Dolnikowski, and E. J. Schaefer. 1999. Human apolipoprotein (apo) B-48 and apoB-100 kinetics with stable isotopes. Arterioscler. Thromb. Vasc. Biol. 19: 2966–2974.[Abstract/Free Full Text]

18. Stacpoole, P. W., K. von Bergmann, L. L. Kilgore, L. A. Zech, and W. R. Fisher. 1991. Nutritional regulation of cholesterol synthesis and apolipoprotein B kinetics: studies in patients with familial hypercholesterolemia and normal subjects treated with a high carbohydrate, low fat diet. J. Lipid Res. 32: 1837–1848.[Abstract]

19. Bordin, P., O. A. Bodamer, S. Venkatesan, R. M. Gray, P. A. Bannister, and D. Halliday. 1998. Effects of fish oil supplementation on apolipoprotein B100 production and lipoprotein metabolism in normolipidaemic males. Eur. J. Clin. Nutr. 52: 104–109.[CrossRef][Medline]

20. Nestel, P. J., W. E. Connor, M. F. Reardon, S. Connor, S. Wong, and R. Boston. 1984. Suppression by diets rich in fish oil of very low density lipoprotein production in man. J. Clin. Invest. 74: 82–89.[Medline]

21. Watts, G. F., R. P. Naoumova, J. M. Kelly, F. M. Riches, K. D. Croft, and G. R. Thompson. 1997. Inhibition of cholesterogenesis decreases hepatic secretion of apoB-100 in normolipidemic subjects. Am. J. Physiol. 273: E462–E470.

22. Malmendier, C. L., J. F. Lontie, C. Delcroix, and T. Magot. 1989. Effect of simvastatin on receptor-dependent low density lipoprotein catabolism in normocholesterolemic human volunteers. Atherosclerosis. 80: 101–109.[CrossRef][Medline]

23. Bilheimer, D. W., N. J. Stone, and S. M. Grundy. 1979. Metabolic studies in familial hypercholesterolemia. Evidence for a gene-dosage effect in vivo. J. Clin. Invest. 64: 524–533.[Medline]

24. Cummings, M. H., G. F. Watts, M. Umpleby, T. R. Hennessy, J. R. Quiney, and P. H. Sonksen. 1995. Increased hepatic secretion of very-low-density-lipoprotein apolipoprotein B-100 in heterozygous familial hypercholesterolaemia: a stable isotope study. Atherosclerosis. 113: 79–89.[CrossRef][Medline]

25. Tremblay, A. J., B. Lamarche, I. L. Ruel, J. C. Hogue, J. Bergeron, C. Gagne, and P. Couture. 2004. Increased production of VLDL apoB-100 in subjects with familial hypercholesterolemia carrying the same null LDL receptor gene mutation. J. Lipid Res. 45: 866–872.[Abstract/Free Full Text]

26. Fisher, W. R., L. A. Zech, L. L. Kilgore, and P. W. Stacpoole. 1991. Metabolic pathways of apolipoprotein B in heterozygous familial hypercholesterolemia: studies with a [³H]leucine tracer. J. Lipid Res. 32: 1823–1836.[Abstract]

27. Fisher, W. R., L. A. Zech, and P. W. Stacpoole. 1994. ApoB metabolism in familial hypercholesterolemia. Inconsistencies with the LDL receptor paradigm. Arterioscler. Thromb. 14: 501–510.[Abstract/Free Full Text]

28. Gent, J., and I. Braakman. 2004. Low-density lipoprotein receptor structure and folding. Cell. Mol. Life Sci. 61: 2461–2470.[CrossRef][Medline]

29. Millar, J. S., C. Maugeais, K. Ikewaki, D. M. Kolansky, P. H. Barrett, E. C. Budreck, R. C. Boston, N. Tada, S. Mochizuki, J. C. Defesche, et al. 2005. Complete deficiency of the low-density lipoprotein receptor is associated with increased apolipoprotein B-100 production. Arterioscler. Thromb. Vasc. Biol. 25: 560–565.[Abstract/Free Full Text]

