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KM0003 Sabouraud Dextrose Agar powder is a general-purpose, non-selective medium which is used for the isolation of yeasts and moulds from clinical, food, pharmaceutical and cosmetic samples. Sabouraud Dextrose Agar is a modification of a medium originally described by Sabouraud. The fungi maintain their typical cultural appearance and thus may be readily identified according to the standard macroscopic characters described by Sabouraud. The formulation conforms to European, United States and Japanese Pharmacopeia requirements. This medium complies with ISO 11133:2014, where it is described as the main reference medium to carry out quantitative testing on culture media intended for fungi. Sabouraud Dextrose Agar is recommended by the UK Standards for Microbiology Investigations for various purposes, including as a standard, supplementary or optional medium. Related Supplements : LS0050 Chloramphenicol Selective Supplement -
This is a selective medium for the isolation of yeasts and fungi and is particularly suitable for use in sterility testing. The low pH (5.6) of the medium is inhibitory to most bacteria and many diagnostic features such as spores and pigmentation are well developed on this medium. The formulation of this medium conforms to the requirements of the Harmonized USP/EP/JP. -
This is a selective medium for the isolation of yeasts and fungi and is particularly suitable for use in sterility testing. The low pH (5.6) of the medium is inhibitory to most bacteria and many diagnostic features such as spores and pigmentation are well developed on this medium. The formulation of this medium conforms to the requirements of the United States Pharmacopoeia & European Pharmacopoeia. This product is wrapped in barrier film to allow for use in Vaporised Hydrogen peroxide sterilisation systems. NB: Final sterilisation of this medium is by Gamma irradiation and it is triple wrapped. Dose Range: Min: 8.0kGy Max: 15.0kGy -
Sabouraud Dextrose Agar with Chloramphenicol (150mg/L) 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. -
Sabouraud Dextrose Agar with Chloramphenicol (50mg/L) & Cyclohexamide (Actidione) (300mg/L) A selective medium for the isolation of 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 (50mg/L) is added to further reduce the risk when processing material that may be heavily contaminated particularly with coliforms. Cycloheximide is also added to suppress the growth of yeasts and saprophytic fungi. -
This is a selective medium for the isolation of yeasts and fungi and is particularly suitable for use in sterility testing. The low pH (5.6) of the medium is inhibitory to most bacteria and many diagnostic features such as spores and pigmentation are well developed on this medium. The formulation of this medium conforms to the requirements of the United States Pharmacopoeia. Lecithin & Polysorbate 80 (Tween 80) are added to inactivate surface disinfectants (Lecithin neutralises quaternary ammonium compounds & Tween neutralises phenols, formalin, hexachlorophene and in combination with the Lecithin ethanol). NB: Final sterilisation of this medium is by Gamma irradiation and it is triple wrapped. Dose Range: Min: 8.0kGy Max: 15.0kGy
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Sabouraud Dextrose Agar with Lecithin, Tween 80, Histidine & Sodium Thiosulphate (VHP) (USP) - Irradiated This is a selective medium for the isolation of yeasts and fungi and is particularly suitable for use in sterility testing. The low pH (5.6) of the medium is inhibitory to most bacteria and many diagnostic features such as spores and pigmentation are well developed on this medium. The formulation of this medium conforms to the requirements of the United States Pharmacopoeia. Lecithin, Polysorbate 80 (Tween 80), Histidine and Sodium Thiosulphate are added to inactivate surface disinfectants (Lecithin neutralises quaternary ammonium compounds, Tween 80 and Histidine neutralises phenols, formalin, hexachlorophene and in combination with the Lecithin ethanol and Sodium Thiosulphate inactivate mercurials). This product is wrapped in barrier film to allow for use in Vaporised Hydrogen peroxide sterilisation systems. NB: Final sterilisation of this medium is by Gamma irradiation and it is triple wrapped. Dose Range: Min: 8.0kGy Max: 15.0kGy
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Sabouraud liquid medium USP is used in sterility testing for the detection of moulds, yeasts and acidophilic microorganisms in pharmaceutical products. This medium is also used for non-sterile testing and for the determination of fungistatic activity. Sabouraud liquid medium USP conforms to the USP and Harmonised Pharmacopeia. The peptic digest of animal tissue and pancreatic digest of casein provides the required nitrogen, carbon and vitamins. 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.
