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The Effect of Fasting on Hepatic Lipid Accumulation and Transcriptional Regulation of Lipid Metabolism Differs between C57BL/6J and BALB/cA Mice Fed a High-fat Diet

Department of Veterinary Pathology, Graduate School of Agricultural and Life Sciences, The University of Tokyo, Tokyo, Japan

Correspondence: Koji Uetsuka, Nippon Institute for Biological Science, 9-2221-1, Shin-Machi, Ome, Tokyo 198-0024, Japan; e-mail:koji_ue{at}nibs.or.jp.

	Abstract

TOP Abstract Introduction Materials and Methods Results Discussion References

 
The effects of fasting on hepatic lipid metabolism in mice fed a high-fat diet (HFD) are still unclear. After fasting, the degree of hepatic lipid accumulation differs between HFD-fed C57BL/6J (B6) and BALB/cA (BALB/c) mice. It is not clear whether this difference is due to sensitivity to fasting or HFD. The aim of this study is to elucidate this difference among strains. After nine weeks of HFD feeding, both B6 and BALB/c mice showed moderate hepatic steatosis. However, after a subsequent twenty-hour fast, the hepatic lipid accumulation was markedly decreased in B6 but not in BALB/c mice. Moreover, the mRNA expression of a transcription factor, Srebp1(regulates hepatic lipid metabolism), and its target genes—malic enzyme, acetyl-CoA carboxylase, fatty acid synthase(regulate fatty acid synthesis), and glycerol-3-phosphate acyltransferase(regulates triacylglycerol synthesis)—were more markedly reduced in B6 than BALB/c mice. In conclusion, fasting may modify hepatic lipid accumulation in HFD-fed B6 and BALB/c mice differently. The difference may be partly owing to a marked downregulation of the expression of some lipid-metabolism–related genes in B6 mice. These results suggest that fasting per se has a significant effect on hepatic lipid accumulation in mouse strains. SREBP1 might play a role in this fasting effect.

Key Words: fasting • fatty liver • mice • inbred strain • lipid metabolism

Abbreviations: ACSs, acyl-coA synthetases • BALB/c, BALB/cA • B6, C57BL/6J • GAPDH, glyceraldehyde-3-phosphate dehydrogenase • HE, hematoxylin and eosin • HFD, high-fat diet • SD, standard deviation • Srebp1, sterol regulatory element binding protein 1 • TAG, triacylglycerol • VLDL, very-low density lipoprotein

	Introduction

TOP Abstract Introduction Materials and Methods Results Discussion References

 
Hepatic lipid metabolism is influenced by the balance between the degradation and synthesis and/or import and export of triacylglycerol (TAG) and fatty acids. Liver incorporates plasma glucose and fatty acids. Glucose is degraded by the glycolytic system, and the acetyl CoA produced by this system is used for fatty acid synthesis. Fatty acids are degraded through β-oxidation, or esterified and then stored as TAG. TAG is degraded into fatty acids and glycerol in the liver, or directly exported to the extrahepatic circulation as very-low–density lipoprotein (VLDL) (Bender and Mayes 2006).

A high-fat diet (HFD) may induce hepatic TAG accumulation, owing to the import of excess amounts of fatty acids into the liver. The excess fatty acids are then esterified and stored as TAG. A methionine- or choline-deficient diet also induces hepatic TAG accumulation, which further induces a reduction in the synthesis of VLDL, and finally results in hepatic steatosis (Kirsch et al. 2003; Lombardi et al. 1968; Powell et al. 2005) with an accumulation of hepatic TAG.

Both satiety and fasting are thought to change the balance of hepatic lipid metabolism. In a satiated state, the concentrations of circulating glucose and insulin are high, and the hepatic import of plasma glucose and synthesis of fatty acids are increased. Then, hepatic TAG is increased. Moreover, β-oxidation of fatty acid is inhibited. As a result, a lipogenic metabolic state occurs in the liver. On the other hand, in a fasted state, the concentrations of circulating glucose and insulin are low, which stimulates the degradation of TAG into fatty acids in adipose tissue. Then, plasma fatty acid levels are increased and they are incorporated into the liver. In the liver, fatty acids are degraded through β-oxidation, and ketone bodies are synthesized to complement energy shortages. Finally, TAG synthesis is inhibited in the liver. The metabolic state of the liver condition is lipolytic (Botham and Mayes 2006). However, in cases in which the quantity of fatty acid taken up exceeds the hepatic lipolytic capability, excess fatty acids are stored in the liver as TAG. Actually, hepatic TAG increases with fasting in mice (Lin et al. 2005).

