by RELATED SUBSTANCES METHOD VERIFICATION PROTOCOL FOR CITALOPRAM HYDROBROMIDE API
| Superseded Protocol No. | Nil |
| Effective Date |
Table of contents :
| Sr. No. | Subject | Page No. |
| Protocol Approval | ||
| Objective | ||
| Scope | ||
| Responsibility | ||
| Product profile | ||
| Methodology | ||
| Specificity | ||
| Response Factor | ||
| Precision | ||
| Linearity | ||
| Limit of Detection (LOD) | ||
| Limit of Quantification (LOQ) | ||
| Solution Stability | ||
| Deviation /Incident | ||
| Validation Summary | ||
| Final Conclusion/Recommendation | ||
| Revision History |
- Protocol Approval:
Prepared By:
| Functional Area | Name | Designation | Signature/ Date |
| Quality Control |
Reviewed By:
| Functional Area | Name | Designation | Signature/Date |
| Quality Assurance | |||
| Head Quality Control |
Approved By:
| Functional Area | Name | Designation | Signature/Date |
| Head QA |
Authorized By:
| Functional Area | Name | Designation | Signature/Date |
| Head Quality |
- Objective:
The objective of this validation is to provide documentary evidence that analytical methodology used in the determination of Related Substance in Citalopram Hydrobromide will yield consistent and reliable results within the predetermined acceptance criteria.
Analytical method validation will be performed by considering thefollowing parameters:
| Parameters | Citalopram Hydrobromide |
| Specificity | yes |
| Precision | yes |
| System Precision | yes |
| Method Precision | yes |
| Intermediate Precision(Ruggedness) | yes |
| Linearity | yes |
| Limit of Detection (LOD) | yes |
| Limit of Quantification (LOQ) | yes |
| Stability in Analytical Solutions | yes |
- Scope :
This protocol is based on SOP and applicable for the validation of Related Substance of Citalopram Hydrobromide.
- Responsibility of Validation Team:
| Departments | Responsibilities |
| QC | Preparation and Review of Validation protocol. |
| Analysis of samples and recording of data. | |
| Compilation and checking of data | |
| Preparation and review of Validation report. | |
| To impart training of protocol to concerned department/persons. | |
| QA | Review and approval of Validation protocol. |
| Co-ordination with QC to carryout Validation. | |
| Review and approval of Validation report. | |
| Head Quality | Authorization of protocol. |
- Product Profile:
| Category | Antidepressant |
| Reason for Validation | First Verification validation |
| Active Ingredient | Citalopram |
| Methodology | Ph. Eur |
| Method Reference | Ph. Eur |
| Specification Limits | |
| Impurities at 230 nm | |
| Impurity D (demthyl Citalopram) | ≤0.2% |
| Impurity B (acid) (Ph. Eur.) | ≤0.15% |
| Other individual impurity | ≤0.1% |
| Total impurities | ≤0.5% |
| Impurities at 254 nm | |
| Impurity G | ≤0.15% |
| Other individual impurity | ≤0.1% |
- Methodology:
Materials and Methods
Related Substance
Reagents:
Ammonium format (AR grade)
Methanol (HPLC grade)
Acetonitrile (HPLC grade)
Milli-Q water
Preparation of mobile phase A:
Prepare a suitable quantity of a mixture of acetonitrile, methanol and water in the ratio of 4: 32: 64. Dissolve about 1.58 g of ammonium format in 500 ml of above prepared mixture. Mix well and degas.
Preparation of mobile phase B:
Prepare a suitable quantity of a mixture of water and acetonitrile in the ratio of 32: 68. Dissolve about 1.58 g of ammonium format in 500 ml of above prepared mixture. Mix well and degas.
Preparation of diluent:
Use mobile phase A as diluent.
Preparation of system suitability solution: (Reference Solution-b)
Dissolve the contents of a vial Citalopram for system suitability CRS (containing impurities B, D, F and G) in 1.0 ml of diluent.