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Saline (0.45%) is suitable for use in preparation of food samples and/or as a rinse fluid during examination of equipment etc. prior to culture. It can also be used as a general purpose diluent in many areas of the laboratory. -
Saline (0.85%) is suitable for use in preparation of food samples and/or as a rinse fluid during examination of equipment etc. prior to culture. It can also be used as a general purpose diluent in many areas of the laboratory. -
Saline (0.9%) is suitable for use in preparation of food samples and/or as a rinse fluid during examination of equipment etc. prior to culture. It can also be used as a general purpose diluent in many areas of the laboratory. -
This is a selective medium for the isolation of Salmonella spp. and Shigella spp. from clinical specimens and food samples. SS agar is a modification of the original DCA medium described by Leifson. The formulation for SS agar was later modified to improve the growth of Shigella spp. SS agar modified differs from SS agar in that it has an alternation to the bile salts mixture, peptone, pH value, and total g/litre. The peptone provides the required carbon, nitrogen and vitamins. Lactose is a fermentable carbohydrate and neutral red is a pH indicator. Sodium thiosulphate and ferric citrate are used to detect hydrogen sulphide production indicated by the black centred colonies of hydrogen sulphite positive organisms. Bile salts, sodium citrate and brilliant green inhibit Gram-positive bacteria and a number of different coliform bacteria.
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Selenite cystine broth is a modification of selenite F broth and is for the selective enrichment of Salmonellae spp. from clinical, food and environmental specimens. The peptone acts as a nitrogen, carbon and vitamin source. Lactose is a fermentable carbohydrate and sodium phosphate is a buffer. L-cystine is used to enhance the recovery of Salmonellae spp. in low numbers. The medium is made selective by the addition of sodium biselenite (KM8021). Following overnight incubation subculture(s) are usually made on to one or more of the many selective enteric solid media.
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A medium for the selective enrichment of Salmonellae spp from both clinical and food samples. It is a buffered Lactose Peptone Broth to which Sodium Biselenite is added as the selective agent and Cystine to enhance the recovery of salmonella in low numbers. Subcultures should be made from the top 1/3 of the broth after not more than 24 hours incubation as after this time there is a loss of selectivity. -
BM0360 Selenite F Broth is a medium for the selective enrichment of Salmonella spp. from both clinical and food samples. Following overnight incubation subculture(s) are usually made on to one or more of the many selective enteric solid media. Selenite F Broth is also recommended by the American Public Health Association (APHA) for the examination of food. Subcultures should be made from the top 1/3 of the broth after not more than 24 hours incubation as after this time there is a loss of selectivity. -
Developed by Leifson, selenite F broth is a medium for the selective enrichment of Salmonella spp. from both clinical and food samples. The peptone acts as a nitrogen, carbon and vitamin source. Lactose is a fermentable carbohydrate and sodium phosphate is a buffer. The medium is made selective by the addition of sodium biselenite (KM8021). Following overnight incubation subculture(s) are usually made on to one or more of the many selective enteric solid media.
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Sheep Blood Agar Base has been developed to provide a nutrient rich medium compatible with sheep blood for the cultivation of many bacteria, especially fastidious Streptococcus spp., without affecting haemolytic reactions. Alternative culture mediums, such as Blood agar base No. 2, can results in mixed haemolytic reactions for some Streptococcus spp. This is thought to occur due to the trace amounts of fermentable carbohydrates in yeast extract and the physiological difference between sheep and horse blood. The tryptone, peptone, and yeast extract provide the required nitrogen, carbon and vitamins in the medium. Sodium chloride maintains the osmotic balance. Related Supplements : LS0008 Staph/Strep Selective Supplement
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This medium can be used as a screening method for the differentiation of Enterobacteriaceae based on the ability of some species to utilise citrate as a sole source of carbon. It is often used as a screening test for Klebsiella pneumoniae (Positive reaction) while Escherichia coli is negative. Other uses included distinguishing between species of citrate positive Salmonellae (e.g. Salmonella enteritidis) and those that are negative (e.g. Salmonella typhi and Salmonella paratyphi A). The medium is inoculated by stabbing the organism (in pure culture) into the medium. A positive result produces a change of colour from green to bright blue and a negative reaction leaves the colour unchanged. -
Six Vented 55mm Crystal Polystyrene Petri Dish Volume(s) : -
