Gluconeogenesis and glycogenolysis

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GLUCONEOGENESIS & GLYCOGENOLYSIS PRESENTED BY- HASNAHANA CHETIA M.Sc Ist Sem, Dept. Of Biotechnology, G.U.

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GLUCONEOGENESIS AND GLYCOGENOLYSIS

Transcript of Gluconeogenesis and glycogenolysis

Page 1: Gluconeogenesis and glycogenolysis

GLUCONEOGENESIS&GLYCOGENOLYSIS

PRESENTED BY-HASNAHANA CHETIAM.Sc Ist Sem,Dept. Of Biotechnology, G.U.

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GLUCONEOGENESIS

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Gluconeogenesis is a metabolic pathway occurring in living beings for synthesis of glucose from non-carbohydrate precursors. It converts pyruvate and its related three- and four-carbon compounds into glucose. It is an irreversible process . It occurs in cytosol.

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PATHWAY CONVERSION OF PYRUVATE TO PHOSPHOENOL

PYRUVATE (PEP)-

Pyruvate is transported from cytosol to mitochondria or generated from alanine by transamination within mitochondria. Then, pyruvate carboxylase, an enzyme that uses biotin as a co-enzyme; converts pyruvate to oxaloacetate.

PYRUVATE + HCO₃⁻ + ATP OXALOACETATE + ADP + Pi

Because mitochondrial membrane has no transporter for oxaloacetate, so pyruvate is reduced to malate by malate dehydrogenase at the expense of NADH.

OXALOACETATE + NADH + H⁺ ↔ L-MALATE + NAD⁺

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Malate leaves the mitochondrion through a specific transporter in the inner mitochondrial membrane and in cytosol, it is re-oxidised to oxaloacetate, with the production of cytosolic NADH.

MALATE + NAD⁺OXALOACETATE + NADH + H⁺

The oxaloacetate is then converted to PEP by phosphoenolpyruvate carboxykinase.

OXALOACETATE + GTP ↔PEP + CO₂ + GDP

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CONVERSION OF PEP TO 2-PHOSPHOGLYCERATE-

This step is reverse of the step in glycolysis. This reaction is performed by Enolase.

CONVERSION OF 2-PHOSPHOGLYCERATE TO 3-PHOSPHOGLYCERATE-

This step is also reverse of the step in glycolysis. This step is catalyzed by the enzyme Phosphoglycerate Mutase.

CONVERSION OF 3-PHOSPHOGLYCERATE TO 1,3-BISPHOSPHOGLYCERATE-

This step is reverse of the step in glycolysis as well. This step is catalyzed by Phosphoglycerate Kinase.

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REDUCTION OF 1,3 BISPHOSPHOGLYCERATE TO GLYCERALDEHYDE-3-PHOSPHATE –

This step is reverse of the step in glycolysis. In this step, 1,3-Bisphosphoglycerate is reduced to Glyceraldehyde-3-phosphate by the enzyme Glyceraldehyde 3-phosphate dehydrogenase.

INTERCONVERSION OF TRIOSE PHOSPHATES-

This step is reverse of the step in glycolysis. The Glyceraldehyde 3-phosphate is interconverted to Dihydroxyacetone phosphate by Triose isomerase phosphate.

CONVERSION OF DIHYDROXYACETONE PHOSPHATE TO FRUCTOSE 1,6-BISPHOSPHATE-

This step is also reverse of the step in glycolysis. This step is performed by the enzyme Fructose 1,6 Bisphosphate Aldolase.

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CONVERSION OF FRUCTOSE 1,6 BISPHOSPHATE TO FRUCTOSE 6- PHOSPHATE –

This is an irreversible step where Fructose 1,6 Bisphosphate is converted to Fructose 6- Phosphate by the Mg⁺⁺-dependent enzyme, Fructose 1,6 Bisphosphatase which promotes the hydrolysis of the C-1 phosphate.

Fructose 1,6 Bisphosphate + H₂O Fructose 6- Phosphate + Pi

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CONVERSION OF FRUCTOSE 6-PHOSPHATE TO GLUCOSE 6-PHOSPHATE –

This step is reverse of the step in glycolysis. This reversible conversion of a ketose to an aldose is done by the enzyme Phosphohexose Isomerase.

CONVERSION OF GLUCOSE 6- PHOSPHATE TO GLUCOSE-

It is the final reaction of gluconeogenesis where Glucose 6-Phosphate is dephosphorylated to yield Glucose by another Mg⁺⁺-dependent enzyme Glucose 6-Phosphatase.