We previously showed that HFD-induced hepatic lipid accumulation is mild in C57BL/6J (B6) mice but still moderate in BALB/cA (BALB/c) mice after a twenty-hour fast (Nishikawa et al. 2007). This result is inconsistent with a report that B6 mice fed a HFD suffered from moderate hepatic steatosis (West et al. 1992). Therefore, the hepatic lipid accumulation in HFD-fed mice would be influenced not only by fasting but also by mouse strain. In many studies of obesity, modifications of liver steatosis in HFD-fed mice during fasting have not been fully considered, and the differences of lipid metabolism with fasting among strains have not yet been taken into full account. Therefore, in the present study, we investigate the effect of fasting on HFD-induced hepatic lipid accumulation in B6 and BALB/c mice.

	Materials and Methods

TOP Abstract Introduction Materials and Methods Results Discussion References

 
Animals
Four-week-old male C57BL/6J Jcl (B6) mice and BALB/cA Jcl (BALB/c) mice were used. The animals, purchased from CLEA Japan (Tokyo, Japan), were housed individually in plastic mouse cages and maintained under a 14:10-hour light:dark cycle. They were fed a standard rodent chow (CE-2, CLEA Japan, Tokyo, Japan) and water ad libitum for one week. Then, the mice were fed a HFD (High Fat Diet 32, CLEA Japan, Tokyo, Japan) for nine weeks. The composition of each of the two diets is shown in Table 1. One half of the mice of each strain were fasted for twenty hours in the ninth week of the experiment (fasted groups). The other half were not fasted (nonfasted groups). Before and after the fasting, the mice were weighed. After the fasting, blood was collected from the tail vein for measuring the plasma glucose concentration. All mice were exsanguinated from the caudal vena cava under ether anesthesia, and the liver and abdominal and subcutaneous fat tissues were collected and weighed. The ratio of fat to body weight was obtained by dividing abdominal and subcutaneous fat tissues weight by body weight. The left lateral lobe of the liver was fixed in 10% neutral buffered formalin for histopathology. The right and caudate lobes were stored at –80°C until used for the examination of gene expression. All procedures involving mice were conducted according to the guidelines for the care and use of laboratory animals approved by the Graduate School of Agricultural and Life Sciences of Tokyo University.

Blood Biochemistry
Serum samples were prepared by centrifugation of total blood at 600 to 1400 x g for ten minutes. Using commercial kits, serum cholesterol, serum triacylglycerol, serum free fatty acid, and serum insulin levels (Cholesterol E-test Wako, Triglyceride E-test Wako, NEFA C-test Wako, Wako, Osaka, Japan and Mouse Insulin ELISA, Mercodia, Uppsala, Sweden, respectively) were measured according to the manufacturer’s instructions.

Histopathological Examination
The left lateral lobe of the liver was embedded in paraffin and 4-µm–thick paraffin sections were stained with hematoxylin and eosin (HE).

Semiquantitative RT-PCR
Total RNA was extracted from the liver tissue using an ISO-GEN kit (Nippon Gene Co. Ltd., Tokyo, Japan). Briefly, the liver tissue was lysed in ISOGEN solution on ice, and a water-soluble layer was obtained after centrifugation, followed by phenol-chloroform extraction and ethanol precipitation. For the first strand cDNA synthesis, a reverse transcriptase reaction was carried out using 5 µg of total RNA, the oligo (dT) primer, and the SUPERSCRIPT Preamplification System (Invitrogen, Carlsbad, CA, USA).

RT-PCR was performed with pairs of oligonucleotide primers corresponding to the cDNA sequence of the mouse mRNA (Table 2). PCR was carried out with 1 or 2 µl of RT product in a 50-µl reaction mixture containing 50 pM of the sense and antisense primers, 1.25 U of rTaq, 10xPCR buffer, and dNTP mixture (Takara, Siga, Japan). This procedure was immediately followed by preheating at 94°C for two minutes, denaturation at 94°C for thirty seconds, annealing at the melting temperature (Table 2) for thirty seconds, and extension at 72°C for one minute using a thermal cycler (TP-400, Takara, Siga, Japan). PCR products were identified by electrophoresis on 2% agarose gels, followed by ethidium bromide staining. Fluorescent gel imaging was carried out using the ultraviolet-CCD video system Fas-III (Toyobo, Osaka, Japan). The band density was digitized and normalized by using glyceraldehyde-3-phosphate dehydrogenase (GAPDH) expression as a reference.