Originally intended as a medium for the enumeration of enterococci in water using Membrane Filtration, this medium has become more popular in many other areas such as food bacteriology. The medium contains Tetrazolium Chloride, which is reduced by enterococci to the insoluble red dye Formazan resulting in dark red colonies of enterococci on the agar. It should be noted that this reaction is not exclusive to enterococci and colonies should be confirmed by additional testing e.g. Aesculin hydrolysis. -
Soda Glass Universal Bottle Type 3, 7ml volume capacity, with an 18mm polypropylene capVolume(s) : 7ml -
Soda Glass Screw Neck Tube with dimensions of 145x17mm and a 13mm gold metal cap Volume(s) : 17ml -
Soda Glass Test Tube with dimensions of 150x16mm and a red coloured push-fit capVolume(s) : 16ml -
Soda Glass Universal Type 3, 30ml, with a 24mm polypropylene capVolume(s) : 30ml -
Soda Glass Universal Type 3, 30ml, with a 24mm polypropylene cap and Durham Tube Volume(s) : 30ml
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This is an aqueous solution of Sodium Hydroxide (2%) with Phenol Red Indicator suitable for use in the digestion of Sputum samples prior to culture of the samples for Mycobacterium spp. It is generally used in conjunction with Sputum Neutralising Buffer (BM1324). -
BM1322 Sodium Hydroxide (4%) is a reagent used in the digestion and decontamination of sputum samples prior to culture for mycobacteria. Most clinical specimens submitted for acid-fast bacilli isolation are contaminated with more quickly developing commensal microbial flora. Additionally, acid-fast bacilli may be retained in respiratory secretions and not released for culture until the material is liquefied. Respiratory specimens, such as sputum, contain mucin which may trap microorganisms. Decontamination and digestion of the mucous components kills contaminating normal flora and allows slower growing mycobacteria to grow. Timely neutralization prevents potential loss of mycobacteria caused by high pH levels of decontaminants, resulting in the preservation of more viable organisms. BM1322 is recommended by the UK Standards for Microbiology Investigations as part of their decontamination/digestion protocol; it is generally used in conjunction with Sputum Neutralising Buffer (BM1325). -
Sodium Hydroxide (4%) with Phenol Red is a reagent used in the digestion and decontamination of sputum samples prior to culture for mycobacteria. Most clinical specimens submitted for acid-fast bacilli isolation are contaminated with more quickly developing commensal microbial flora. Additionally, acid-fast bacilli may be retained in respiratory secretions and not released for culture until the material is liquefied. Respiratory specimens, such as sputum, contain mucin which may trap microorganisms. Decontamination and digestion of the mucous components kills contaminating normal flora and allows slower growing mycobacteria to grow. Timely neutralization prevents potential loss of mycobacteria caused by high pH levels of decontaminants, resulting in the preservation of more viable organisms. Phenol red is used to indicate changes in pH. BM1320 is recommended by the UK Standards for Microbiology Investigations as part of their decontamination/digestion protocol; it is generally used in conjunction with Sputum Neutralising Buffer without Phenol Red (BM1324). -
Sorbitol MacConkey agar is a differential medium for the isolation of Escherichia coli 0157:H7 based on the formulation by Rappaport and Henig. It differs from other MacConkey mediums in that lactose has been replaced by sorbitol. As Escherichia coli 0157:H7 does not ferment sorbitol it produces pale translucent colonies whereas most other strains of Escherichia coli are sorbitol positive and produce pink colonies. Although it should be noted that colonies that are sorbitol positive can revert and possibly be mistaken as sorbitol negative. Tryptone and meat peptone provide the required carbon, nitrogen and vitamins. Sorbitol is a fermentable carbohydrate and neutral red is a pH indicator. Bile Salts no.3 and crystal violet are selective agents and together inhibit Gram-positive cocci. Sodium chloride maintains the osmotic balance. If required, the selectivity of the medium may be increased by the addition of cefixime (0.05mg/L) and potassium tellurite (2.5mg/L). Related Supplements : LS0013 Escherichia coli 0157 Selective Supplement
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Sorbitol MacConkey with Cefixime & Tellurite (CT-Smac) This is a selective differential medium for the isolation of Escherichia coli O157:H7. It differs from other MacConkey medium in that Lactose has been replaced by Sorbitol. As Escherichia coli O157:H7 does not ferment Sorbitol it produces pale translucent colonies whereas most other strains of Escherichia coli are Sorbitol positive and produce pink colonies. The medium is made more selective by the addition of the antimicrobial Cefixime and Potassium Tellurite. -
Soy peptone is manufactured from the enzymatic hydrolysis of soybean. This product provides a good source of nitrogen, carbohydrates, and vitamins. It is recommended for use in microbiological media for the detection and isolation of a wide variety of bacteria and fungi.