Glucose 6-Phosphate + H₂O Glucose + Pi

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THE THREE BYPASS REACTIONS Almost all the steps of Gluconeogenesis are

reverse of Glycolysis except three reactions-1. CONVERSION OF PYRUVATE TO PHOSPHOENOL

PYRUVATE

2. CONVERSION OF FRUCTOSE 1,6 BISPHOSPHATE TO FRUCTOSE 6- PHOSPHATE

3. CONVERSION OF GLUCOSE 6- PHOSPHATE TO GLUCOSE

Here a different set of enzymes are utilized than Glycolysis and are characterized by a large –ve free energy change, ∆G whereas in the other reactions, the value of ∆G is near to 0.

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REGULATION There are 3 steps involved in

regulation of Gluconeogenesis.1. CONVERSION OF PYRUVATE TO

OXALOACETATE- When the cell’s energy need is

being met, oxidative phosphorylation slows down, NADH:NAD⁺ rises and inhibits citric acid cycle due to which Acetyl-CoA accumulates. Since Acetyl-CoA is an positive allosteric modulator of Pyruvate Carboxylase, it stimulates gluconeogenesis and increases the formation of glucose from pyruvate.

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2. CONVERSION OF FRUCTOSE 1,6-BISPHOSPHATE TO FRUCTOSE 6-PHOSPHATE-

The enzyme FBPase-1 involved in this reaction is strongly inhibited by AMP. So, when a high proportion of the cell’s adenylate is in the form of ATP, gluconeogenesis is favored.

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3. HORMONAL REGULATION OF GLUCONEOGENESIS-

The hormonal regulation of gluconeogenesis is mediated by Fructose 2,6-Bisphosphate, an allosteric effector for the enzyme FBPase-1. The hormones epinephrine and glucagon decreases the concentration of Fructose 2,6-Bisphosphate by raising cAMP and bringing about phosphorylation, i.e., inactivation of PFK-2 and activates FBPase-2 leading to breakdown of Fructose 2,6-Bisphosphate. Insulin increases the concentration of Fructose 2,6-Bisphosphate by dephosphorylating PFK-2.

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GLYCOGENOLYSIS

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Glycogenolysis is a metabolic  process by which glycogen, the primary carbohydrate stored in the liver and muscle cells of animals, is broken down into glucose to provide immediate energy and to maintain blood glucose levels during fasting.

Glycogen is catabolized by removal of a glucose monomer through cleavage with inorganic phosphate to produce glucose-1-phosphate.This derivative of glucose is then converted to glucose-6-phosphate, an intermediate in glycolysis.

It takes place in the muscle and liver tissues, where glycogen is stored, as a hormonal response to epinephrine and/or glucagon.

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PATHWAY First step- The overall reaction for the 1st step is: Glycogen (n residues) + Pi ↔ Glycogen (n-1

residues)+ G1P Here, glycogen phosphorylase cleaves

the bond at the C1 position by substitution of a phosphoryl group. It breaks down glucose polymer at [α14] linkages until 4 linked glucoses are left on the branch.

Pyridoxal phosphate is an important co-factor in this reaction, as its phosphate group acts as a general acid catalyst, promoting attack by Pi on the glycosidic bond.

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Second step- The second step

involves the enzyme oligo α[1→6] to α[1→4] glucantransferase or debranching enzyme, which transfers the three remaining glucose units to another 1,4 terminal of glycogen, which exposes the α[1→6] branching point.

The final action of this enzyme is the hydrolysis of the remaining glucose attached at the α[1→6] branch point, which gives one free glucose molecule.

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Third step- The third and last stage

converts G1P (glucose-1-phosphate) to G6P (glucose-6-phosphate) through the enzyme phosphoglucomutase.

G1P ↔ G6P Here the enzyme donates a phosphoryl

group to C-6 of the substrate and accepts a phosphoryl group from C-1.

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FATES OF GLUCOSE 6 PHOSPHATE This G6P can enter glycolysis and serve as

an energy source to support muscle contraction.

In liver, it releases glucose into blood when blood glucose level drops.

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REGULATION OF GLYCOGEN PHOSPHORYLASE Glycogen phosphorylase is activated in

response to Glucagon or Epinephrine which raise the [cAMP] level and activate Protein KinaseA. PKA phosphorylates and activates Phosphorylase Kinase, which converts Glycogen Phosphorylase B to its active A form.

Phosphoprotein Phosphatase 1 reverses the phosphorylation of Glycogen Phosphorylase A, inactivating it.

Glucose binds to the liver isozyme of Glycogen Phosphorylase,favoring its dephosphorylation and inactivation.

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REFERENCES

Lehninger’s principles of Biochemistry by David L. Nelson and Michael M. Cox

www.wikipedia.org Britannica Online Encyclopaedia

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