YERSINIA SELECTIVE AGAR (CIN)

INTENDED USE
Remel Yersinia Selective Agar (CIN) is a solid medium recommended for selective and differential isolation of Yersinia enterocolitica from
clinical specimens and food.

SUMMARY AND EXPLANATION

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In 1979, Schiemann described a selective and differential medium for isolation of Y. enterocolitica which contained cefsulodin, Irgasan ,
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novobiocin, bile salts, and crystal violet as selective agents. He later modified the formula by substituting sodium desoxycholate for bile salts
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and reduced novobiocin to 2.5 mg/liter, further improving growth and recovery of Y. enterocolitica. In a study comparing selective and
differential media for isolation of enteric pathogens, Yersinia Selective Agar was found to be superior to other media (e.g., SS (Salmonella-
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Shigella), MacConkey, CAL (cellobiose, arginine, lysine), and Y agars) for isolation of Yersinia spp. Some strains of Yersinia may require
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cold enrichment (4°C) in phosphate buffered saline prior to inoculation of Yersinia Selective Agar. Yersinia Selective Agar complies with the
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specifications of the AOAC International.

PRINCIPLE
Peptones provide nitrogen, amino acids, and peptides necessary for bacterial growth. Sodium chloride is a source of essential electrolytes
and maintains osmotic equilibrium. Yeast extract provides B-complex vitamins. Mannitol is the carbohydrate which, in combination with
neutral red dye, enables differentiation of enteric gram-negative bacilli. Organisms which ferment mannitol produce a localized pH drop
around the colony which is followed by absorption of the neutral red dye. This results in a characteristic “bulls-eye” colony which has a
colorless, translucent border and a red center. Colonies of Y. enterocolitica typically develop a “bulls-eye” appearance after 24-48 hours
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incubation at 25°C. Crystal violet, sodium desoxycholate, cefsulodin, Irgasan (triclosan), and novobiocin are selective agents which inhibit
Escherichia coli, Klebsiella pneumoniae, Proteus mirabilis, and Pseudomonas aeruginosa, as well as gram-positive organisms.

REAGENTS (CLASSICAL FORMULA)*

Mannitol....................................................................... 20.0 g Neutral Red ...............................................................30.0 mg
Peptone....................................................................... 10.0 g Cefsulodin ...................................................................4.0 mg
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Beef Extract................................................................... 5.0 g Irgasan .......................................................................4.0 mg
Meat Peptone................................................................ 5.0 g Novobiocin...................................................................2.5 mg
Sodium Pyruvate........................................................... 2.0 g Crystal Violet ...............................................................1.0 mg
Yeast Extract................................................................. 2.0 g Magnesium Sulfate......................................................1.0 mg
Sodium Chloride............................................................ 1.0 g Agar...........................................................................12.0 g
Sodium Desoxycholate ................................................. 0.5 g Demineralized Water.............................................1000.0 ml
pH 7.4 ± 0.2 @ 25°C
*Adjusted as required to meet performance standards.

PROCEDURE
1. Inoculate the specimen as soon as possible after it is received in the laboratory.
2. If the material is being cultured directly from a swab, roll the swab over a small area of the agar surface and streak for isolation.
3. Incubate plates aerobically at 25°C for 24-48 hours.
4. If cold enrichment is preferred, inoculate the specimen into Phosphate Buffered Saline (PBS) (REF R062582 or a suitable alternative)
and hold at 4°C for up to 21 days. Periodically subculture PBS onto plates of Yersinia Selective Agar, following established laboratory
guidelines. Incubate plates aerobically at 25°C for 24-48 hours.
5. Examine plates for typical colonies of Y. enterocolitica which develop a dark red “bulls-eye” center with a translucent border. Further
biochemical and/or serological testing may be required to definitively identify Y. enterocolitica. Consult appropriate references for further
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instructions.

Pour Tube: Melt Yersinia Selective Agar pour tube (REF R09999) in a boiling water bath and cool to 45-50°C. Add rehydrated CN Selective
Supplement (REF R45050). Mix and dispense into a sterile petri dish and proceed with the instructions above.

QUALITY CONTROL
All lot numbers of Yersinia Selective Agar (CIN) have been tested using the following quality control organisms and have been found to be
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acceptable. This quality control testing meets or exceeds CLSI standards. Testing of control organisms should be performed in accordance
with established laboratory quality control procedures. If aberrant quality control results are noted, patient results should not be reported.

CONTROL INCUBATION RESULTS

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*Yersinia enterocolitica ATCC 9610 Aerobic, 24-48 h @ 25°C Growth, clear colonies w/ deep red center
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*Enterococcus faecalis ATCC 29212 Aerobic, 24-48 h @ 25°C Inhibition (partial to complete)
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*Escherichia coli ATCC 25922 Aerobic, 24-48 h @ 25°C Inhibition (partial to complete)
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Proteus mirabilis ATCC 12453 Aerobic, 24-48 h @ 25°C Inhibition (partial to complete)
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*Pseudomonas aeruginosa ATCC 27853 Aerobic, 24-48 h @ 25°C Inhibition (partial to complete)
*CLSI recommended organism

LIMITATIONS
1. Gram-negative bacilli other than Y. enterocolitica grow on Yersinia Selective Agar, including Aeromonas, Serratia, Enterobacter, and
Citrobacter. These organisms cannot be differentiated from Y. enterocolitica on the basis of colony morphology alone. Further
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biochemical and/or serological testing is required for definitive identification of Y. enterocolitica.

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BIBLIOGRAPHY
1. Schiemann, D.A. 1979. Can. J. Microbiol. 25:1298-1304.
2. Schiemann, D.A. 1982. Appl. Environ. Microbiol. 43:14-27.
3. Head, C.B., D.A. Whitty, and S. Ratnam. 1982. J. Clin. Microbiol. 16:615-621.
4. Weissfeld, A.S. and A.C. Sonnenwirth. 1982. J. Clin. Microbiol. 15:508-510.
5. Food and Drug Administration. 2000. Bacteriological Analytical Manual Online. AOAC International, Gaithersburg, MD.
6. Clinical and Laboratory Standards Institute (CLSI). 2004. Quality Control for Commercially Prepared Microbiological Culture Media; Approved
Standard, 3rd ed. M22-A3. CLSI, Wayne, PA.
7. Kelly, M.T., E.M.D. Stroh, and J. Jessop. 1988. J. Clin. Microbiol. 26:1738-1740.
8. MacFaddin, J.F. 1985. Media for Isolation-Cultivation-Identification-Maintenance of Medical Bacteria. Vol. 1. Williams and Wilkins, Baltimore, MD.
9. Isenberg, H.D. 2004. Clinical Microbiology Procedures Handbook. 2nd ed., Vol. 2. ASM Press, Washington, D.C.

Refer to the front of Remel Technical Manual of Microbiological Media for General Information regarding precautions, product storage and
deterioration, specimen collection, storage and transportation, materials required, quality control, and limitations.

ATCC is a registered trademark of American Type Culture Collection.

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IFU 1998, Revised March 2, 2010 Printed in U.S.A.

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