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This is a sterile aqueous solution of Potassium di-hydrogen phosphate (16.0 % w/v) with Phenol Red Indicator suitable for use in the neutralisation following the digestion of sputum with Sodium hydroxide prior to culture. It is generally used in conjunction with BM1322 Sodium hydroxide 4%. -
This is a sterile aqueous solution of Potassium Di-Hydrogen Ortho-phosphate (16.0 % w/v) suitable for use in the neutralisation following the digestion of Sputum with Sodium Hydroxide prior to culture. It is generally used in conjunction with Sodium Hydroxide 4% with Phenol Red Indicator 0.2%. -
Staph/Strep Selective Supplement E&O Laboratories Ltd Staph/Strep Selective Supplement (LS0008) is an antibiotic supplement used to enhance the selective isolation of Staphylococci and Streptococci species. -
E&O Heat Inactivated Serum is derived from horse serum and is suitable for use in diagnostic assays. One of the reasons for the heat inactivation of serum (heating to 56°C for 30 min) is to inactivate complement, a group of proteins present in serum that are part of the immune response. This is sometimes important for cells that will be used to prepare or assay viruses, used in cytotoxicity assays or other systems where complement may have an unwanted influence. The use of Heat Inactivated Serum is also usually recommended for growing embryonic stem cells. After filtration the dispensing and bottle filling processes are carried out in a state-of-the-art clean room under laminar flow. Once labelled the filled bottles are then subjected to controlled heat inactivation and are frozen and stored at -20°C without delay. The filter sterile Heat Inactivated Horse Serum is supplied in 100 or 500 ml PETG bottles. All E&O products are for in vitro use only. E&O products are intended only for use by qualified professionals who will safely handle and dispose of products they receive. All biologically derived materials (e.g. blood, sera) should be handled as if a potential biohazard. E&O media that contain antibiotics should be handled with care. Chemical resistant gloves, eye protection and laboratory coat should be worn. -
All E&O products are for in vitro use only. E&O products are intended only for use by qualified professionals who will safely handle and dispose of products they receive. All biologically derived materials (e.g. blood, sera) should be handled as if a potential biohazard. E&O media that contain antibiotics should be handled with care. Chemical resistant gloves, eye protection and laboratory coat should be worn. -
This is an egg-based medium for the isolation and presumptive identification of Mycobacterium spp particularly Mycobacterium bovis. This medium is used primarily in the veterinarian sector. The medium is based on the original formulation of Lowenstein that was subsequently modified by Jensen, the medium contains pyruvate and egg which provide the required protein and fatty acids. It differs from Lowenstein-Jensen Medium in that Sodium Pyruvate has replaced the Glycerol, which has been demonstrated to be inhibitory to some species, particularly M.bovis. The coagulation of the egg albumin during preparation also provides a solid surface for inoculation purposes. Malachite green is incorporated into the medium to inhibit contaminating organisms other than the mycobacteria that may still be present in the specimen after decontamination. Lowenstein-Jensen slopes should be inoculated with pre-treated specimens and incubated at 35-37°C for 8 weeks in 5-10% CO2. Container caps should be left loose for the first week of incubation to allow for circulation of the carbon dioxide as this will help to stimulate growth. Caps should then be tightened to prevent any dehydration of the medium. -
This product may be used as an alternative pre-treatment solution to lessen the background flora of samples before the testing for Mycobacteria species. This reagent should only be used for samples that routinely produce contaminated cultures after processing with an alkaline digestant. -
This product may be used as a pre treatment solution to lessen the background commensal flora of samples before the testing for Mycobacteria species. -
This buffer is intended primarily for use as a neutralising agent following treatment with alkaline compounds during the decontamination and homogenisation process of Sputum specimens prior to inoculation onto appropriate culture media for the isolation of Mycobacterium spp. -
Thiosulphate Citrate Bile Salts Sucrose (TCBS) Agar TCBS is a selective isolation medium for culture of pathogenic Vibrio spp. from clinical samples. The formulation was developed by Kobayashi, Enomoto, Skazaki and Kuwahara. This medium inhibits most enterobacteriacae for at least 24 hours. For the isolation of Vibrio spp. other than V.cholerae in environmental bacteriology, it is advisable to incubate at the lower temperature range of 20°C – 30°C. NB - It is not recommended to perform an oxidase test on any presumptive positive isolates directly from TCBS medium. -
Thiosulphate Citrate Bile Salts Sucrose (TCBS) Agar is a selective isolation medium for culture of pathogenic Vibrio spp. from clinical and food samples. The formulation was developed by Kobayashi et al. which was modified from Nakanishi’s formulation. Vibrio species are most widely recognized for their role in human intestinal infections and cholera worldwide. Thiosulphate Citrate Bile Salts Sucrose (TCBS) Agar is recommended by the FDA BAM, the UK Standards for Microbiology Investigations, and complies with the standard laid out by ISO 21872.
