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9th International Master class NutrigenomicsWageningen Defining healthFrom basic science to industrial relevance  1 1
Nutrigenomics Masterclass2011 How to use Nutrigenomics & molecular nutrition research?  From challenges to solutions Michael MüllerNetherlands Nutrigenomics Centre & Nutrition, Metabolism and Genomics GroupDivision of Human Nutrition, Wageningen University
Why we need Nutrigenomics To understand nutrition & metabolic health To comprehensively phenotype To validate FFQs To enable strategies to optimize personal health To provide scientific evidence for health claims of “functional” foods Mechanisms Biomarkers Nutritional Science 2.0 Personal Nutrition Health claim support 3
Key questions What is your scientific problem? Why do you need nutrigenomics? What are the best suitable genomics tools for your nutrition research and how to apply them? One key question: What is the role of nutrition in the genotype-phenotype relationship? What is healthy and how to measure and quantify the health status? What is the impact of nutrigenomics for nutrition? What are the applications? What is the impact of nutrigenomics for the food (& pharma) industry?
Challenge 1: Successful ageingStay healthy as long as possible 100 % Health/ “Quality of life” time
Challenge 2: What's healthy?
Challenge 3: We have a tsunami of health problems
Challenge 4:Our “paleolithic” genes + modern diets Paleolithic era Modern Times 1.200.000 Generations between feast en famine 2-3 Generations in energy abundance % Energy % Energy 100 100 Grain Milk/-products Isolated Carbohydrates Isolated Fat/OilAlcohol Low-fat meatChicken Eggs Fish 50 Meat Chicken Fish 50 Fruit Vegetables (carrots) Nuts Honey Fruit Vegetables Beans 0 0
We are different
You are what you eat
How many human genes do we have?Not so many but….
Paternal Haplogroup:R1b1b2a1a1 a subgroup of R1b1b2                    Maternal Haplogroup: X2c1 is a subgroup of X .                                                          Where I am coming from? Locations of haplogroup R1b1b2 circa 500 years ago, before the era of intercontinental travel Locations of haplogroupX circa 500 years ago, before the era of intercontinental travel
Genotype A genotype is an individual's collection of genes. The term also can refer to the two alleles inherited for a particular gene.  The genotype is expressed when the information encoded in the genes. DNA is used to make protein and RNA molecules.  The expression of the genotype contributes to the individual's observable traits, called the phenotype.
Phenotype  A phenotype is an individual's observable traits, such as height, eye color, and blood type.  The genetic contribution to the phenotype is called the genotype.  Some traits are largely determined by the genotype, while other traits are largely determined by environmental factors (including nutrition).
Phenotype plasticity 	Phenotypic plasticity is the ability of an organism to change its phenotype in response to changes in the environment (e.g. nutrition).
1 Genotype => 5 nutritional phenotypes 155 kg 76 kg
Duality of biological information:Epigenetic & Genetic
Nutrigenomics Quantification of the nutritional genotype-phenotype  Lifestyle Nutrition Environment
Nutrigenomics will provide solutions ….but only if ask the right questions Complex Nutrition + Complex Genotypes + Complex Lifestyles + Complex Omics Technologies Simple solutions?
From mouse to men: From big to small signals Small Human muscle High Fat Diet decreases mRNA for genes involved in OXPHOS in healthy young men and mice Big Mouse muscle Diabetes 54:1926-1933, 2005
Challenges in nutrigenomics research: Small signals 24 H fasting 20 W high-fat 6 H WY KO mice vs C.
Nutrigenomics: The two strategies SignaturesProfilesBiomarkers Target GenesMechanismsPathways Molecular Nutrition& Genomics NutritionalSystems Biology ,[object Object]
Identification of dietary sensors
Identification of target genes
Reconstruction of signaling pathways
Measurement of stress signatures
Identification of early biomarkers
Nutritional plasma proteome  and metabolome + ++++ Complexity L. Afman & M. Müller J Am Diet Assoc. 2006;106:569-576.
