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DR MUHAMMAD MUSTANSAR
 Membrane component
 Precurser to

    ◦ Bile acids
    ◦ Vitamin D
    ◦ Steroid hormones
   Dietary cholesterol
    ◦ From chylomicron remnants
   Cholesterol from extra-hepatic tissues
    ◦ Reverse cholesterol transport via HDL
      Chylomicron remnants
      IDL
   De novo synthesis
   VLDL -> LDL
    ◦ Transport to extra-hepatic tissues
   Direct excretion into bile
    ◦ Gallstones commonly are precipitates of cholesterol
      Occurs when bile becomes supersaturated with cholesterol
        Obesity, biliary stasis, infections
   Bile acid synthesis and excretion into bile
   Primary site: liver (~1g/d)
    ◦ Secondary sites: adrenal cortex, ovaries, testes
   Overall equation:
O          OH          O
          −
           O    C   CH2   C     CH2   C   SCoA

                          CH3

               hydroxymethylglutaryl-CoA

Hydroxymethylglutaryl-coenzyme A (HMG-CoA)
is the precursor for cholesterol synthesis.
HMG-CoA is also an intermediate on the pathway for
synthesis of ketone bodies from acetyl-CoA.
The enzymes for ketone body production are located in
the mitochondrial matrix.
HMG-CoA destined for cholesterol synthesis is made by
equivalent, but different, enzymes in the cytosol.
O            O

                            H3C   C     CH2    C     SCoA
          H2 O + O                      acetoacetyl-CoA
          H3 C   C     SCoA
          acetyl-CoA                  HMG-CoA
                       HSCoA          Synthase

                        O          OH            O
                 −
                 O      C   CH2    C     CH2     C   SCoA

                                   CH3
                               hydroxymethylglutaryl-CoA
   HMG-CoA is formed by condensation of acetyl-CoA &
    acetoacetyl-CoA, catalyzed by HMG-CoA Synthase.
   HMG-CoA Reductase catalyzes production of mevalonate
    from HMG-CoA.
   Formation of HMG CoA (cyto)
    ◦ Analogous to KB synthesis (mito)


   Conversion of HMG CoA to activated
    isoprenoids
   Condensation of
    isoprenoids to
    squalene
    ◦ Six isoprenoids
      condense to form 30-C
      molecue
   Conversion of Squalene to
    Cholesterol
 All carbons from acetyl-CoA
 Requires NADPH, ATP, & O
                              2

   Stages
    ◦ One: forms HMG CoA
    ◦ Two: forms activated 5 carbon intermediates (isoprenoids)
    ◦ Three: six isoprenoids form squalene
    ◦ Four: squalene + O2 form cholesterol
   Cellular cholesterol content exerts transcriptional control
    ◦ HMG-CoA reductase
       Half life = 2 hours
    ◦ LDL-receptor synthesis
   Nutrigenomics:
    ◦ interactions between environment and individual genes and how
      these interactions affect clinical outcomes
   Covalent Modification of
    HMG-CoA Reductase
    ◦ Insulin induces protein
      phosphatase
    ◦ Activates HMG-CoA reductase
   Feeding promotes
    cholesterol synthesis
    ◦ Activates reg. enzyme
    ◦ Provides substrate: acetyl CoA
    ◦ Provides NADPH
   Covalent Modification of
    HMG-CoA Reductase
    ◦ Glucagon stimulates
      adenyl cyclase producing
      cAMP
    ◦ cAMP activates protein
      kinase A
    ◦ Inactivates HMG-CoA
      reductase
   Fasting inhibits
    cholesterol synthesis
   Major excretory form of cholesterol
    ◦ Steroid ring is not degraded in humans
    ◦ Occurs in liver
   Bile acid/salts involved in dietary lipid digestion
    as emulsifiers
   Primary bile acids
    ◦ Good emulsifying agents

