Dehydrated Culture Media

  • Nutrient Broth No.2 is used for the cultivation of fastidious pathogens and other microorganisms. This general use medium, rich in nutrients, allows the growth of bacteria when there is a low level of cells. The medium is particularly suitable as a secondary growth medium for staphylococci to be tested for coagulase production and also be used for sterility testing of aerobic organisms. Beef extract and peptone provide the required carbon, nitrogen and vitamins. Sodium chloride maintains osmotic balance.  
  • O-F Medium is used for the determination of oxidative and fermentative metabolism of carbohydrates by Gram-negative bacilli (1). This is on the basis of the acid reaction in either the open or closed system that has been covered with sterile paraffin oil. Changes in the covered agar are considered to be due to true fermentation, while changes in the open tubes are due to the oxidative utilization of the carbohydrate present. O-F Base Medium requires the addition of the specific carbohydrate being investigated. The enzymatic digest of casein provides the required nitrogen, carbon and vitamins in the media. Sodium chloride maintains the osmotic balance. Di-potassium hydrogen phosphate acts as a buffer and bromothymol blue is a pH indicator. The agar is a solidifying agent. Reference (1) Hugh, R. and Leifson, E.J. 1953. Bacteriol. 66:24-26.
  • Palcam agar is a selective differential medium for the isolation of Listeria monocytogenes from food, clinical and environmental specimens. The Columbia peptone mix and starch provide the required carbon, nitrogen and vitamins. Glucose is a fermentable carbohydrate. Differentiation of Listeria spp. from enterococci and staphylococci occurs through aesculin hydrolysis and mannitol fermentation. Listeria monocytogenes will hydrolyse aesculin and the associated reaction with the ferric ammonium citrate gives rise to a brown/black precipitate around the colonies. Listeria spp. do not however ferment mannitol. Mannitol fermentation is seen through a colour change of the colony or the area around the colony from red to yellow due to the production of acidic end products. Phenol red is the pH indicator in the medium. Lithium chloride is included to inhibit enterococci. The associated Palcam selective supplement, LS0038, contains polymyxin B, acriflavine and ceftazidime to inhibit other Gram-positive and Gram-negative organisms that may be present in specimens. Related Supplements : LS0038 PALCAM Selective Supplement
  • Pasteurella Agar Base is an non-selective medium capable of supporting the growth of Pasteurella spp. Pasteurella spp.are spherical, ovoid or rod-shaped cells 0.3-1.0μm in diameter and 1.0-2.0μm in length. Cells are Gram negative, and occur singly, or in pairs or short chains. Bipolar staining may be seen and capsules may be present. All species are non-motile, and are facultatively anaerobic.(1) With further enrichment using 5-10% blood and selective antimicrobials, most Pasteurella spp. can be isolated. There is no haemolysis on blood agar for Pasteurella spp. and the organism will not regularly exhibit satellitism around colonies of Staphylococcus spp. The peptones act as carbon, nitrogen and vitamin sources in this medium. Sodium chloride maintains the osmotic balance and the agar is a solidifying agent. The medium is made selective through the addition of LS0057, Pasteurella agar selective supplement. REFERENCE (1) Standards Unit, Microbiology Services, PHE. 1995. UK Standards for Microbiology Investigations. Identification of Pasteurella species and Morphologically Similar Organisms. 3, 1-28.
  • KM0149