Nutrigenomics – molecular nutrition and genomics 5 -10000 (?)metabolites 90000 (?)proteins 100000 (?) transcripts 20000 genes Müller & Kersten NRG 2003
24 A scientific question: What is the role of “free fatty acids”? During fasting During long endurance activity In obese people  “Hunger” signal or “Need for glucose” signal ? time (hours)
Fats FFA Remnant LPL VLDL Chylomicrons We are what we eat
Transcription-factor pathways mediating nutrient-gene interactions Müller & Kersten NRG 2003
Orphans? Endocrine receptorsSteroid hormonesHigh affinity Endocrine receptorsLipidsLow affinity Chawla, Science 2001  Nuclear hormone receptors
Intestine LXR   Decreased cholesterol absorption FXR    Increased bile salt recirculation PPARα    Improved lipid handling Regulation of Cholesterol and Lipid Handling in Metabolic Organ Systems by Nuclear Receptors
Nuclear receptors – how does it work?
Understanding NutritionHow nutrients regulate our genes: via sensing molecular switches Improved organcapacity by PUFAs Am J ClinNutr. 2009; 90:415-24Am J ClinNutr. 2009;90:1656-64Mol CellBiology2009;29:6257-67 Am J ClinNutr. 2010;91:208-17BMC Genomics2009 Physiol. Genomics2009Circulation 2010Diabetes 2010 Cell Metabolism 2010 Am J Clin Nutr. 2007;86(5):1515-23 PLOS ONE 2008;3(2):e1681 BMC Genomics 2008; 9:231BMC Genomics 2008; 9:262J Biol Chem. 2008;283:22620-7Arterioscler Thromb Vasc Biol. 2009;29:969-74. Plos One 2009;4(8):e6796HEPATOLOGY 2010;51:511-522 J Clin Invest. 2004;114:94-103 J Biol Chem. 2006;28:934-44  Endocrinology. 2006;147:1508-16 Physiol Genomics. 2007;30:192-204Endocrinology. 2007;148:2753-63  BMC Genomics 2007; 8:267 Arterioscler Thromb Vasc Biol. 2007;27:2420-7
Is PPARa the hepatic fatty acid sensor?  YES!
Disturbance of hepatic lipid handling leads to steatosis Mitochondrial fatty acid oxidation/ Fatty acid binding/activation ketone body synthesis Lipid transport Lipogenesis Peroxisomal/microsomal fatty acid oxidation Steatosis Lipases
PPARa controls lipid metabolism Mitochondrial fatty acid oxidation/ Fatty acid binding/activation ketone body synthesis Acsl1 Acsl3 Acsl4 Lipid transport Acsl5 Acsm3 Hahd2 Acaa2 Acss2 Hadha Adad8 Fabp1 Acot2 Hadhb Acad9 Fabp2 Acot9 Hadhsc Acad10 Cpt1a Fabp3 Abca1 Hibch Acads Slc27a1 Cpt1b Fabp4 Abcb4 Npc1 Hmgcl Acadm Slc27a2 Fabp5 Cpt2 Vldlr Abcb11 Hmgcs2 Acadl Crat Slc27a4 Abcg5 Lrp4 Slc25a20 Cd36 Acadvl Dci Abcg8 Slc22a5 Acat1 Decr1 Lipogenesis Miscellaneous Acaca Elovl5 Acacb Peroxisomal/microsomal Elovl6 Agpat2 Elovl7 Acot1 fatty acid oxidation Agpat3 Acot7 Gpam Agpat5 Hsd17b12 Acot10 Agpat6 Mod1 Acot12 Fads1 Adfp Mogat1 Scd2 Fads2 Mttp Adipor2 Slc25a10 Acaa1a Fasn Bdh Acox1 Scd1 Srebf1 Cyp4a10 Acaa1b Dgat1 Crot1 G0s2 Cyp4a12 Acot3 Ech1 Lepr Cyp4a14 Acot4 Ehhadh Lpin2 Aldh3a 2 Acot5 Lrp4 Decr2 Acot8 Hsd17b4 Mlycd Abcd2 Peci Scrab2 Glycerol metabolism Abcd3 Pctp Ppar a Pdk4 Gpd1 Pltp Pnlpa2 Gpd2 Ppargc1a Mgll Gyk Ucp2 Lipe Aqp3 Ucp3 Aqp7 Lipases Lipl Lipg Angptl4
DIETome database forevidence-basednutrition Evidence-basedNutrition Genes regulated by fatty acidsGenes regulated by high fat Genes also regulated by inflammation Query DIET GenomeEpigenomeTranscriptomeProteomeMetabolome “DIETome”database Query Nutrigenomics Potential BiomarkersOrgan-specific secreted proteins
Adipocytes at the crossroads of energy homeostasis
