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Principle:

The nitrate reduction test, which measures enzyme activity, is a key element in differentiating M. tuberculosis from other tubercle bacilli.

Nitrate reductase enzyme converts nitrate into nitrite, which is detected by a colourimetric test. M. tuberculosis exhibits strong nitrate reduction activity, whereas M. bovis gives a negative or weak reaction; M. Africanum strains are usually negative, but approximately 20% of strains give a positive test reaction.

The test must be carried out on pure cultures otherwise it will yield false results.

Reagents and Solutions:

Note: Discard any reagent if the colour changes or a precipitate forms.

1. Sodium nitrate substrate in buffer, pH 7

Sodium nitrate (NaNO3)                                                                          0.085 g

Potassium dihydrogen phosphate (KH2PO4)                                          0.117 g

Disodium hydrogen phosphate dodecahydrate (Na2HPO4.12H2O)                        0.485 g

Distilled water                                                                                          100 ml

Check pH using a pH meter. Then, sterilize by autoclaving at 121°C for 15 minutes. 

2 ml aliquots of the substrate solution are aseptically dispensed into sterile screw-cap tubes when needed.

2.  Reagent 1: Hydrochloric acid solution

Concentrated hydrochloric acid (HCl, 36%)                                            10 ml

Distilled water                                                                                          10 ml

Add concentrated HCI slowly to distilled water.

3.  Reagent 2: Sulfanilamide solution, 0.2%

Sulfanilamide  (C6H8N2O2S)                                                                   0.2 g            

Distilled water                                                                                          100 ml

Dissolve sulfanilamide in distilled water and store it in an amber bottle in the dark in a refrigerator.

4.  Reagent 3: N-naphthylethylene diamine solution, 0.1%

N-naphthylethylene diamine dihydrochloride                                          0.1 g

Distilled water                                                                                          100 ml

Dissolve N-naphthylethylene diamine in distilled water.

Store in an amber bottle in the dark in a refrigerator.

Procedure:

The entire procedure must be carried out in a biological safety cabinet.

  1. Add 0.2 ml of distilled water to a 16 x 100 mm screw-cap tube.

  2. Take 2 loopful of colonies from positive culture and emulsify in water. 

  3. Add 2.0 ml of NaNO3 substrate to the tube and mix well.

  4. Place in the water bath at 37 °C for 2 hours.

  5. Remove the tube from the water bath.

  6. Add 1 drop of reagent 1, 2 drops of reagent 2, and 2 drops of reagent 3.

  7. Examine immediately for the development of a pink to red colour.

Result and interpretation:

Pink colour  = positive result

No colour     = negative result

Add a small amount of zinc powder to all negative tests:

  • If nitrate is still present, it will be reduced by the zinc powder, and the colour will turn red (true negative). 

  • If no colour develops the original reaction was positive, but nitrate was reduced beyond nitrite.

  • Resource

    Standard Operating Procedures (Nitrate Reduction Test).

    Assessment

Question 1

Answer 1

Answer 2

Answer 3

Answer 4

Correct Answer

Correct Explanation

Page id

Part of Pre-Test

Part of Post-Test

 M. tuberculosis exhibits strong nitrate reduction activity.

True

False

 

 

True

A strong nitrate reduction activity is a key element in differentiating, a M. tuberculosis from other tubercle bacilli.

 

Yes

Yes

Question 2

 

 

 

 

 

 

 

 

 

Development of pink colour in Nitrate Reduction Test indicates a positive reaction.

True

False

 

 

True

The development of pink colour in Nitrate Reduction Test indicates the positive reactionTest.

 

Yes

Yes

 

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