30. Zulewski, H., R. Ninnis, A. R. Miserez, M. W. Baumstark, and U. Keller. 1998. VLDL and IDL apolipoprotein B-100 kinetics in familial hypercholesterolemia due to impaired LDL receptor function or to defective apolipoprotein B-100. J. Lipid Res. 39: 380–387.[Abstract/Free Full Text]

31. Gaffney, D., L. Forster, M. J. Caslake, D. Bedford, J. P. Stewart, G. Stewart, G. Wieringa, M. Dominiczak, J. P. Miller, and C. J. Packard. 2002. Comparison of apolipoprotein B metabolism in familial defective apolipoprotein B and heterogeneous familial hypercholesterolemia. Atherosclerosis. 162: 33–43.[CrossRef][Medline]

32. Pietzsch, J., B. Wiedemann, U. Julius, S. Nitzsche, S. Gehrisch, S. Bergmann, W. Leonhardt, W. Jaross, and M. Hanefeld. 1996. Increased clearance of low density lipoprotein precursors in patients with heterozygous familial defective apolipoprotein B-100: a stable isotope approach. J. Lipid Res. 37: 2074–2087.[Abstract]

33. Schaefer, J. R., H. Scharnagl, M. W. Baumstark, H. Schweer, L. A. Zech, H. Seyberth, K. Winkler, A. Steinmetz, and W. Marz. 1997. Homozygous familial defective apolipoprotein B-100. Enhanced removal of apolipoprotein E-containing VLDLs and decreased production of LDLs. Arterioscler. Thromb. Vasc. Biol. 17: 348–353.[Abstract/Free Full Text]

34. Maxwell, K. N., and J. L. Breslow. 2004. Adenoviral-mediated expression of Pcsk9 in mice results in a low-density lipoprotein receptor knockout phenotype. Proc. Natl. Acad. Sci. USA. 101: 7100–7105.[Abstract/Free Full Text]

35. Park, S. W., Y. A. Moon, and J. D. Horton. 2004. Post-transcriptional regulation of low density lipoprotein receptor protein by proprotein convertase subtilisin/kexin type 9a in mouse liver. J. Biol. Chem. 279: 50630–50638.[Abstract/Free Full Text]

36. Lalanne, F., G. Lambert, M. J. Amar, M. Chetiveaux, Y. Zair, A. L. Jarnoux, K. Ouguerram, J. Friburg, N. G. Seidah, H. B. Brewer, Jr., et al. 2005. Wild-type PCSK9 inhibits LDL clearance but does not affect apoB-containing lipoprotein production in mouse and cultured cells. J. Lipid Res. 46: 1312–1319.[Abstract/Free Full Text]

37. Benjannet, S., D. Rhainds, R. Essalmani, J. Mayne, L. Wickham, W. Jin, M. C. Asselin, J. Hamelin, M. Varret, D. Allard, et al. 2004. NARC-1/PCSK9 and its natural mutants: zymogen cleavage and effects on the low density lipoprotein (LDL) receptor and LDL cholesterol. J. Biol. Chem. 279: 48865–48875.[Abstract/Free Full Text]

38. Ouguerram, K., M. Chetiveaux, Y. Zair, P. Costet, M. Abifadel, M. Varret, C. Boileau, T. Magot, and M. Krempf. 2004. Apolipoprotein B100 metabolism in autosomal-dominant hypercholesterolemia related to mutations in PCSK9. Arterioscler. Thromb. Vasc. Biol. 24: 1448–1453.[Abstract/Free Full Text]

39. Twisk, J., D. L. Gillian-Daniel, A. Tebon, L. Wang, P. H. Barrett, and A. D. Attie. 2000. The role of the LDL receptor in apolipoprotein B secretion. J. Clin. Invest. 105: 521–532.[Medline]

40. Cohen, J., A. Pertsemlidis, I. K. Kotowski, R. Graham, C. K. Garcia, and H. H. Hobbs. 2005. Low LDL cholesterol in individuals of African descent resulting from frequent nonsense mutations in PCSK9. Nat. Genet. 37: 161–165.[CrossRef][Medline]

41. Cohen, J. C., E. Boerwinkle, T. H. Mosley, Jr., and H. H. Hobbs. 2006. Sequence variations in PCSK9, low LDL, and protection against coronary heart disease. N. Engl. J. Med. 354: 1264–1272.[Abstract/Free Full Text]

