MLT Validation Protocol
MLT Validation Protocol
Protocol No.
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Page No: 2 of 11
TABLE OF CONTENTS
2.0 OBJECTIVE………………………………………………………………….
3.0 SCOPE………………………………………………………………………...
5.0 RESPONSIBILITY…………………………………………………………...
10 CONCLUSION………………………………………………………………...
11 KEY CONSIDERATIONS………………………………………………..
12 ABBERIVATIONS…………………………………………………………….
14 POST APPROVAL…………………………………………………………….
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2.0 OBJECTIVE:
To establish the documentary evidence that the method for Microbial limit test
for Non-sterile materials is capable of correctly estimating the microbial counts
in the Materials. The validity of the test results largely upon the adequacy of a
Demonstration that the test specimens to which they are applied do not, of
them -selves, inhibit the multiplication, under the test condition, of
microorganisms that may be present.
The validation exercise shall demonstrate that the method employed is capable
for correct enumeration of microorganisms without adversely effecting the
Growth even in case of materials, which have antimicrobial activity.
3.0 SCOPE:
This validation protocol is applicable for validating the Microbial limit test of on-
sterile products and raw materials.
The protocol shall be used for validation of the methods applicable for all Dosage
forms and materials, which have requirement for Microbial limit test.
Whenever the method is used for Microbial limit test for scale up/ scale down
Formulation, the validation shall be done on only one strength of product.
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5.0 RESPONSIBILITY:
Trained Microbiologist or a suitable trained authorized person
6.1.2 Prepared six test tube containing 10 ml each from Solution A (1:10) and
follow the same for the other preparation i.e. Solution B (1:50) and Solution
C (1:100) respectively.
6.1.3 Grow the bacterial cultures separately in Soyabean casein digest medium at
300C to 350C for 24 hours and Fungal cultures separately in Soyabean casein
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digest medium at 200C to 250C for 48 hours. The organisms to be used are as
mentioned
below.
- E.coli
- S. aures
- Salmonella
- Pseudomonas aeruginosa
- C. albicans
- A. niger
-Bile tolerant gram-negative bacteria (replaced the EP
procedure "Test for Enterobacteria and Certain Other Gram-
Negative Bacteria")
6.1.4 Prepare reference suspension separately of the above organisms by diluting
the broth cultures to get containing about not less than 103 viable
microorganisms per ml.
6.1.6 From each set pipette out 1 ml separately in two pre- sterilized Petri plate
.Pour 20-22 ml of liquefied Soyabean casein digest agar for the cultivation of
bacteria and 20-22 ml of liquefied Sabouraud dextrose agar for the cultivation
of fungi.
6.1.7 Incubate plates of soyabean casein digest agar at 30 0C to 350C for 5 days
and plates of Sabouraud dextrose agar at 200C to 250C for 5 days.
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Page No: 6 of 11
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6.2.3 Grow the bacterial culture separately in soyabean casein digest medium at
300C to 350C for 24 hours. The organisms to be used are as mentioned
below.
- E.coli
- S. aures
- Salmonella
- Pseudomonas aeruginosa
6.2.5 Incubate the tube of soyabean casein digest medium and Fluid lactose
medium at 300C to 350C for 24 to 48 hours and proceed for Isolation and
Identification of Staphylococcus aureus, Pseudomonas aeruginosa,
Salmonella, Escherichia coli from this broth as per specified SOP.
7.0 ACCEPTANCE CRITERIA
7.1 Recovery of the test organisms should not be less than 70 % of the calculated
value of the inoculum suspension is to be obtained.
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Major change in method for Microbial limit test like method for deactivation of
Antimicrobial activity.
10.0 CONCLUSION
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Abbreviations
QA Quality Assurance
SOP Standard Operative Procedure
GMP Good Manufacturing Practice
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Page No: 10 of 11
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Page No: 11 of 11
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Checked by
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Approved by
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