      All OH groups on same side
      pKa = 6 (partially ionized)
   Conjugated bile salts
    ◦ Amide bonds with glycine
      or taurine
    ◦ Very good emulsifier
      pKa lower than bile acids
   Hydroxylation
    ◦ Cytochrome P-450/mixed
      function oxidase system
   Side chain cleavage
   Conjugation
   Secondary bile acids
    ◦ Intestinal bacterial
      modification
       Deconjugation
       Dehydroxylation
          Deoxycholic acid
          Lithocholic acid
   Enterohepatic circulation
    ◦ 98% recycling of bile acids
   Cholestyramine
    Treatment
    ◦ Resin binds bile acids
    ◦ Prevents recycling
    ◦ Increased uptake of LDL-C
      for bile acid synthesis
Plant stanols
No double bond on B ring




Plant sterols
Different side chains
Structures of
Common statin
drugs
   8 yo girl
    ◦ Admitted for heart/liver transplant
   History
    ◦   CHD in family
    ◦   2 yo xanthomas appear on legs
    ◦   4 yo xanthomas appear on elbows
    ◦   7 yo admitted w/ MI symptoms
           [TC] = 1240 mg/dl
           [TG] = 350 mg/dl
           [TC]father = 355 mg/dl
           [TC]mother = 310 mg/dl
    ◦ 2 wks after MI had coronary bypass surgery
    ◦ Past year severe angina & second bypass
    ◦ Despite low-fat diet, cholestyramine, & lovastatin, [TC] = 1000
      mg/dl
   Raised, waxy
    appearing, often yellow
    skin lesions (shown
    here on knee)
    ◦ Associated with hyperlipidemia
   Tendon xanthomas common
    on Achilles and hand
    extensor tendons
Xanthomas of the eyelid
Eruptive Xanthomas           -generally associated with
-generally associated with   hypercholesterolemia
hypertriglyceridemia
   Aldosterone
    ◦ C21 derivative of cholesterol
    ◦ Promotes renal
       Sodium retention
       Potassium excretion
   Glucocorticoids (cortisol)
    ◦ Starvation
       Hepatic gluconeogenesis
       Muscle protein degradation
       Adipose lipolysis
   Adrenal androgens
    ◦ Dehydroepiandroterone (DHEA)
       Precurser to potent androgens in extra-
        adrenal tissues

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CHOLESTEROL METABOLISM muhammad mustansar FJMC LAHORE