Alternatively:
Accurately weigh and transfer about 1 mg each of impurity a standard and impurity G standard to a 25 ml volumetric flask. Add about 15 ml of diluent and sonicate to dissolve. Make up the volume with diluent and mix (Impurity mixture)
Accurately weigh and transfer about 1.5 mg of impurity D standard and Citalopram Hydrobromide working standard / Citalopram Hydrobromide CRS equivalent to about 0.25 mg of Citalopram to a 50 ml volumetric flask. Add about 30 ml of diluent and 1 ml of impurity mixture. Sonicate to dissolve and make up the volume with diluents and mix.
Preparation of standard solution: (Reference Solution-a)
Accurately weigh and transfer Citalopram Hydrobromide working standard / Citalopram Hydrobromide CRS equivalent to about 50 mg of Citalopram to a 100 ml volumetric flask. Add about 70 ml of diluent and sonicate to dissolve. Make up the volume with diluent and mix (stock solution).
Dilute 1 ml of stock solution to 100 ml with diluent and mix. Further dilute 1 ml to 10 ml with diluent and mix. Filter through 0.45 µm nylon membrane filter.
Preparation of sample solution:
Transfer to about 25 mg of Citalopram to a 50ml volumetric flask. Add about 30 ml of diluent and shake well. Make up the volume with diluent and mix. Filter through 0.45 µm nylon membrane filter.
Chromatographic parameters:
Column : Phenomenex synergi hydro-RP80A, 4µm (250mm x 4.6 mm)
Column oven temperature : 40°C
Injection volume : 40µl
Wavelength : UV at 230 and 254 nm
Flow rate : 1.0 ml/min
Run time : 40 min
Gradient program
| Time (min) | Mobile Phase A | Mobile Phase B |
| 0 | 100 | 0 |
| 2 | 100 | 0 |
| 25 | 40 | 60 |
| 32 | 40 | 60 |
| 33 | 100 | 0 |
| 40 | 100 | 0 |
Evaluation of system suitability:
Inject the system suitability solution into the chromatograph and record the chromatogram at 230 nm.
The system is suitable for analysis if and only if:
The resolution between impurity D and Citalopram peaks is not less than 1.5.
- Inject the standard solution into the chromatograph and record the chromatograms.
The column efficiency determined from Citalopram peak is not less than 40000 theoretical plates at 230 nm.
The relative standard deviation for six replicate injections is not more than 5.0 % at 230 nm and 254 nm.
Make the adjustments if necessary to meet the system suitability requirements.
Procedure:
Inject the Blank and sample solution into the chromatograph and record the chromatograms. Disregard the peaks observed in the sample chromatogram which are observed at the same retention time in the Blank chromatogram. Also disregard the peak due to impurity G at RRT 0.63 in the sample solution at 230 nm. The retention time of Citalopram peak is about 19 min.
Note:
Extract the chromatograms of Blank and sample at 254 nm for the calculations of Impurity G.
The relative retention times (RRT’s) of the eluting peaks are:
| Sr. No. | Name of the impurities | RRT | RF |
| 1. | Impurity G | ~ 0.63 | 0.6 |
RRT’s are calculated with respect to Citalopram peak (with delay volume of the instrument about 1 ml)
Note: Peak due to impurity A and impurity G may get swapped. Retention time of Impurity G can be confirmed from system suitability solution 254 nm.
Calculations:
AT DS P
- Impurity G = ————- x ——— x ———- x 100 x RF
(% m/m) (At 254 nm) AS DT 100
AT1 DS P
- Any individual known Impurity= ————- x ——— x ———- x 100
(% w/w) (At 230 nm) AS1 DT 100
AT2 DS P
- Other individual Impurity= ————- x ——— x ———- x 100 x RF
(% w/w) (At 230 nm) AS1 DT 100
AT3 DS P
- Other individual Impurity= ————- x ——— x ———- x 100 x
(% w/w) (At 254 nm) AS DT 100
- Total (% m/m) =2 + 3
Where,
AT = Area counts of impurity G peak in the chromatogram of the sample solution at 254 nm.