42. Bilheimer, D. W., S. M. Grundy, M. S. Brown, and J. L. Goldstein. 1983. Mevinolin and colestipol stimulate receptor-mediated clearance of low density lipoprotein from plasma in familial hypercholesterolemia heterozygotes. Proc. Natl. Acad. Sci. USA. 80: 4124–4128.[Abstract/Free Full Text]

43. Grundy, S. M., G. L. Vega, and D. W. Bilheimer. 1985. Influence of combined therapy with mevinolin and interruption of bile-acid reabsorption on low density lipoproteins in heterozygous familial hypercholesterolemia. Ann. Intern. Med. 103: 339–343.[Abstract/Free Full Text]

44. Uauy, R., G. L. Vega, S. M. Grundy, and D. M. Bilheimer. 1988. Lovastatin therapy in receptor-negative homozygous familial hypercholesterolemia: lack of effect on low-density lipoprotein concentrations or turnover. J. Pediatr. 113: 387–392.[CrossRef][Medline]

45. Watts, G. F., M. H. Cummings, M. Umpleby, J. R. Quiney, R. Naoumova, G. R. Thompson, and P. H. Sonksen. 1995. Simvastatin decreases the hepatic secretion of very-low-density lipoprotein apolipoprotein B-100 in heterozygous familial hypercholesterolaemia: pathophysiological and therapeutic implications. Eur. J. Clin. Invest. 25: 559–567.[Medline]

46. Parhofer, K. G., P. H. Barrett, J. Dunn, and G. Schonfeld. 1993. Effect of pravastatin on metabolic parameters of apolipoprotein B in patients with mixed hyperlipoproteinemia. Clin. Investig. 71: 939–946.[Medline]

47. Winkler, K., J. R. Schafer, B. Klima, C. Nuber, A. Sattler, I. Friedrich, W. Koster, A. Steinmetz, H. Wieland, and W. Marz. 1999. Lifibrol enhances the low density lipoprotein apolipoprotein B-100 turnover in patients with hypercholesterolemia and mixed hyperlipidemia. Atherosclerosis. 144: 167–175.[CrossRef][Medline]

48. Parhofer, K. G., P. H. Barrett, T. Demant, W. O. Richter, and P. Schwandt. 1996. Effects of weekly LDL-apheresis on metabolic parameters of apolipoprotein B in heterozygous familial hypercholesterolemia. J. Lipid Res. 37: 2383–2393.[Abstract]

49. Parhofer, K. G., P. H. Barrett, T. Demant, and P. Schwandt. 2000. Acute effects of low density lipoprotein apheresis on metabolic parameters of apolipoprotein B. J. Lipid Res. 41: 1596–1603.[Abstract/Free Full Text]

50. Geiss, H. C., S. Bremer, P. H. Barrett, C. Otto, and K. G. Parhofer. 2004. In vivo metabolism of LDL subfractions in patients with heterozygous FH on statin therapy: rebound analysis of LDL subfractions after LDL apheresis. J. Lipid Res. 45: 1459–1467.[Abstract/Free Full Text]

51. Barrett, P. H., and K. G. Parhofer. 1998. Low-density lipoprotein-apolipoprotein B metabolism following apheresis: simulation studies of mass changes and tracer kinetics. Metabolism. 47: 478–483.[CrossRef][Medline]

51. Barrett, P. H. R., D. C. Chan, and G. F. Watts. 2006. Design and analysis of lipoprotein tracer kinetics studies in humans. J. Lipid Res. 47: 1607–1619.[Abstract/Free Full Text]

52. Chan, D. C., P. H. Barrett, and G. F. Watts. 2006. Recent studies of lipoprotein kinetics in the metabolic syndrome and related disorders. Curr. Opin. Lipidol. 17: 28–36.[Medline]

53. Cummings, M. H., G. F. Watts, A. M. Umpleby, T. R. Hennessy, R. Naoumova, B. M. Slavin, G. R. Thompson, and P. H. Sonksen. 1995. Increased hepatic secretion of very-low-density lipoprotein apolipoprotein B-100 in NIDDM. Diabetologia. 38: 959–967.[Medline]

