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This is a selective medium for the isolation of Staphylococcus and Streptococcus spp. Based on Columbia Agar, it is enriched by the addition of Sheep Blood (7%) the medium is also made selective by the inclusion of Colistin and Naladixic Acid to suppress the growth of the majority of Gram negative bacteria. The addition of sheep blood the medium allows for good colonial appearance, pigment production and excellent haemolysis from beta-haemolytic streptococci. -
Columbia Blood Agar with 5% Defibrinated Horse Blood & Cap Selective Supplement This is a medium for the selective isolation of Staphylococcus spp. and Streptococcus spp. primarily from clinical specimens. Based on Columbia Agar Base enriched with 5% Horse Blood the medium is made selective by the inclusion of Colistin and Aztreonam to suppress the growth of the majority of Gram negative bacteria. -
Side 1: Columbia Agar with 5% Horse Blood This is a general-purpose medium enriched with 5% defibrinated horse blood that is suitable for the isolation of most organisms, including many fastidious anaerobes. Side 2: Columbia Agar with 5% Horse Blood and CAP Selective Supplement This is a medium for the selective isolation of Staphylococcus spp. and Streptococcus spp. primarily from clinical specimens. Based on Columbia Agar Base enriched with 5% horse blood the medium is made selective by the inclusion of colistin and aztreonam to suppress the growth of the majority of Gram-negative bacteria. -
Side 1 – Columbia Agar w 5% Horse Blood This is a general-purpose medium with 5% defibrinated horse blood suitable for isolation of most organisms including fastidious anaerobes. Side 2- Chocolate Agar w 5% Horse Blood This is a highly nutritious medium supplemented with defibrinated horse blood and chocolated by heating to 70°C for 5 minutes. It will support the growth of a wide range of pathogens including the most fastidious organisms and is particularly useful for the cultivation of Haemophilus spp. and Neisseria spp -
Side 1: Columbia Blood Agar with 7% Sheep Blood & CNA Supplement This is a selective medium for the isolation of Staphylococcus and Streptococcus spp. Based on columbia agar, it is enriched by the addition of sheep blood (7%) the medium is also made selective by the inclusion of colistin and nalidixic acid to suppress the growth of the majority of Gram negative bacteria. The addition of sheep blood to the medium allows for good colonial appearance, pigment production and excellent haemolysis from beta-haemolytic streptococci. Side 2: Sabouraud Dextrose Agar with Chloramphenicol A selective medium for the isolation of yeasts and fungi. Sabouraud dextrose agar is suitable for use in all areas of Mycology. The low pH of the medium inhibits most bacteria, however in this formulation chloramphenicol (150mg/L) is added to further reduce the risk when processing material that may be heavily contaminated particularly with coliforms. -
This is a selective medium for the cultivation of Taylorella equigenitalis or the contagious equine metritis organism (CEMO) that is the etiological agent for contagious equine metritis. Enzymatic digest of casein and soy peptone provide the required nitrogen, carbon and vitamins, and sodium chloride maintains the osmotic balance of the medium. Sodium sulphite is a reducing agent and L-cystine is an essential amino acid. In addition to this, the medium is further enriched by the inclusion of 7% chocolated horse blood. Amphotericin B is added to suppress the growth of contaminating fungi and yeasts and both clindamycin and trimethoprim are added to suppress bacterial contaminants. -
This is a selective medium for the cultivation of Taylorella equigenitalis or the contagious equine metritis organism (CEMO) that is the etiological agent for contagious equine metritis. Enzymatic digest of casein and soy peptone provide the required nitrogen, carbon and vitamins, and sodium chloride maintains the osmotic balance of the medium. Sodium sulphite is a reducing agent and L-cystine is an essential amino acid. In addition to this, the medium is further enriched by the inclusion of 7% chocolated horse blood. Amphotericin B is added to suppress the growth of contaminating fungi and yeasts. -
This is a selective medium for the cultivation of Taylorella equigenitalis or the contagious equine metritis organism (CEMO) that is the etiological agent for contagious equine metritis. Enzymatic digest of casein and soy peptone provide the required nitrogen, carbon and vitamins, and sodium chloride maintains the osmotic balance of the medium. Sodium sulphite is a reducing agent and L-cystine is an essential amino acid. In addition to this, the medium is further enriched by the inclusion of 7% chocolated horse blood. Amphotericin B and streptomycin are added to suppress the growth of fungal/yeast and bacterial contaminants, respectively. -
Dermatophyte Test Medium with Chloramphenicol & Cyclohexamide (Actidione) This is a selective medium for the isolation of dermatophytes that includes a Phenol Red indicator to assist in the differentiation between dermatophytes and other pathogenic fungi. Although the low pH (5.5) of the medium inhibits most bacteria, Chloramphenicol is added to further reduce the risk when processing material that may be more heavily contaminated. Cyclohexamide (Actidione) is also added to suppress the growth of most yeasts and saprophytic fungi. Dermatophytes appear as fluffy white colonies and produce a red colour on the medium while other fungi cause the medium to become yellow due to acid production. Yeasts will also grow on this medium but are readily distinguished by their distinct white/creamy colonies and distinctive smell. NB: Prolonged incubation should be avoided as this may cause fungi other than dermatophytes to turn the medium red -