Nutrition Pharma   Insulin ± oral agents Oral combination Oral monotherapy Diet & exercise Nutritional prevention of complex diseases needs new biomarkers Complex Disease 100 Different & similar targets 80 60 DISEASE STATE (%)  40 20 0 TIME (months/years) HomeostasisHealth L. Afman & M. Müller J Am Diet Assoc. 2006;106:569-576.
Metabolic defects leading to the development of hepatic steatosis
Metabolism & Inflammation
Liver, FAT & NASH/NAFLD ,[object Object]
Different stages in NAFLD progression:
Molecular events involved in NASH pathogenesis:
Role of PPARa (Endocrinology 2008 & Hepatology 2010)
Role Kupffer cells (Hepatology 2010)
Role of macrophages in lipid metabolism (JBC 2008; Cell Metabolism 2010)hepatic steatosis 		              steatohepatitis (NASH) & fibrosis	cirrhosis
Interaction between WAT and liver tissue essential for NASH/NAFLD in C57Bl/6 mice Objective:  Nonalcoholic fatty liver disease (NAFLD) is strongly linked to obesity and diabetes, suggesting an important role of adipose tissue in the pathogenesis of NAFLD.  Here we aimed to investigate the interaction between adipose tissue and liver in NAFLD, and identify potential early plasma markers that predict NASH.
Experimental Design tissue collection run-in diet 20 weeks diet intervention ,[object Object],multiple proteinassays ,[object Object]
stratification on body weightfrozen sections: histological feat. lipid content RNA extraction:Affx microarrays 10 LFD 0 2 4 8 12 16 20 weeks 20 LFD -3 quality control & data analysis pipeline 10 HFD Mouse  genome  430 2.0 10% low  fat diet  (palm oil) 45% high fat diet (palm oil) ,[object Object],paraffin sections: histological feat. RNA extraction: real-time PCR
High fat diet-induced obesity 0 2 4 8 12 16 20 HFL LFL HFH LFH 25 20 * * 15 ** BW gain (g) * 10 * * * * 5 0 weeks under diet intervention Liver TG content Hepatomegaly ALT plasma activity 200 10 100 *** *** ** 160 8 80 ** 120 6 60 * Ratio LW/BW (%) mg TG/g liver ALT activity (UI) 80 4 40 * * 40 2 20 0 0 0 LFL LFH HFL HFH
Adipose dysfunction in HFH mice Leptin
A subpopulation of mice fed HFD develops NASH

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Intro into Nutrigenomics & molecular nutrition research

  • 1. 9th International Master class NutrigenomicsWageningen Defining healthFrom basic science to industrial relevance 1 1
  • 2. Nutrigenomics Masterclass2011 How to use Nutrigenomics & molecular nutrition research? From challenges to solutions Michael MüllerNetherlands Nutrigenomics Centre & Nutrition, Metabolism and Genomics GroupDivision of Human Nutrition, Wageningen University
  • 3. Why we need Nutrigenomics To understand nutrition & metabolic health To comprehensively phenotype To validate FFQs To enable strategies to optimize personal health To provide scientific evidence for health claims of “functional” foods Mechanisms Biomarkers Nutritional Science 2.0 Personal Nutrition Health claim support 3
  • 4. Key questions What is your scientific problem? Why do you need nutrigenomics? What are the best suitable genomics tools for your nutrition research and how to apply them? One key question: What is the role of nutrition in the genotype-phenotype relationship? What is healthy and how to measure and quantify the health status? What is the impact of nutrigenomics for nutrition? What are the applications? What is the impact of nutrigenomics for the food (& pharma) industry?