  • 2.
  • 3.  Membrane component  Precurser to ◦ Bile acids ◦ Vitamin D ◦ Steroid hormones
  • 4. Dietary cholesterol ◦ From chylomicron remnants  Cholesterol from extra-hepatic tissues ◦ Reverse cholesterol transport via HDL  Chylomicron remnants  IDL  De novo synthesis
  • 5. VLDL -> LDL ◦ Transport to extra-hepatic tissues  Direct excretion into bile ◦ Gallstones commonly are precipitates of cholesterol  Occurs when bile becomes supersaturated with cholesterol  Obesity, biliary stasis, infections  Bile acid synthesis and excretion into bile
  • 6. Primary site: liver (~1g/d) ◦ Secondary sites: adrenal cortex, ovaries, testes  Overall equation:
  • 7. O OH O − O C CH2 C CH2 C SCoA CH3 hydroxymethylglutaryl-CoA Hydroxymethylglutaryl-coenzyme A (HMG-CoA) is the precursor for cholesterol synthesis. HMG-CoA is also an intermediate on the pathway for synthesis of ketone bodies from acetyl-CoA. The enzymes for ketone body production are located in the mitochondrial matrix. HMG-CoA destined for cholesterol synthesis is made by equivalent, but different, enzymes in the cytosol.
  • 8. O O H3C C CH2 C SCoA H2 O + O acetoacetyl-CoA H3 C C SCoA acetyl-CoA HMG-CoA HSCoA Synthase O OH O − O C CH2 C CH2 C SCoA CH3 hydroxymethylglutaryl-CoA  HMG-CoA is formed by condensation of acetyl-CoA & acetoacetyl-CoA, catalyzed by HMG-CoA Synthase.  HMG-CoA Reductase catalyzes production of mevalonate from HMG-CoA.
  • 9. Formation of HMG CoA (cyto) ◦ Analogous to KB synthesis (mito)  Conversion of HMG CoA to activated isoprenoids
  • 10. Condensation of isoprenoids to squalene ◦ Six isoprenoids condense to form 30-C molecue
  • 11. Conversion of Squalene to Cholesterol
  • 12.  All carbons from acetyl-CoA  Requires NADPH, ATP, & O 2  Stages ◦ One: forms HMG CoA ◦ Two: forms activated 5 carbon intermediates (isoprenoids) ◦ Three: six isoprenoids form squalene ◦ Four: squalene + O2 form cholesterol
  • 13. Cellular cholesterol content exerts transcriptional control ◦ HMG-CoA reductase  Half life = 2 hours ◦ LDL-receptor synthesis  Nutrigenomics: ◦ interactions between environment and individual genes and how these interactions affect clinical outcomes
  • 14. Covalent Modification of HMG-CoA Reductase ◦ Insulin induces protein phosphatase ◦ Activates HMG-CoA reductase  Feeding promotes cholesterol synthesis ◦ Activates reg. enzyme ◦ Provides substrate: acetyl CoA ◦ Provides NADPH
  • 15. Covalent Modification of HMG-CoA Reductase ◦ Glucagon stimulates adenyl cyclase producing cAMP ◦ cAMP activates protein kinase A ◦ Inactivates HMG-CoA reductase  Fasting inhibits cholesterol synthesis
  • 16. Major excretory form of cholesterol ◦ Steroid ring is not degraded in humans ◦ Occurs in liver  Bile acid/salts involved in dietary lipid digestion as emulsifiers
  • 17. Primary bile acids ◦ Good emulsifying agents  All OH groups on same side  pKa = 6 (partially ionized)  Conjugated bile salts ◦ Amide bonds with glycine or taurine ◦ Very good emulsifier  pKa lower than bile acids
  • 18. Hydroxylation ◦ Cytochrome P-450/mixed function oxidase system  Side chain cleavage  Conjugation  Secondary bile acids ◦ Intestinal bacterial modification  Deconjugation  Dehydroxylation  Deoxycholic acid  Lithocholic acid
  • 19. Enterohepatic circulation ◦ 98% recycling of bile acids  Cholestyramine Treatment ◦ Resin binds bile acids ◦ Prevents recycling ◦ Increased uptake of LDL-C for bile acid synthesis
  • 20. Plant stanols No double bond on B ring Plant sterols Different side chains
  • 22.
  • 23. 8 yo girl ◦ Admitted for heart/liver transplant  History ◦ CHD in family ◦ 2 yo xanthomas appear on legs ◦ 4 yo xanthomas appear on elbows ◦ 7 yo admitted w/ MI symptoms  [TC] = 1240 mg/dl  [TG] = 350 mg/dl  [TC]father = 355 mg/dl  [TC]mother = 310 mg/dl ◦ 2 wks after MI had coronary bypass surgery ◦ Past year severe angina & second bypass ◦ Despite low-fat diet, cholestyramine, & lovastatin, [TC] = 1000 mg/dl
  • 24. Raised, waxy appearing, often yellow skin lesions (shown here on knee) ◦ Associated with hyperlipidemia  Tendon xanthomas common on Achilles and hand extensor tendons
  • 25. Xanthomas of the eyelid Eruptive Xanthomas -generally associated with -generally associated with hypercholesterolemia hypertriglyceridemia
  • 26.
  • 27. Aldosterone ◦ C21 derivative of cholesterol ◦ Promotes renal  Sodium retention  Potassium excretion  Glucocorticoids (cortisol) ◦ Starvation  Hepatic gluconeogenesis  Muscle protein degradation  Adipose lipolysis  Adrenal androgens ◦ Dehydroepiandroterone (DHEA)  Precurser to potent androgens in extra- adrenal tissues