54. Adiels, M., J. Boren, M. J. Caslake, P. Stewart, A. Soro, J. Westerbacka, B. Wennberg, S. O. Olofsson, C. Packard, and M. R. Taskinen. 2005. Overproduction of VLDL1 driven by hyperglycemia is a dominant feature of diabetic dyslipidemia. Arterioscler. Thromb. Vasc. Biol. 25: 1697–1703.[Abstract/Free Full Text]

55. Dane-Stewart, C. A., G. F. Watts, P. H. Barrett, B. G. Stuckey, J. C. Mamo, I. J. Martins, and T. G. Redgrave. 2003. Chylomicron remnant metabolism studied with a new breath test in postmenopausal women with and without type 2 diabetes mellitus. Clin. Endocrinol. (Oxf.). 58: 415–420.[CrossRef][Medline]

56. Riches, F. M., G. F. Watts, R. P. Naoumova, J. M. Kelly, K. D. Croft, and G. R. Thompson. 1998. Hepatic secretion of very-low-density lipoprotein apolipoprotein B-100 studied with a stable isotope technique in men with visceral obesity. Int. J. Obes. Relat. Metab. Disord. 22: 414–423.[CrossRef][Medline]

57. Watts, G. F., D. C. Chan, P. H. Barrett, A. V. Susekov, J. Hua, and S. Song. 2003. Fat compartments and apolipoprotein B-100 kinetics in overweight-obese men. Obes. Res. 11: 152–159.[Medline]

58. Adiels, M., M. R. Taskinen, C. Packard, M. J. Caslake, A. Soro-Paavonen, J. Westerbacka, S. Vehkavaara, A. Hakkinen, S. O. Olofsson, H. Yki-Jarvinen, et al. 2006. Overproduction of large VLDL particles is driven by increased liver fat content in man. Diabetologia. 49: 755–765.[CrossRef][Medline]

59. Ginsberg, H. N., and L. S. Huang. 2000. The insulin resistance syndrome: impact on lipoprotein metabolism and atherothrombosis. J. Cardiovasc. Risk. 7: 325–331.[Medline]

60. Ng, T. W., G. F. Watts, M. S. Farvid, D. C. Chan, and P. H. Barrett. 2005. Adipocytokines and VLDL metabolism: independent regulatory effects of adiponectin, insulin resistance, and fat compartments on VLDL apolipoprotein B-100 kinetics? Diabetes. 54: 795–802.[Abstract/Free Full Text]

61. Kabir, M., K. J. Catalano, S. Ananthnarayan, S. P. Kim, G. W. Van Citters, M. K. Dea, and R. N. Bergman. 2005. Molecular evidence supporting the portal theory: a causative link between visceral adiposity and hepatic insulin resistance. Am. J. Physiol. Endocrinol. Metab. 288: E454–E461.[Abstract/Free Full Text]

62. Lehrke, M., and M. A. Lazar. 2005. The many faces of PPARgamma. Cell. 123: 993–999.[CrossRef][Medline]

63. Tataranni, P. A., and E. Ortega. 2005. A burning question: does an adipokine-induced activation of the immune system mediate the effect of overnutrition on type 2 diabetes? Diabetes. 54: 917–927.[Abstract/Free Full Text]

64. Gill, J. M., J. C. Brown, D. Bedford, D. M. Wright, J. Cooney, D. A. Hughes, C. J. Packard, and M. J. Caslake. 2004. Hepatic production of VLDL1 but not VLDL2 is related to insulin resistance in normoglycaemic middle-aged subjects. Atherosclerosis. 176: 49–56.[CrossRef][Medline]

65. Lamarche, B., S. Rashid, and G. F. Lewis. 1999. HDL metabolism in hypertriglyceridemic states: an overview. Clin. Chim. Acta. 286: 145–161.[CrossRef][Medline]

66. Barrett, P. H., and G. F. Watts. 2003. Kinetic studies of lipoprotein metabolism in the metabolic syndrome including effects of nutritional interventions. Curr. Opin. Lipidol. 14: 61–68.[CrossRef][Medline]

