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CH3COCH3Ê®3I2Ê®4NaOH      CHI3Ê®CH3COONaÊ®3NaIÊ®3H2O
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(3)      15% ÈýÂÈÒÒËá¡£
(4)      10£¥ NaOHÈÜÒº¡£
(5)      10£¥ HClÈÜÒº¡£
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5.0 ml
5.0 ml
0.1mol/L I2-KI
3.0 ml
3.0 ml
3.0 ml
10% NaOH
3.0 ml
3.0 ml
3.0 ml

 

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Experiment 11  Production and Degradation of Ketone Bodies
 
¡¾Purpose¡¿
Understand the production organs and master the method used for production and degradation of ketone bodies measurement.
¡¾Principle¡¿
Within the mitochondria of liver, the excess acetyl-CoA produced during fatty acid β-oxidation is converted to acetoacetate, β-hydroxybutyrate, and acetone, this group of molecules is called the ketone bodies. Liver can not use ketone bodies as an energy source. Only in several tissues out of liver, most notably cardiac and skeletal muscle, ketone bodies are converted to acetyl-CoA, the acetyl-CoA is then oxidated to generate energy .
We use butyric acid as initial stuff in this experiment, the butyric acid is heated with the liver plasm, and then measure the content of ketone bodies in liver plasm. Moreover, measure the content of ketone bodies under the condition of coexistence of liver plasm and skeletal muscle in reaction system. We can comprehend the above theories from the difference of the ketone bodies content under the two different conditions. We determine the content of acetone in this experiment.
The ketone bodies measurement principle is shown below: In alkaline aqua the iodine can oxidize acetone to become iodoform , titrate the remainder iodine in the reaction system with hyposulphite, we can calculate the consumption of iodine according to the result of hyposulphite titration, we can also calculate the content of ketone bodies (take acetone as to represent) according to the titration result.The equation of Reaction is as follows:
CH3COCH3Ê®3I2Ê®4NaOH      CHI3Ê®CH3COONaÊ®3NaIÊ®3H2O
I2Ê®2Na2S2O3      Na2S4O6Ê®2NaI
¡¾Materials¡¿
1. Apparatus:
Tubes, Pipets, Flasks Burettes and burette support.
2. Reagents:
(1)    0.1% aqua of starch.
(2)    0.9% aqua of NaCl.
(3)    15% trichlorine acetic acid.
(4)    10% aqua of NaOH.
(5)    10% aqua of HCl.
(6) 0.5mol/L butyric acid: Dissolve 5ml butyric acid in 100ml 0.5mol/L NaOH.
¢Ë         0.1mol/L aqua of iodine: Dissolve I2 12.5g and KI 25g in distilled water, dilute the solution to 1L, demarcate the solution with 0.1mol/L Na2S2O3.
¢Ì         0.02 mol/L Na2S2O3: Dissolve 24.82 g Na2S2O3 · 5 H2O and 400 mg anhydrous Na2CO3 in 1L fresh boiled water to get 0.1 mol/L solution, demarcate the solution with 0.1 mol/L KIO3. Dilute the solution to 0.02 mol/L just before using.
¡¾Procedures¡¿
1. Preparation of the specimen:
Execute the rabbit, take out the liver, scour off the blood with 0.9% NaCl, put the liver on filter paper to suck away the surface humidity, weigh 5 g of the liver organize, place it into the mortar, add a few 0.9% NaCl to total volume 10 ml. Then take 5 g muscle of rear leg, make it into the liver organization plasm according to above- mentioned method and comparisons.
2. Heat preservation and precipitation of the protein:
Take three tubes, number the tubes and operate as the table followed£º
 

 

Tube No.
Reagent
A
B
C
The liver organization plasm
2.0 ml
2.0 ml
The liver organizationn plasm that boiled in advance
2.0 ml
Phosphoric acid salt buffer liquid of pH7.6
4.0 ml
4.0 ml
4.0 ml
orthobutyric acid
2.0 ml
2.0 ml
2.0 ml

 

Heat preservation at 43¡æ water bath for 60 minutes.

 

The muscle organization plasm
4.0 ml
The muscle organization plasm that boiled in advance
4.0 ml
4.0 ml

 

Heat preservation at 43¡æ water bath for 60 minutes.

 

15% trichlorine acetic acid
3.0 ml
3.0 ml
3.0 ml

 

 
Filter with the filter paper after shaking evenly, collect the filtrate respectively in 3 tubes, then we get the filtrate without protein.
3. Determination of the ketone bodies
Take 3 flasks, operate as below-mentioned serial number in proper order: 

 

                 Flask No
Reagent
1
2
3
Filtrate without protein
5.0 ml
5.0 ml
5.0 ml
0.1mol/L I2-KI
3.0 ml
3.0 ml
3.0 ml
10% NaOH
3.0 ml
3.0 ml
3.0 ml

 

Place Statically for 10 minutes after shaking evenly, add 10% HCl 3ml to each tube, and add one drop of 1% starch liquid to each tube, then we can see the solution presents the color of orchid, titrate with 0.02mol/L Na2S2O3 until the solution presents the color of bright green respectively.
¡¾Result and calculation¡¿
Ketone bodies produced in liver( mmol/g)=(C£­A)×Moore content of the Na2S2O3 ×1/6
Ketone bodies consumed in muscle ( mmol/g)=(C£­B)×Moore content of the Na2S2O3 ×1/6
A: volume of the Na2S2O3 (ml) consumed during titration of sample 1 
B: volume of the Na2S2O3 (ml) consumed during titration of sample 2
C: volume of the Na2S2O3 (ml) consumed during titration of sample£³
¡¾Advisement after experiment¡¿
Ketone bodies are oxidated to generate energy only in several tissues out of liver. Why?
±à¼­£ºsongjiajie2010

 
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