  • 5. Challenge 1: Successful ageingStay healthy as long as possible 100 % Health/ “Quality of life” time
  • 7. Challenge 3: We have a tsunami of health problems
  • 8. Challenge 4:Our “paleolithic” genes + modern diets Paleolithic era Modern Times 1.200.000 Generations between feast en famine 2-3 Generations in energy abundance % Energy % Energy 100 100 Grain Milk/-products Isolated Carbohydrates Isolated Fat/OilAlcohol Low-fat meatChicken Eggs Fish 50 Meat Chicken Fish 50 Fruit Vegetables (carrots) Nuts Honey Fruit Vegetables Beans 0 0
  • 10. You are what you eat
  • 11. How many human genes do we have?Not so many but….
  • 12. Paternal Haplogroup:R1b1b2a1a1 a subgroup of R1b1b2                   Maternal Haplogroup: X2c1 is a subgroup of X .                                                         Where I am coming from? Locations of haplogroup R1b1b2 circa 500 years ago, before the era of intercontinental travel Locations of haplogroupX circa 500 years ago, before the era of intercontinental travel
  • 13. Genotype A genotype is an individual's collection of genes. The term also can refer to the two alleles inherited for a particular gene. The genotype is expressed when the information encoded in the genes. DNA is used to make protein and RNA molecules. The expression of the genotype contributes to the individual's observable traits, called the phenotype.
  • 14. Phenotype A phenotype is an individual's observable traits, such as height, eye color, and blood type. The genetic contribution to the phenotype is called the genotype. Some traits are largely determined by the genotype, while other traits are largely determined by environmental factors (including nutrition).
  • 15. Phenotype plasticity Phenotypic plasticity is the ability of an organism to change its phenotype in response to changes in the environment (e.g. nutrition).
  • 16. 1 Genotype => 5 nutritional phenotypes 155 kg 76 kg
  • 17. Duality of biological information:Epigenetic & Genetic
  • 18. Nutrigenomics Quantification of the nutritional genotype-phenotype Lifestyle Nutrition Environment
  • 19. Nutrigenomics will provide solutions ….but only if ask the right questions Complex Nutrition + Complex Genotypes + Complex Lifestyles + Complex Omics Technologies Simple solutions?
  • 20. From mouse to men: From big to small signals Small Human muscle High Fat Diet decreases mRNA for genes involved in OXPHOS in healthy young men and mice Big Mouse muscle Diabetes 54:1926-1933, 2005
  • 21. Challenges in nutrigenomics research: Small signals 24 H fasting 20 W high-fat 6 H WY KO mice vs C.
  • 22.
  • 28. Nutritional plasma proteome and metabolome + ++++ Complexity L. Afman & M. Müller J Am Diet Assoc. 2006;106:569-576.
  • 29. Nutrigenomics – molecular nutrition and genomics 5 -10000 (?)metabolites 90000 (?)proteins 100000 (?) transcripts 20000 genes Müller & Kersten NRG 2003
  • 30. 24 A scientific question: What is the role of “free fatty acids”? During fasting During long endurance activity In obese people “Hunger” signal or “Need for glucose” signal ? time (hours)
  • 31. Fats FFA Remnant LPL VLDL Chylomicrons We are what we eat
  • 32. Transcription-factor pathways mediating nutrient-gene interactions Müller & Kersten NRG 2003
  • 33. Orphans? Endocrine receptorsSteroid hormonesHigh affinity Endocrine receptorsLipidsLow affinity Chawla, Science 2001 Nuclear hormone receptors
  • 34. Intestine LXR Decreased cholesterol absorption FXR Increased bile salt recirculation PPARα Improved lipid handling Regulation of Cholesterol and Lipid Handling in Metabolic Organ Systems by Nuclear Receptors
  • 35. Nuclear receptors – how does it work?