67. Riches, F. M., G. F. Watts, J. Hua, G. R. Stewart, R. P. Naoumova, and P. H. Barrett. 1999. Reduction in visceral adipose tissue is associated with improvement in apolipoprotein B-100 metabolism in obese men. J. Clin. Endocrinol. Metab. 84: 2854–2861.[Abstract/Free Full Text]

68. Mittendorfer, B., B. W. Patterson, and S. Klein. 2003. Effect of weight loss on VLDL-triglyceride and apoB-100 kinetics in women with abdominal obesity. Am. J. Physiol. Endocrinol. Metab. 284: E549–E556.[Abstract/Free Full Text]

69. Chan, D. C., G. F. Watts, P. H. Barrett, L. J. Beilin, T. G. Redgrave, and T. A. Mori. 2002. Regulatory effects of HMG CoA reductase inhibitor and fish oils on apolipoprotein B-100 kinetics in insulin-resistant obese male subjects with dyslipidemia. Diabetes. 51: 2377–2386.[Abstract/Free Full Text]

70. Gylling, H., and T. A. Miettinen. 1996. Effects of inhibiting cholesterol absorption and synthesis on cholesterol and lipoprotein metabolism in hypercholesterolemic non-insulin-dependent diabetic men. J. Lipid Res. 37: 1776–1785.[Abstract]

71. Chan, D. C., G. F. Watts, P. H. Barrett, T. A. Mori, L. J. Beilin, and T. G. Redgrave. 2002. Mechanism of action of a 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitor on apolipoprotein B-100 kinetics in visceral obesity. J. Clin. Endocrinol. Metab. 87: 2283–2289.[Abstract/Free Full Text]

72. Bilz, S., S. Wagner, M. Schmitz, A. Bedynek, U. Keller, and T. Demant. 2004. Effects of atorvastatin versus fenofibrate on apoB-100 and apoA-I kinetics in mixed hyperlipidemia. J. Lipid Res. 45: 174–185.[Abstract/Free Full Text]

73. Forster, L. F., G. Stewart, D. Bedford, J. P. Stewart, E. Rogers, J. Shepherd, C. J. Packard, and M. J. Caslake. 2002. Influence of atorvastatin and simvastatin on apolipoprotein B metabolism in moderate combined hyperlipidemic subjects with low VLDL and LDL fractional clearance rates. Atherosclerosis. 164: 129–145.[CrossRef][Medline]

74. Ouguerram, K., T. Magot, Y. Zair, J. S. Marchini, B. Charbonnel, H. Laouenan, and M. Krempf. 2003. Effect of atorvastatin on apolipoprotein B100 containing lipoprotein metabolism in type-2 diabetes. J. Pharmacol. Exp. Ther. 306: 332–337.[Abstract/Free Full Text]

75. Arad, Y., R. Ramakrishnan, and H. N. Ginsberg. 1990. Lovastatin therapy reduces low density lipoprotein apoB levels in subjects with combined hyperlipidemia by reducing the production of apoB-containing lipoproteins: implications for the pathophysiology of apoB production. J. Lipid Res. 31: 567–582.[Abstract]

76. Myerson, M., C. Ngai, J. Jones, S. Holleran, R. Ramakrishnan, L. Berglund, and H. N. Ginsberg. 2005. Treatment with high-dose simvastatin reduces secretion of apolipoprotein B-lipoproteins in patients with diabetic dyslipidemia. J. Lipid Res. 46: 2735–2744.[Abstract/Free Full Text]

77. Isley, W. L., J. M. Miles, B. W. Patterson, and W. S. Harris. 2006. The effect of high-dose simvastatin on triglyceride-rich lipoprotein metabolism in patients with type 2 diabetes mellitus. J. Lipid Res. 47: 193–200.[Abstract/Free Full Text]

78. Ginsberg, H. N. 2006. Review. Efficacy and mechanisms of action of statins in the treatment of diabetic dyslipidemia. J. Clin. Endocrinol. Metab. 91: 383–392.[Abstract/Free Full Text]

79. Watts, G. F., P. H. Barrett, J. Ji, A. P. Serone, D. C. Chan, K. D. Croft, F. Loehrer, and A. G. Johnson. 2003. Differential regulation of lipoprotein kinetics by atorvastatin and fenofibrate in subjects with the metabolic syndrome. Diabetes. 52: 803–811.[Abstract/Free Full Text]