    Peptone Water

    Peptone water is a general-purpose medium that supports thecultivation of non-fastidious organisms. This non-selective medium can be used a basal medium for biochemical tests such as carbohydrate fermentation and production of indole. Tryptone and peptone act as sources of carbon, nitrogen and vitamins in this medium and sodium chloride maintains osmotic balance.  
  • Perfringens Agar Base is a base medium that allows the enumeration of Clostridium perfringens from food samples. As a base medium, Perfringens Agar Base can have several supplementary and selective agents added to increase selectivity. The addition of Eye Yolk Emulsion (BM0140) allows the detection of lecithinase activity as precipitates are formed by C. perfringens. The addition of D-cycloserine (LS0023) can be used to inhibit other facultative anaerobes, as used in Tryptose-Sulphite-Cycloserine (TSC) agar. (1&2) Alternately, kanamycin and polymyxin B (LS0025) can be used to inhibit other coliforms generally found in food samples, as used in Shahidi-Ferguson Perfringens (SFP) agar.(3) The tryptose and soy peptone provide the required nitrogen, carbon and minerals. Yeast extract provide the essential vitamins, including the vitamin B group, needed for growth. The ferric ammonium citrate and sodium metabisulphite allows the reduction of sulphites to hydrogen sulphide by C. perfringens, which produces black colonies. References (1) ISO- 7937:2004. Microbiology of food and animal feeding stuffs- Horizontal method for the enumeration of Clostridium perfringens - Colony count technique (2) Harmon, S.M., Kauttar, D.A. and Peeler, J.T. 1971. Improved Medium for Enumeration of Clostridium perfringens. Appl. Microbiol. 22:688-692. (3) Shahidi S. A. and Ferguson A. R. 1971 New Quantitative, Qualitative, and Confirmatory Media for Rapid Analysis of Food for Clostridium perfringens. Appl. Microbiol. 21:500-506
  • Phosphate-buffered saline (PBS) is a buffer solution used in biological research. It is a water-based salt solution containing sodium phosphate, sodium chloride and, in some formulations, it contains potassium chloride and potassium phosphate. The osmolality and ion concentrations of the solutions match those of the human body (isotonic) and are non-toxic to most cells. This balanced salt solution is issued to meet the requirements of those tissue culture workers who use the Dulbecco Solution with and without calcium and magnesium.
  • Plate Count Agar is formulated to the A.P.H.A. specification developed by Buchbinder et al. This medium is intended for use in food, dairy and water bacteriology to perform Total Viable Counts. Tryptone and yeast extract provide the required carbon, nitrogen and vitamins. Glucose is a fermentable carbohydrate.  
  • Potato dextrose agar is recommended for the detection and enumeration of yeasts and moulds in food and dairy products.It can also be used for the cultivation of fungi although with the prolonged incubation necessary cultures may become overgrown by bacteria. The low pH (5.6) suppresses the growth of most bacteria and the low mineral content ensures good pigment production by fungi where appropriate. This medium meets the requirements of the Harmonised USP/EP/JP.(1,2&3) REFERENCES (1) United States Pharmacopeial Convention. 2007. The United States pharmacopeia, 31st ed., Amended Chapters 61, 62, 111. The United States Pharmacopeial Convention, Rockville, MD. (2) Directorate for the Quality of Medicines of the Council of Europe (EDQM). 2007. The European Pharmacopoeia, Amended Chapters 2.6.12, 2.6.13, 5.1.4, Council of Europe, 67075 Strasbourg Cedex, France. (3) Japanese Pharmacopoeia. 2007. Society of Japanese Pharmacopoeia. Amended Chapters 35.1, 35.2, 7. The Minister of Health, Labor, and Welfare.
  • Primary Membrane Lactose Glucuronide Agar (mLGA) is used for the differentiation and enumeration of Escherichia coli and other coliforms through a single membrane filtration technique. The peptone and yeast extract provide the required nitrogen, carbon and vitamins. Sodium pyruvate protects injured cells enhancing recovery and growth of coliforms. Sodium lauryl sulphate is a selective agent that inhibits Gram-positive organisms. Lactose is a fermentable carbohydrate and phenol red is a pH indicator. Lactose fermentation will result in yellow colonies. X-glucuronide is a chromogenic substrate which can be cleaved by the enzyme ß-glucuronidase present in E. coli. This results in a blue colony, but in combination with lactose fermentations colonies will appear green. NB: Prepared plates stored at 2–8°C may show formation of surface crystals which will disappear when plates are warmed to >20°C Related Supplements :
  • Recent developments in culture media have given rise to the use of chromogenic substrates as a means of differentiating bacteria particularly among the coliform group of organisms. This is one such medium and has been developed with the aim of simplifying the differentiation and presumptive identification of the main organisms usually found in Urinary Tract Infections (UTI). The peptone is the source of the required nitrogen, carbon and vitamins. Based on the traditional CLED medium, to prevent the swarming of Proteus spp., two chromogens are present in the medium. One allows the detection of enterococci giving rise to blue colonies whilst the second results in purple colonies of E. coli. Phenylalanine and tryptophan are also included as indicators of tryptophan deaminase activity producing brown colonies of Proteus spp. Related Supplements : SHS500 Sterile Horse Serum 500ml
  • This is a selective medium for the isolation of Pseudomonas spp. primarily in food, water and environmental samples. Pseudomonas agar base is on Kings A medium which uses magnesium and potassium salts to enhance pigment production. The gelatine peptone and acid hydrolysed casein acts as a nitrogen, vitamins, and carbon source. Magnesium chloride and potassium sulphate promotes production of pyocyanin. The medium can be made selective for P. aeruginosa by the addition of Pseudomonas CN Supplement (LS0006). Alternatively, the medium can be made selective for Pseudomonas spp. generally by the addition of Pseudomonas CFC Selective Supplement (LS0026). The presence of blue/green or brown pigmentation or fluorescence is indicative of presumptive Pseudomonas spp. It should be noted however that further testing must be carried out to confirm the full identity of the organism.
  • KM0082