  • 36. Understanding NutritionHow nutrients regulate our genes: via sensing molecular switches Improved organcapacity by PUFAs Am J ClinNutr. 2009; 90:415-24Am J ClinNutr. 2009;90:1656-64Mol CellBiology2009;29:6257-67 Am J ClinNutr. 2010;91:208-17BMC Genomics2009 Physiol. Genomics2009Circulation 2010Diabetes 2010 Cell Metabolism 2010 Am J Clin Nutr. 2007;86(5):1515-23 PLOS ONE 2008;3(2):e1681 BMC Genomics 2008; 9:231BMC Genomics 2008; 9:262J Biol Chem. 2008;283:22620-7Arterioscler Thromb Vasc Biol. 2009;29:969-74. Plos One 2009;4(8):e6796HEPATOLOGY 2010;51:511-522 J Clin Invest. 2004;114:94-103 J Biol Chem. 2006;28:934-44 Endocrinology. 2006;147:1508-16 Physiol Genomics. 2007;30:192-204Endocrinology. 2007;148:2753-63 BMC Genomics 2007; 8:267 Arterioscler Thromb Vasc Biol. 2007;27:2420-7
  • 37. Is PPARa the hepatic fatty acid sensor? YES!
  • 38. Disturbance of hepatic lipid handling leads to steatosis Mitochondrial fatty acid oxidation/ Fatty acid binding/activation ketone body synthesis Lipid transport Lipogenesis Peroxisomal/microsomal fatty acid oxidation Steatosis Lipases
  • 39. PPARa controls lipid metabolism Mitochondrial fatty acid oxidation/ Fatty acid binding/activation ketone body synthesis Acsl1 Acsl3 Acsl4 Lipid transport Acsl5 Acsm3 Hahd2 Acaa2 Acss2 Hadha Adad8 Fabp1 Acot2 Hadhb Acad9 Fabp2 Acot9 Hadhsc Acad10 Cpt1a Fabp3 Abca1 Hibch Acads Slc27a1 Cpt1b Fabp4 Abcb4 Npc1 Hmgcl Acadm Slc27a2 Fabp5 Cpt2 Vldlr Abcb11 Hmgcs2 Acadl Crat Slc27a4 Abcg5 Lrp4 Slc25a20 Cd36 Acadvl Dci Abcg8 Slc22a5 Acat1 Decr1 Lipogenesis Miscellaneous Acaca Elovl5 Acacb Peroxisomal/microsomal Elovl6 Agpat2 Elovl7 Acot1 fatty acid oxidation Agpat3 Acot7 Gpam Agpat5 Hsd17b12 Acot10 Agpat6 Mod1 Acot12 Fads1 Adfp Mogat1 Scd2 Fads2 Mttp Adipor2 Slc25a10 Acaa1a Fasn Bdh Acox1 Scd1 Srebf1 Cyp4a10 Acaa1b Dgat1 Crot1 G0s2 Cyp4a12 Acot3 Ech1 Lepr Cyp4a14 Acot4 Ehhadh Lpin2 Aldh3a 2 Acot5 Lrp4 Decr2 Acot8 Hsd17b4 Mlycd Abcd2 Peci Scrab2 Glycerol metabolism Abcd3 Pctp Ppar a Pdk4 Gpd1 Pltp Pnlpa2 Gpd2 Ppargc1a Mgll Gyk Ucp2 Lipe Aqp3 Ucp3 Aqp7 Lipases Lipl Lipg Angptl4
  • 40. DIETome database forevidence-basednutrition Evidence-basedNutrition Genes regulated by fatty acidsGenes regulated by high fat Genes also regulated by inflammation Query DIET GenomeEpigenomeTranscriptomeProteomeMetabolome “DIETome”database Query Nutrigenomics Potential BiomarkersOrgan-specific secreted proteins
  • 41. Adipocytes at the crossroads of energy homeostasis
  • 42. Nutrition Pharma Insulin ± oral agents Oral combination Oral monotherapy Diet & exercise Nutritional prevention of complex diseases needs new biomarkers Complex Disease 100 Different & similar targets 80 60 DISEASE STATE (%) 40 20 0 TIME (months/years) HomeostasisHealth L. Afman & M. Müller J Am Diet Assoc. 2006;106:569-576.