	Results

TOP Abstract Introduction Materials and Methods Results Discussion References

 
Histopathological Examination of the Liver
The severity of hepatic lipid accumulation after nine weeks on the HFD was moderate in nonfasting, but mild in fasting B6 mice (Figure 1). By contrast, it was moderate in BALB/c mice of both the fasted and nonfasted groups.

View larger version (697K): [in this window] [in a new window]   Figure 1 Histopathological findings of the liver at 9 WAF. A: fasted B6 mouse, B: nonfasted B6 mouse, C: fasted BALB/c mouse, D: nonfasted BALB/c mouse. The severity of lipid accumulation changed to mild in B6 mice with fasting. Scale bar =200 µm. H & E.

View larger version (25K): [in this window] [in a new window]   Figure 2 Pathway of lipid metabolism and function of each enzyme in the liver. Squares with dotted lines represent enzymes. Solid blue arrows show results of mRNA expression in fasted B6 mice. Dashed blue arrows show the hypothesis about the behavior of the compounds in fasted B6 mice.

Ppar

Ppar

Ppar

Ppar,

View larger version (35K): [in this window] [in a new window]   Figure 3 Semiquantitative RT-PCR analyses of mRNA levels in the liver at 9 WAF. (A) Srebp1, (B) Ppar,(C) Ppar, (D) Foxa2, (E) Gpam, (F) Lipc, (G) Mttp, (H) Lipe, (I) Cd36, (J) Acads, (K) Cpt1a, (L) Acaca, (M) malic enzyme, (N) FASN, (O) Acsl1, (P) Acsl3, and (Q) Acsl5. White and black bars represent the fasted and nonfasted groups, respectively. Gene expression values are expressed as band density relative to GAPDH. Values represent the average ± SD from four or five mice. Significant differences are indicated by * and ** (fasted vs. nonfasted) at p<.05 and p<.01, respectively.

Acyl-coA synthetases (ACSs) are needed for both anabolic and catabolic reactions. The expression of Acsl1significantly increased in fasted compared to nonfasted BALB/c mice, but did not change in B6 mice (Figure 3O). The expression of Acsl3significantly decreased in both strains with fasting (Figure 3P). That of Acsl5was not changed by fasting (Figure 3Q).

	Discussion

TOP Abstract Introduction Materials and Methods Results Discussion References

 
In the present study, the hepatic lipid accumulation decreased with fasting in B6 mice, but not in BALB/c mice. Before fasting, energy uptake and body weight were the same between the fasted and nonfasted groups of both strains. Therefore, HFD-induced hepatic lipid accumulation may be affected by fasting, and the result differs between B6 and BALB/c mice.

Fasting induced decreases in circulating fatty acid, TAG, cholesterol, and glucose levels in both B6 and BALB/c mice. On the other hand, body weight and the ratio of fat weight to body weight were decreased in B6 mice, but not in BALB/c mice. These results suggest systemic differences in the reaction to fasting between HFD-fed B6 and BALB/c mice. Such strain differences of hepatic lipid accumulation are considered to be owing to differences in the expression of genes concerning lipid metabolism in the liver (Desvergne et al. 2006).

The mRNA expression of Gpam, which is involved in TAG synthesis, was significantly reduced in B6 mice, but not in BALB/c mice. This reduction may directly reflect the difference in hepatic lipid accumulation between B6 and BALB/c mice. It was reported that there was less hepatic TAG in Gpam-deficient mice than in wild-type mice (Hammond et al. 2002; Hammond et al. 2005). Moreover, it has also been shown that an increase in hepatic TAG was induced by overexpression of Gpamin mice (Linden et al. 2006). In rat hepatocytes, excess Gpamexpression leads to a decrease in β-oxidation and an increase in glycerolipid synthesis (Linden et al. 2004). Considering these findings, the fasting-induced reduction of GpammRNA expression may contribute to the difference in hepatic lipid accumulation between B6 and BALB/c mice (Figures 2and 4).

View larger version (18K): [in this window] [in a new window]   Figure 4 Hypothesis for the mechanism behind the differences of hepatic lipid accumulation between B6 and BALB/c mice. Squares with dotted lines represent enzymes.

ACS is needed for both anabolic and catabolic reactions, however details are not clear. In the present study, fasting-induced increases in Acsl1and Acsl3mRNA expression differed between B6 and BALB/c mice. This finding may reflect the differences in lipid metabolism between the two strains.