Desoxycholate Citrate Agar (DCA) (Hynes) One of several media designed for the differential selective isolation of Salmonella and Shigella spp from clinical and environmental samples. Lactose is added to the medium together with Neutral Red indicator to assist in the differentiation of Lactose and Non-Lactose fermenting organisms. The medium is made selective by the inclusion of Sodium Desoxycholate and Sodium Thiosulphate, which will inhibit most gram-positive organisms. The Sodium Thiosulphate is also broken down by the enzyme thiosulphate reductase to form Sodium Sulphite and Hydrogen Sulphide. The Hydrogen Sulphide, if present, will in turn react with the ferric ions to produce a black precipitate of Ferrous Sulphide and give rise to the classical black centre of most Salmonellae. It has been suggested that this medium may be more suitable for secondary post-enrichment isolation while the original formulation is more appropriate for the primary inoculation of samples. -
DN'ase Medium DNase Agar is used primarily in clinical laboratories to differentiate Staphylococcus aureus from other Staphylococci based on deoxyribonuclease activity. Following incubation of the plate and confirmation of a pure growth of Staphylococci, the surface of the medium is covered with a small quantity of 1M Hydrochloric Acid to precipitate the DNA. Staphylococcus aureus produce DNase enzymes that hydrolyse DNA resulting in a clear area around the colonies, described as being DNase positive, whereas coagulase negative Staphylococci do not produce clearing. NB: As with most tests of this type a positive result should not be taken in isolation and other appropriate tests, e.g. Coagulase Test, Latex Agglutination etc, should be carried out. -
DNase Agar is used primarily in clinical laboratories to differentiate Staphylococcus aureus from other staphylococci based on deoxyribonuclease activity. Staphylococcus aureus produce DNase enzymes that hydrolyse DNA resulting in a colourless zone around the colonies, described as being DNase positive, whereas coagulase negative staphylococci do not produce clearing. This particular formulation can also be used for Streptococci and Serratia. NB: As with most tests of this type a positive result should not be taken in isolation and other appropriate tests, e.g. Coagulase Test, Latex Agglutination etc, should be carried out. -
Edwards Medium (Modified) with 7% Sheep Blood This is a medium for the selective isolation of streptococci, particularly Streptococcus agalactiae, involved in bovine mastitis. The medium is enriched by the addition of 7% Sheep Blood and made selective by the inclusion of Crystal Violet and Thallous Sulphate. Aesculin is also present and assists in the differentiation of Streptococcus agalactiae, which give rise to blue colonies, from Aesculin positive Group D streptococci which produce black colonies. -
Fastidious Anaerobe Agar is intended as a primary isolation medium capable of supporting most clinically significant anaerobes including fastidious organisms. The formulation is complex and includes detoxification agents (Starch & Sodium Bicarbonate), growth enhancing agents (Cysteine, Arginine, Vitamin K, Sodium Succinate, Glucose and pyrophosphate) as well as Haemin to encourage pigment production in Porphyromonas melaninogenicus. Sodium Pyruvate is also included to help neutralise Hydrogen Peroxide. One side of the bi-plate consists of standard FAA supplemented with 7% horse blood; the other side is FAA with horse blood and Neomycin (75mg/L) for the selective isolation of target organisms. -
Fastidious Anaerobe Agar (FAA) with 5% Sheep Blood Fastidious Anaerobe Agar is intended as a primary isolation medium capable of supporting most clinically significant anaerobes including fastidious organisms. The formulation is complex and includes detoxification agents (Starch & Sodium Bicarbonate) growth enhancing agents (Cysteine, Arginine, Vitamin K, Sodium Succinate, Glucose and pyrophosphate) as well as Haemin to encourage pigment production in Porphyromonas melaninogenicus. Sodium Pyruvate is also included to help neutralise Hydrogen Peroxide. In this instance the medium is further enriched by the addition of 5% Sheep Blood. -
Fastidious Anaerobe Agar is intended as a primary isolation medium capable of supporting most clinically significant anaerobes including fastidious organisms. The formulation is complex and includes detoxification agents (starch and sodium bicarbonate), growth enhancing agents (cysteine, arginine, vitamin K, sodium succinate, glucose and pyrophosphate), as well as haemin to encourage pigment production in Porphyromonas melaninogenicus. Sodium pyruvate is also included to help neutralise hydrogen peroxide. In this instance the medium is further enriched by the addition of 5% horse blood. This product is suitable for use with the EUCAST disc diffusion method for selected rapidly growing anaerobic bacteria.