  • 43. Metabolic defects leading to the development of hepatic steatosis
  • 45.
  • 46. Different stages in NAFLD progression:
  • 47. Molecular events involved in NASH pathogenesis:
  • 48. Role of PPARa (Endocrinology 2008 & Hepatology 2010)
  • 49. Role Kupffer cells (Hepatology 2010)
  • 50. Role of macrophages in lipid metabolism (JBC 2008; Cell Metabolism 2010)hepatic steatosis steatohepatitis (NASH) & fibrosis cirrhosis
  • 51. Interaction between WAT and liver tissue essential for NASH/NAFLD in C57Bl/6 mice Objective: Nonalcoholic fatty liver disease (NAFLD) is strongly linked to obesity and diabetes, suggesting an important role of adipose tissue in the pathogenesis of NAFLD. Here we aimed to investigate the interaction between adipose tissue and liver in NAFLD, and identify potential early plasma markers that predict NASH.
  • 52.
  • 53.
  • 54. High fat diet-induced obesity 0 2 4 8 12 16 20 HFL LFL HFH LFH 25 20 * * 15 ** BW gain (g) * 10 * * * * 5 0 weeks under diet intervention Liver TG content Hepatomegaly ALT plasma activity 200 10 100 *** *** ** 160 8 80 ** 120 6 60 * Ratio LW/BW (%) mg TG/g liver ALT activity (UI) 80 4 40 * * 40 2 20 0 0 0 LFL LFH HFL HFH
  • 55. Adipose dysfunction in HFH mice Leptin
  • 56. A subpopulation of mice fed HFD develops NASH
  • 57. Immunohistochemicalstaining confirms enhanced inflammation and early fibrosis in HFH mice Macrophage CD68 Collagen Stellate cell GFAP
  • 58. Results I Mice exhibited pronounced heterogeneity in liver histological scoring, leading to classification into 4 subgroups: LF-low (LFL) responders displaying normal liver morphology, LF-high (LFH) responders showing benign hepatic steatosis, HF-low (HFL) responders displaying pre-NASH with macrovesicular lipid droplets, HF-high (HFH) responders exhibiting overt NASH characterized by ballooning of hepatocytes, presence of Mallory bodies, and activated inflammatory cells.
  • 59. Upregulation of inflammatory and fibrotic gene expression in HFH responder mice
  • 61. Change in adipose gene expression indicate adipose tissue dysfunction
  • 62. Plasma proteins as early predictive biomarker for NASH in C57Bl/6 mice
  • 63. Conclusions Our data support the existence of a tight relationship between adipose tissue dysfunction and NASH pathogenesis. It points to several novel potential predictive biomarkers for NASH. Diabetes. 2010;59:3181-91.
  • 64.
  • 65. To quantify the nutritional needs for optimized fitness at different life stages (“personalized” nutrition);
  • 66. To improve early diagnostics of nutrition related disorders (“challenge tests”);
  • 67. To support the development of “smart healthy food patterns” for modern mankind (healthy and tasty, sustainable, affordable)
  • 68.