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A nutritious broth medium formulated by Todd and Hewitt for the production of antigenic streptococcal haemolysin. The broth is also used to cultivate streptococci prior to serological grouping. Normally the use of fermentable sugars in the broth would inactivate the haemolysin due to acid production. This is prevented by the use of buffers to maintain the pH in this broth. -
This medium is based on the formula described by Kupferburg, Johnson and Sprince for the selective isolation of Trichomonas spp. The medium is selective due to the inclusion of the broad spectrum antibiotic, chloramphenicol, to inhibit a wide range of Gram-positive and Gram-negative bacterial species. This medium does not contain an antifungal agent and Candida spp. will not be suppressed. However, the growth of Candida spp. does not interfere with that of Trichomonas spp. The inclusion of methylene blue as a redox indicator allows for the visualisation of any significant oxygen diffusion in the medium. Cultures may be examined microscopically after 48 hours incubation at 37°C for the presence of flagellate protozoans. If a negative result is obtained then the culture may be re-incubated for a further 72 hours. -
Trichomonas Broth (CPLM) with Nystatin is for the selective isolation of Trichomonas spp. This medium is based on the formula described by Kupferburg et al.. The superiority of the culture procedure over the wet mount procedure for detecting the presence of trichomonads in clinical specimens was demonstrated by Williams, and Kean and Day. Feinberg and Whittington demonstrated the greater accuracy of the culture procedure for detecting trichomonads in clinical material. The tryptone and liver extract act as carbon, nitrogen and vitamin sources in this medium. Maltose is a fermentable carbohydrate. The agar and cysteine HCl reduce the oxygen tension in the medium which aids the growth of Trichomonas spp.. Methylene blue is a redox indictor and allows for the visualisation of any significant oxygen diffusion in the medium. The medium is selective due to the inclusion of chloramphenicol and nystatin to inhibit a wide range of both Gram-positive and Gram-negative bacterial species as well as yeasts and fungi. Cultures may be examined microscopically after 48 hours incubation at 37 ± 1°C for the presence of flagellate protozoans. If a negative result is obtained, then the culture may be re-incubated for a further 72 hours.
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Triphenyltetrazolium Chloride Soya Tryptone (TSAT) Agar Complete Triphenyltetrazolium Chloride (TTC) has been added as an indicator to various media, and recommended by several workers as being helpful in the early recognition and identification of a variety of bacteria including Escherichia coli, Vibrio parahaemolyticus and enterococci. This particular formulation is based on a Tryptone Soya Agar with added Sucrose and is particularly useful when performing counts on food and food product samples. Many of the enterobacteriaceae and enterococci will reduce the TTC to a formazan which colours the colonies deep red making them easier to distinguish and identify. The presence of the Sucrose can also assist in the differentiation of Sucrose fermenting and non-fermenting strains. -
Triple sugar iron agar is used to differentiate between some of the enterobacteriacae on the basis of four reactions: fermentation of lactose, glucose and sucrose and the production of hydrogen sulphide. Beef extract, yeast extract and peptone provide the required nitrogen, carbon and vitamins. Lactose, sucrose and glucose are carbohydrates. Acid production from their fermentation is detected by the phenol red pH indictor. Sodium thiosulphate is reduced to hydrogen sulphide which is detected by the ferric citrate indicator. Sodium chloride maintains osmotic balance.
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This is a medium that can be used to differentiate between some of the Enterobacteriacae on the basis of four reactions, fermentation of Lactose, Glucose and Sucrose and the production of H2S. For use the medium is inoculated using a pure culture of the test organism which should be smeared onto the surface of the slope and stabbed into the butt of the medium. For details of the many reactions that may arise during the use of this medium reference should be made to one of the many standard textbooks.
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Triple Vented 140mm Crystal Polystyrene Petri Dish Volume(s) : -
Triple Vented 90mm Crystal Polystyrene Petri Dish Volume(s) :
