Citrex610 k-en-spa 4 citrex en eqiuipos de procesamiento

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EVALUATION OF THE BACTERIAL INHIBITORY/CIDAL ACTIVITY OF THE CITREX® MOLECULE IN : HAROLD EDUARDO DURANGO G. Medical Mycology Bacteriologist. Professor of Microbiology and Parasitology. Faculty of Medicine, U. of A. JOSE IGNACIO BARGUIL P. Food Microbiology Bacteriologist. Technical Consultant in Food Protection. Consultant for Banco Interamericano de Desarrollo, BID. Technical Director, Continua Consultores. Pediatric Infectology Research Laboratory, H.U.S.V.P. 1) FOOD DIRECT CONTACT SURFACE AREAS 2) FOOD PRODUCTION ROOM ENVIRONMENT

Transcript of Citrex610 k-en-spa 4 citrex en eqiuipos de procesamiento

Page 1: Citrex610 k-en-spa 4 citrex en eqiuipos de procesamiento

EVALUATION OF THE BACTERIAL INHIBITORY/CIDAL ACTIVITY OF THE CITREX® MOLECULE IN :

HAROLD EDUARDO DURANGO G.Medical Mycology Bacteriologist.Professor of Microbiology and Parasitology.Faculty of Medicine, U. of A.

JOSE IGNACIO BARGUIL P.Food Microbiology Bacteriologist.Technical Consultant in Food Protection.Consultant for Banco Interamericano de Desarrollo, BID.Technical Director, Continua Consultores.

Pediatric Infectology Research Laboratory, H.U.S.V.P.

1) FOOD DIRECT CONTACT SURFACE AREAS

2) FOOD PRODUCTION ROOM ENVIRONMENT

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Surfaces, tools, and pieces of equipment in direct contact with foods for human consumption used in 3 different industries (i.e. dairy, meat, and agri-industry) were studied.

All 3 stages of cleaning (i.e.: rinsing/removing coarse materials, detergent application with mechanic force [i.e.: scrubbing], and final rinsing/clarification) were practiced.

METHOD FOR SURFACE AREAS

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Two disinfecting concentrations (200 and 400 ppm) of Citrex® were applied by spray until dripping. The product was allowed to work for 15 or 30 minutes. Sampling was performed using PCA agar, for the determination of livable mesophyllic microflora, Violet Red Bile Agar (VRBA), and Brilla broth using the brush technique described by W. Mannheimer and T. Ibáñez (1971), covering 25 cm2 of the treated surface area. For total coliform and E. coli determination rubbing was performed on VRBA agar, while Brilla Broth was used for quantitative test purposes. Positive tubes were replicated then subjected to the E. coli confirmation indole test.

METHOD FOR SURFACE AREAS

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Cleaning, disinfection and sampling

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Cleaning, disinfection, and sampling

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CULTURE

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SURFACEAREAS

MESOPHYLLICORGANISNSCFUs/25 cm2

TOTALCOLIFORMS E. coli

Small cheeseMolds Countless Countless Positive

CurdlingVats 380 90 Positive

ProcessingTables 290 167 Positive

Lyre 276 68 Positive

Mill Countless 380 Positive

Cutter Countless Countless Positive

Inner pulpRemover Countless 234 Positive

Small tools(knives, cutting

boards, etc.)

432 60 Positive

SURFACEAREAS

MESOPHYLLIC ORGANISMSCFUs/25 cm2

TOTALCOLIFORMS

E. coli

Small cheesemolds 43 0 Negative

Curdlingvats 12 0 Negative

Processingtables 8 0 Negative

Lyre 23 0 Negative

Mill 16 0 Negative

Cutter 7 0 Negative

Inner pulpRemover 67 0 Negative

Small tools(knives, cutting

boards, etc.)

2 0 Negative

Surface areas prior to and after treatment with Citrex ®.

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Surface areas prior to and after treatment with 400 ppm Citrex ®

BEFORE 15 MINUTES 30 MINUTES

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For production room environmental analysis prior to fogging 400 ppm Citrex®, OGY plates were exposed to the environment for 10 minutes. After Citrex® fogging new OGY plates were exposed to the environment for 10 minutes. All plates were incubated at ambient temperature for seven (7) days. Results were then read and interpreted.

METHOD FOR ENVIRONMENT

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ENVIRONMENT

No. of molds and yeasts, 10-min

exposure

ProcessingRoom 1

12

ProcessingRoom 2

18

ProcessingRoom 3

10

Warehouse 22

ENVIRONMENT

No. of molds and yeasts, 10-min

exposure

Processing Room 1

3

Processing Room 2

7

ProcessingRoom 3

2

Warehouse 8

Room environments prior to and after treatment with 400 ppm Citrex®

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Room environments prior to and after treatment with 400 ppm Citrex®