  • 69. 2 Meals a day, work as long as possible & embrace challenge Walter Breuning (1896 - 2011)
  • 70. Thanks Lydia Afman Mark Bouwens Susan van Dijk DiederikEsser Sergio Lopez Lisette de Groot Marianne Geleijnse Ondine van de Rest MariekeBos Edith Feskens RikHeijligenberg Dianne Hoelen Jeanne de Vries Geert Heidema

Notas do Editor

  1. Inflammation has been associated with many disease phenotypes including steatohepatitis or diabetes. This relationship is in particular when inflammation is chronic or non-resolving. There is an interaction between metabolism and inflammation with positive or negative consequences with respect to organ and systemic health.In my talk I will briefly discuss two unpublished studies, one investigating the important interaction of WAT and liver in particular under conditions of diet-induced obesity. Organ-specific macrophages in WAT and liver play an crucial role in progressing organ-specific inflammatory phenotypes. In the second study we found very interesting interaction between dietary fat and macrophages in mesenteric lymph nodes that are exposed postprandially to very high concentrations of chylomicrons. We used a k.o. mouse for ANGPTL4 and could show that chronic consumption of saturated fat can be deadly.
  2. A) Bodyweight changes in the 4 subgroups during the 21 week dietary intervention. White squares: LFL, Light grey squares: LFH, dark grey squares: HFL, black squares: HFH. B) Mean daily energy intake. C) Positive correlation between final bodyweight and liver triglyceride concentration (P<0.05). D) Weight of epididymal fat depot. E) Adipose tissue leptin mRNA expression as determined by qPCR. Mean expression in LFL mice was set at 100%. F) Plasma free fatty acid levels. Error bars reflect standard deviation. * = significantly different from HFL mice according to Student’s t-test (P<0.05). Number of mice per group: n=4 (LFL, HFL, HFH), n=6 (LFH).
  3. A subpopulation of mice fed HFD develops NASH. Haematoxylin and eosin staining (D) and oil red O staining (E) of representative liver sections of the 4 subgroups
  4. (Immuno)histochemical staining confirms enhanced inflammation and early fibrosis in HFH miceImmunohistochemical staining of macrophage activation in representative liver section of HFL and HFH mice using antibody against the specific macrophagemarker Cd68Collagen staining using fast green FCF/sirius red F3B. Staining of stellate cell activation using antibody against GFAP.
  5. - Number of genes up- or down-regulated in the various subgroups in comparison to the LFL mice, as determined by Affymetrix GeneChip analysis. Genes with a p-value below 0.05 were considered significantly regulated. - Heat map showing changes in expression of selected genes involved in lipid metabolism, inflammation and fibrosis in liver. Changes in gene expression of selected genes as determined by real-time quantitative PCR. Mean expression in LFL mice was set at 100%. Error bars reflect standard deviation. Bars with different letters are statistically different (P<0.05 according to Student’s t-test). Number of mice per group: n=4 (LFL, HFL, HFH), n=6 (LFH).
  6. Haematoxylin and eosin staining of representative adipose tissue sections. Immunohistochemical staining of macrophages using antibody against Cd68. Collagen staining using fast green FCF/sirius red F3B.
  7. Adipose tissue mRNA expression of a selected group of genes was determined by quantitative real-time PCR after 21 weeks of dietary intervention. Mean expression in LFL mice was set at 100%. Error bars reflect standard deviation. * = significantly different from HFL mice according to Student’s t-test (P<0.05). Number of mice per group: n=4 (LFL, HFL, HFH), n=6 (LFH).
  8. . A) Plasma concentration of haptoglobin, TIMP-1, IL-1β, leptin and insulin were determined by multiplex assay at specific time points during the 21 weeks of dietary intervention after a 6h fast. White squares: LFL, Light grey squares: LFH, dark grey squares: HFL, black squares: HFH. Error bars reflect standard deviation. * = significantly different from HFL mice according to Student’s t-test (P<0.05). Number of mice per group: n=4 (LFL, HFL, HFH), n=6 (LFH).