We showed that the expression of Srebp1mRNA was reduced by fasting in B6 mice. This finding is consistent with results reported by another group (Horton et al. 1998). Srebp1is a transcription factor associated with lipid metabolism, and it regulates the expression of many lipid-metabolism–related genes. Actually, Gpam, Acaca, FASN,and malic enzymeare the target genes of Srebp1(Horton et al. 2002). Therefore, the reduction in the mRNA expression of these genes in the present study may be partly caused by the reduction in Srebp1mRNA expression (Figures 2and 4).

In rats, the Srebp1mRNA level decreased with the injection of streptozotocin which abolished insulin secretion, and rose again with the injection of insulin (Shimomura et al. 1999). This finding suggests that the plasma insulin level would affect Srebp1mRNA expression. In the present study, plasma insulin concentrations decreased with fasting in both B6 and BALB/c mice. However, Srepb1mRNA expression was reduced by fasting in B6 mice, but not in BALB/c mice. This finding suggests that an insulin-associated reduction in Srebp1mRNA expression occurs only in B6 mice. Insulin resistance in B6 mice may be one possible cause of this impairment. However, we previously showed that glucose intolerance is similar between B6 and BALB/c mice (Nishikawa et al. 2007), suggesting that insulin sensitivity would not differ between B6 and BALB/c mice. Nevertheless, this result cannot completely exclude a difference in insulin sensitivity between B6 and BALB/c mice. Because previous glucose tolerance testing showed systemic glucose intolerance, insulin sensitivity and insulin signaling pathways under abnormal conditions (fasting or diabetes) differ between tissues, including skeletal muscle, adipose tissue, and liver (Heijboer et al. 2005; Kim et al. 1999; Rondinone et al. 1997), and lipid metabolism and glucose metabolism are regulated by different insulin-signaling pathways (Wolfrum et al. 2004). More investigations are needed to clarify the mechanism that leads to the strain differences.

PPAR regulates the expression of some genes related to β-oxidation (Aoyama et al. 1998; Leone et al. 1999). Hashimoto (2000)showed that PPAR-deficient mice developed severe fatty liver when fasting. This suggests that PPAR is crucial for lipid metabolism in the fasting condition. In the present study, however, the expression of PPAR mRNA did not differ between B6 and BALB/c mice, suggesting PPAR is not involved in the difference in hepatic lipid accumulation between B6 and BALB/c mice.

The activity of an enzyme is regulated not only by mRNA expression but also by reversible phosphorylation and allosteric activation of the protein by an allosteric modifier (Kennelly and Rodwell 2006). For example, the activity of Acaca, an allosteric enzyme, is stimulated by citric acid and inhibited by acetyl-CoA. Moreover, glucagon and epinephrine inhibit Acaca activity through phosphorylation of the enzyme, and insulin stimulates Acaca activity through dephosphorylation. Another example is CPT1, which is inhibited by malonyl-CoA produced by Acaca. In the present study, only the expression of lipid metabolism-related enzymes was examined, and the activities of the enzymes were not measured. The activities of each enzyme should be examined.

In conclusion, we showed that fasting induced differences in hepatic lipid accumulation between B6 and BALB/c HFD mice. This difference may be partly owing to the marked reduction in levels of Srebp1, Gpam, Acaca, malic enzymeand FASNcaused by fasting in B6 mice (Figure 4). The results suggest that fasting per se had a significant effect on HFD-induced hepatic lipid accumulation, which depends on the strain of mouse.

	Acknowledgments

 
This work was partly supported by CLEA Japan Inc.

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This version was published on October 1, 2008

Toxicologic Pathology, Vol. 36, No. 6, 850-857 (2008)
DOI: 10.1177/0192623308323920


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This Article Abstract Free Full Text (Free PDF) Free All Versions of this Article: 0192623308323920v1 36/6/850    most recent Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Add to Saved Citations Download to citation manager Request Permissions Request Reprints Add to My Marked Citations Citing Articles Citing Articles via Google Scholar Citing Articles via Scopus Google Scholar Articles by Nishikawa, S. Articles by Uetsuka, K. Search for Related Content PubMed PubMed Citation Articles by Nishikawa, S. Articles by Uetsuka, K. Pubmed/NCBI databases Compound via MeSH Substance via MeSH Hazardous Substances DB CHOLESTEROL Medline Plus Health Information Dietary Fats Diets Social Bookmarking                         What's this?