80. Chan, D. C., G. F. Watts, T. A. Mori, P. H. Barrett, L. J. Beilin, and T. G. Redgrave. 2002. Factorial study of the effects of atorvastatin and fish oil on dyslipidaemia in visceral obesity. Eur. J. Clin. Invest. 32: 429–436.[CrossRef][Medline]

81. Parhofer, K. G., P. H. Barrett, and P. Schwandt. 2000. Atorvastatin improves postprandial lipoprotein metabolism in normolipidemlic subjects. J. Clin. Endocrinol. Metab. 85: 4224–4230.[Abstract/Free Full Text]

82. Ginsberg, H. N. 1987. Changes in lipoprotein kinetics during therapy with fenofibrate and other fibric acid derivatives. Am. J. Med. 83: 66–70.[Medline]

83. Frost, R. J., C. Otto, H. C. Geiss, P. Schwandt, and K. G. Parhofer. 2001. Effects of atorvastatin versus fenofibrate on lipoprotein profiles, low-density lipoprotein subfraction distribution, and hemorheologic parameters in type 2 diabetes mellitus with mixed hyperlipoproteinemia. Am. J. Cardiol. 87: 44–48.[Medline]

84. Parhofer, K. G., C. Otto, H. C. Geiss, E. Laubach, and B. Goke. 2005. Effect of pioglitazone on lipids in well controlled patients with diabetes mellitus type 2—results of a pilot study. Exp. Clin. Endocrinol. Diabetes. 113: 49–52.[CrossRef][Medline]

85. Nagashima, K., C. Lopez, D. Donovan, C. Ngai, N. Fontanez, A. Bensadoun, J. Fruchart-Najib, S. Holleran, J. S. Cohn, R. Ramakrishnan, et al. 2005. Effects of the PPARgamma agonist pioglitazone on lipoprotein metabolism in patients with type 2 diabetes mellitus. J. Clin. Invest. 115: 1323–1332.[CrossRef][Medline]

86. Millar, J. S., M. E. Brousseau, M. R. Diffenderfer, P. H. Barrett, F. K. Welty, A. Faruqi, M. L. Wolfe, C. Nartsupha, A. G. Digenio, J. P. Mancuso, et al. 2006. Effects of the cholesteryl ester transfer protein inhibitor torcetrapib on apolipoprotein B100 metabolism in humans. Arterioscler. Thromb. Vasc. Biol. 26: 1350–1356.[Abstract/Free Full Text]

87. Stalenhoef, A. F., M. J. Malloy, J. P. Kane, and R. J. Havel. 1986. Metabolism of apolipoproteins B-48 and B-100 of triglyceride-rich lipoproteins in patients with familial dysbetalipoproteinemia. J. Clin. Invest. 78: 722–728.[Medline]

88. Turner, P. R., C. Cortese, R. Wootton, C. Marenah, N. E. Miller, and B. Lewis. 1985. Plasma apolipoprotein B metabolism in familial type III dysbetalipoproteinaemia. Eur. J. Clin. Invest. 15: 100–112.[Medline]

89. Haffner, S. M., R. S. Kushwaha, and W. R. Hazzard. 1989. Metabolism of chylomicrons in subjects with dysbetalipoproteinaemia (type III hyperlipoproteinaemia). Eur. J. Clin. Invest. 19: 486–490.[Medline]

90. Redgrave, T. G., G. F. Watts, I. J. Martins, P. H. Barrett, J. C. Mamo, S. B. Dimmitt, and A. D. Marais. 2001. Chylomicron remnant metabolism in familial dyslipidemias studied with a remnant-like emulsion breath test. J. Lipid Res. 42: 710–715.[Abstract/Free Full Text]

91. Tremblay, A. J., B. Lamarche, I. L. Ruel, J. C. Hogue, Y. Deshaies, C. Gagne, and P. Couture. Effects of fenofibrate on apolipoprotein kinetics in patients with coexisting dysbetalipoproteinemia and heterozygous familial hypercholesterolemia. Atherosclerosis. Epub ahead of print. December 5, 2005; doi:10.1016/j.atherosclerosis.2005.10.037.

