Specifications
Proteose peptone 10.000 G/LCasein enzymic hydrolysate 5.000 G/LYeast exctract 5.000 G/LDextrose 10.000 G/LSodium chloride 5.000 G/LSodium thioglycollate 2.000 G/LSodium formaldehyde sulfoxylate 1.000 G/LResazurin 0.002 G/LAgar 15.000 G/LFinal pH (at 25°C) 7.2 ñ 0.2 G/LpH range 7.00 - 7.40Reaction reaction of 3.5% w/v aqueous solution at 25°C pH 7.2 ñ 7.40Directions :Suspend 53 grams in 1000 ml distilled water. Heat to boiling to dissolve the medium completely. Sterilizeby autoclaving at 15 lbs pressure (121°C) for 15 minutes. Cool to 45-50°C. Mix well and pour into sterilePetri plates.Principle :Proteose peptone, casein enzymichydrolysate, yeast extract provides nitrogen, vitamin and amino acids.Dextrose is a carbohydrate source. This medium contains sodium thioglycollate and sodium formaldehydesulphoxylate that provide adequate anaerobiosis, which is indicated by resazurin present in the medium.Resazurin imparts pink colour to the medium in presence of oxygen. Brewer devised this medium for usewith Brewer anaerobic cover to permit surface growth of anaerobes and microaerophiles on agar withoutthe use of anaerobic jar. For best results, use porous tops on the plates containing the medium duringsolidification to obtain a dry surface. After inoculation of the medium, cover with Brewer anaerobic petriplate cover. The sealing ring inside the cover should make a perfect contact with the medium and mustnot be broken before the end of the incubation period.