Buffered Glucose HiVeg™ Broth, Granulated (Glucose Phosphate HiVeg™ Broth, Granulated) (MR-VP HiVeg™ Medium, Granulated)

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GMV070
For studying Methyl Red and Voges Proskauer tests to differentiate amongst coli-aerogenes group.


Composition**

Ingredients Gms / Litre
Buffered HiVeg peptone 7.000
Dextrose 5.000
Dipotassium phosphate 5.000
Final pH (at 25°C) 6.9±0.2

**Formula adjusted, standardized to suit performance parameters

Directions

Suspend 17 grams in 1000 ml of distilled water. Heat, if necessary to disslove the medium completely. Distribute in test tubes in 10 ml amounts or as desired and sterilize by autoclaving at 15 lbs pressure (121°C) for 15 minutes.

Principle And Interpretation

Buffered Glucose HiVeg Broth is prepared by using vegetable peptones in place of animal peptones which is free from BSE/ TSE risks. Methyl Red and Voges-Proskauer test are among the two various tests used in the biochemical identification of bacterial species. These tests were originally studied by Voges, Proskauer (1) and subsequently by Clark and Lubs (2) to differentiate between members of the coli- aerogenes group. Both the tests are based on the detection of specific breakdown products of carbohydrate metabolism. All members of Enterobacteriaceae are, by definition, glucose fermenters. In MR-VP Broth, after 18-24 hours of incubation, fermentation produces acidic metabolic byproducts. Therefore initially all enterics will give a positive MR reaction if tested (3-5). However, after further incubation, required by the test procedure (2-5 days), MR - positive organisms continue to produce acids, resulting in a low pH (acidic) that overcomes the phosphate buffering system and maintain an acidic environment in the medium (pH 4.2 or less). MR-negative organisms further metabolize the initial fermentation products by decarboxylation to produce neutral acetyl methylcarbinol (acetoin), which results in decreased acidity in the medium and raises the pH towards neutrality (pH 6.0 or above) (6). In the presence of atmospheric oxygen and alkali, the neutral end products, acetoin and 2, 3-butanediol, are oxidized to diacetyl, which react with creatine to produce a red colour. The Methyl Red (MR) test is performed after 5 days of incubation at 30°C (7,8). The Voges-Proskauer test (VP) cultures are incubated at 30°C for 24-48 hours (9). Various test procedures have been suggested for performing the VP test by Werkman, OMeara (7) Levine, et al and Voughn et al. Werkmans Test: Add 2 drops of a 2% solution of ferric chloride to 50 ml culture and 5 ml of 10% sodium hydroxide. Shake the tube to mix well. Stable copper colour developing in a few minutes is positive reaction. OMeara Test: Add 25 mg of solid creatine to 5 ml culture and then add 5 ml concentrated (40%) sodium hydroxide. Red colour development in a few minutes after shaking the tube well is a positive reaction. Levine, Epstein and Voughn modified OMeara technique by dissolving the creatine in a concentrated solution of potassium hydroxide (R031, OMeara Reagent). Voughn, Mitchell and Levine recommended the method of Barritt as, addition of 1 ml of Barritt Reagent B (R030 - 40% potassium hydroxide) and 3 ml of Barritt Reagent A (R029 - 5% α-naphthol in absolute ethanol) to 5 ml culture. Positive test is indicated by eosin pink colour within 2-5 minutes. The MR and VP tests should not be relied upon as the only means of differentiating from the groups. Also occasionally a known acetoin-positive organism fails to give a positive VP reaction. To overcome this possibility, gently heat the culture containing the VP reagents.

Quality Control

Appearance
Cream to yellow coloured granular medium

Prepared Medium
Light yellow clear solution in tubes

Reaction

Reaction of 1.7% w/v aqueous solution at 25°C. pH : 6.9±0.2

pH

6.70-7.10

Cultural Response

Cultural characteristics observed after an incubation at 30°C for 48 hours.

Organism Growth MR Test VP Test
Enterobacter aerogenes ATCC 13048 luxuriant Negative reaction, yellow colour Positive reaction, eosin pink / red colour within 2-5 minutes
Escherichia coli ATCC 25922 luxuriant Positive reaction, bright red colour Negative reaction, no colour change
Klebsiella pneumoniae ATCC 23357 luxuriant Negative reaction, yellow colour Positive reaction, eosin pink / red colour within 2-5 minutes

Storage and Shelf Life

Store below 30°C in tightly closed container and the prepared medium at 2 -8°C. Use before expiry date on the label.

More Information
Product Name Buffered Glucose HiVeg™ Broth, Granulated (Glucose Phosphate HiVeg™ Broth, Granulated) (MR-VP HiVeg™ Medium, Granulated)
SKU GMV070
Product Type Granulated
Physical Form Granular
Origin Animal Free (Veg)
Packaging type HDPE
References 1.Voges O. and Proskauer B., 1898, Z. Hyg. Infektionskr., 28:20.
2.Clark W. M. and Lubs H. K., 1915, J. Infect. Dis., 17:160.
3.Barry A. L., Bernsohn K. L., Adams A. B., Thrup L. D., Appl. Microbiol., 1970, 20 (6), 866-870.
4.Branson D., Methods in Clinical Bacteriology, Springerfield, IL: Charles C Thomas, 1972, 32-33.
5.Cowan S. T., Cowan and Stuls Manual for the Identification of Medical Bacteria, 2nd Ed., Cambridge, Cambridge UniversityPress, 1974, 37,48.
6.MacFaddin J. F., 2000, Biochemical tests for Identification of Medical Bacteria, 3rd Ed., Lippincott, Williams and Wilkins,Baltimore.
7.MacFaddin J. F., 1985, Media for Isolation-Cultivation-Identification-Maintenance of Medical Bacteria, Vol. 1, Williamsand Wilkins, Baltimore.
8.Vaughn R. H., Mitchell N. B. and Levine M., 1939, J. Am. Water Works Association, 31:993.9.Ruchhoft C. C., Kallas J. G., Chinn B. and Coulter E. W., 1931, J.Bacteriol., 22 : 125.10.Werkman C. H., 1930, J. Bact., 20: 121.
11.OMeara R. A. Q., 1931, J. Path. Bacteriol., 34 : 401.
12.Levine M., Epstein S. S. and Voughn R. H., 1934, Am. J. Publ. Health, 24: 505.
13.Ewing W. H., 1986, Edwards and Ewings Identification of Enterobacteriaceae, 4th Ed., Elsevier Science Publishing Co.,Inc., New York.
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