92. Schonfeld, G. 2003. Familial hypobetalipoproteinemia: a review. J. Lipid Res. 44: 878–883.[Abstract/Free Full Text]

93. Schonfeld, G., X. Lin, and P. Yue. 2005. Familial hypobetalipoproteinemia: genetics and metabolism. Cell. Mol. Life Sci. 62: 1372–1378.[CrossRef][Medline]

94. Hooper, A. J., F. M. van Bockxmeer, and J. R. Burnett. 2005. Monogenic hypocholesterolaemic lipid disorders and apolipoprotein B metabolism. Crit. Rev. Clin. Lab. Sci. 42: 515–545.[CrossRef][Medline]

95. Parhofer, K. G., P. H. Barrett, D. M. Bier, and G. Schonfeld. 1992. Lipoproteins containing the truncated apolipoprotein, apo B-89, are cleared from human plasma more rapidly than apo B-100-containing lipoproteins in vivo. J. Clin. Invest. 89: 1931–1937.[Medline]

96. Gabelli, C., C. Bilato, S. Martini, G. E. Tennyson, L. A. Zech, A. Corsini, M. Albanese, H. B. Brewer, Jr., G. Crepaldi, and G. Baggio. 1996. Homozygous familial hypobetalipoproteinemia. Increased LDL catabolism in hypobetalipoproteinemia due to a truncated apolipoprotein B species, apo B-87Padova. Arterioscler. Thromb. Vasc. Biol. 16: 1189–1196.[Abstract/Free Full Text]

97. Krul, E. S., K. G. Parhofer, P. H. Barrett, R. D. Wagner, and G. Schonfeld. 1992. ApoB-75, a truncation of apolipoprotein B associated with familial hypobetalipoproteinemia: genetic and kinetic studies. J. Lipid Res. 33: 1037–1050.[Abstract]

98. Parhofer, K. G., P. H. Barrett, C. A. Aguilar-Salinas, and G. Schonfeld. 1996. Positive linear correlation between the length of truncated apolipoprotein B and its secretion rate: in vivo studies in human apoB-89, apoB-75, apoB-54.8, and apoB-31 heterozygotes. J. Lipid Res. 37: 844–852.[Abstract]

99. Yao, Z., and R. S. McLeod. 1994. Synthesis and secretion of hepatic apolipoprotein B-containing lipoproteins. Biochim. Biophys. Acta. 1212: 152–166.[Medline]

100. Aguilar-Salinas, C. A., P. H. Barrett, K. G. Parhofer, S. G. Young, D. Tessereau, J. Bateman, C. Quinn, and G. Schonfeld. 1995. Apoprotein B-100 production is decreased in subjects heterozygous for truncations of apoprotein B. Arterioscler. Thromb. Vasc. Biol. 15: 71–80.[Abstract/Free Full Text]

101. Latour, M. A., B. W. Patterson, J. Pulai, Z. Chen, and G. Schonfeld. 1997. Metabolism of apolipoprotein B-100 in a kindred with familial hypobetalipoproteinemia without a truncated form of apoB. J. Lipid Res. 38: 592–599.[Abstract]

102. Chan, D. C., G. F. Watts, T. G. Redgrave, T. A. Mori, and P. H. Barrett. 2002. Apolipoprotein B-100 kinetics in visceral obesity: associations with plasma apolipoprotein C-III concentration. Metabolism. 51: 1041–1046.[CrossRef][Medline]

103. Hardman, D. A., C. R. Pullinger, R. L. Hamilton, J. P. Kane, and M. J. Malloy. 1991. Molecular and metabolic basis for the metabolic disorder normotriglyceridemic abetalipoproteinemia. J. Clin. Invest. 88: 1722–1729.[Medline]

104. Welty, F. K., A. H. Lichtenstein, P. H. Barrett, G. G. Dolnikowski, J. M. Ordovas, and E. J. Schaefer. 1997. Production of apolipoprotein B-67 in apolipoprotein B-67/B-100 heterozygotes: technical problems associated with leucine contamination in stable isotope studies. J. Lipid Res. 38: 1535–1543.[Abstract]

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