    R2A Agar

    R2A agar is used for the enumeration and cultivation of bacteria from drinking water. R2A agar developed by Reasoner and Geldreich is a low nutrient medium that can used in pour plate, spread plate, and membrane filtration methods for heterotrophic plate counts. In combination with a lower incubation temperature and longer incubation period R2A agar stimulates the growth of stressed and chlorine-tolerant bacteria. Traditionally nutritionally rich media have been used for this purpose but these media support the growth of fast-growing bacteria and may suppress slow growing or stressed bacteria found in treated water. Enzymatic digest of casein, proteose peptone, acid hydrolysate of casein and yeast extract provide the required nitrogen, carbon and vitamins. Glucose is a fermentable carbohydrate. Dipotassium hydrogen phosphate is a buffering agent. Magnesium sulphate is a source of divalent cations and sulphate. Starch and sodium pyruvate aid in the recovery of stressed organisms.  
  • Rappaport-Vassiliadis (MSRV) Medium Semi-Solid is a modification of Rappaport-Vassiliadis Soy Broth for detecting motile Salmonella spp. in faeces and food products.[1] The original research on MSRV Medium revealed a semi-solid could be used as a rapid and sensitive test for isolating motile Salmonella spp. from food products following pre-enrichment or selective enrichment.[2] The semi-solid medium allows motility to be detected as halos of turbid growth around the original point of inoculation. The peptones are to provide vitamins, nutrients and nitrogen to encourage growth of Salmonella spp. The salt maintains the osmotic balance and potassium dihydrogen phosphate is a buffer for stabilising the pH of the medium. Malachite green is included as a selective agent that inhibits Gram-positive organisms and some Gram-negative organisms. References (1) ISO 6579-1:2017. Microbiology of the food chain – Horizontal method for the detection, enumeration and serotyping of Salmonella – Part 1: Detection of Salmonella spp. (2) De Smedt J.M., Bolderdikj R., Rappold H. and Lautenschlaeger D. 1986. Rapid Salmonella Detection in Foods by Motility Enrichment on a Modified Semi-Solid Rappaport-Vassiliadis Medium. J. Food Prot. 49:510-514
  • Rappaport-Vassiliadis Soya Broth is used for the enrichment and selective isolation of Salmonella spp. This medium is a modification of the original formulation by Rappaport et al. and has been formulated to exploit the full characteristics of Salmonella spp. These characteristics include the ability to survive at relatively high osmotic pressure, to multiply at low pH values and greater resistance to malachite green. This formulation also has the correct amount of magnesium chloride as previous formulations did not take into account the volume of displacement caused by dissolving large amounts of magnesium chloride in water. This formulation has been shown to be superior to tetrathionate broth and selenite broth for the isolation of Salmonella spp. from meat products. Soya peptone provides the required carbon, nitrogen and vitamins. Potassium dihydrogen phosphate and di-potassium hydrogen phosphate act as buffers. Magnesium chloride raises the osmotic pressure in the medium. Malachite green is an inhibitory substance. NB: This formulation is very hygroscopic and will produce a slight exothermic reaction when mixed with water.  
  • Sabouraud Dextrose Agar is one of several media available for theisolation of yeasts and fungi suitable for use in all areas of mycology. Sabouraud Dextrose Agar is a modification of a medium originally described by Sabouraud. The tryptone and meat peptone provide the nitrogen and vitamins required for organism growth in Sabouraud Dextrose Agar. The high concentration of dextrose is included as an energy source and in tandem with the acidic pH (5.6) facilitates the growth of fungi whilst providing limited selective properties. Higher levels of selectivity can be achieved against bacterial species by the addition of chloramphenicol. NB: This is a basic medium only and contains no additional supplements. Related Supplements : LS0050 Chloramphenicol Selective Supplement