AT1 = Area counts of any individual known impurity peak in the chromatogram of the sample solution at 230 nm
AT2 = Area counts of other individual impurity peak in the chromatogram of the sample solution at 230 nm
AT3 = Area counts of other individual impurity peak in the chromatogram of the sample solution at 254 nm
AS = Average area counts of the Citalopram peak in the chromatogram of the standard solution at 254 nm
AS1 = Average area counts of the Citalopram peak in the chromatogram of the standard solution as obtained under system suitability at 230 nm
DS = Dilution factor for standard solution
DT = Dilution factor of sample solution
P = Percent potency of Citalopram Hydrobromide working standard / Citalopram Hydrobromide CRS, on as is basis.
RF = Response factor.
Note:
Impurity B (Ph. Eur.): 1-[3-(Dimethylamino)propyl]-1-(4-fluorophenyl)-3-hydroxy-1,3-dihydroisobenzofuran-5-carbonitrile.
Impurity D: (1RS)-1-(4-fluorophenyl)-1-[3-methylamino) propyl]-1’3-dihydroisobenzofuran-5-carbonitrile.
Impurity G: 4-(Dimethylamino)-1-[(1RS)-1-[3-dimethylamino) propyl]-1-(4-fluorophenyl)-1,3-dihydroisobenzofuran-5-yl]butan-1-one.
- Specificity:
Specificity of analytical method is its ability to assess unequivocally the analyte in presence of components that may be expected to be present in the sample.
Prepare and inject blank, reference solution, known impurity individually 0.1% of target concentration of test and sample solution spiked with known impurities at specification level. Check the peak purity of main peak and known impurities.
Analysis sequence
| Sample | Type | Injections |
| System Suitability | Standard | 1 |
| Blank Solution | Unknown | 1 |
| Placebo Solution | Unknown | 1 |
| System Suitability | Standard | 1 |
| Reference Solution | Standard | 6 |
| Known impurity solution | Standard | 1 |
| Sample Solution | Unknown | 1 |
| System Suitability (Bracketing) | Validate | 1 |
| Reference Solution (Bracketing) | Validate | 1 |
Each chromatograph shall be monitored individually to examine the interference.
Acceptance criteria
No peak shall be eluted at the retention time of Citalopram. Peak purity of the Citalopram and impurity should be passed.
- Response / Correction factor
To evaluate the correction factor for Impurity-A, Impurity-B (IH), Impurity-B (Ph.Eur), Impurity-C, Impurity-D & Impurity-G with respect to Citalopram, the standards having concentration 1.0% with respect to the target concentration was prepared and injected. Response and correction factor of -A, Impurity-B (IH), Impurity-B (Ph.Eur), Impurity-C, Impurity-D & Impurity-G with respect to Citalopram should calculated and the results are recorded.
Analysis sequence
| Sample | Type | Injections |
| System Suitability | Standard | 1 |
| Blank Solution | Unknown | 1 |
| System Suitability | Standard | 1 |
| Reference Solution | Standard | 6 |
| Standard Solution | Standard | 2 |
| Known impurity solution (A, B, C, D & G) | Standard | 2 |
| System Suitability (Bracketing) | Validate | 1 |
| Reference Solution (Bracketing) | Validate | 1 |
Where
AS : Areas of Citalopram standard
AI : Area of Impurity
PI : Purity of Impurity
PS : Purity of Citalopram standard
CI : Concentration of Impurity
CS : Concentration of Citalopram standard
- Precision:
- System Precision:
The system precision is the closeness of agreement between the responses of detector. It is usually expressed as the standard deviation (SD) or the relative standard deviation (RSD).
Prepare and inject separately System Suitability diluents (Blank), and Reference solution as per methodology procedure and record the area response of main peak in the Reference solution. Calculate the % RSD of response for six replicate.
Analysis sequence
| Sample | Type | Injections |
| System suitability solution | Standard | 1 |
| Blank solution | Unknown | 1 |
| System suitability solution | Standard | 1 |
| Reference solution | Standard | 6 |
| System suitability solution (Bracketing) | Validate | 1 |
Acceptance criteria
The relative standard deviation for peak area should be not more than 2.0%.
- Method Precision: (Repeatability)
The precision of an analytical method is the degree of agreement among individual test results when the procedure is applied repeatability to multiple samplings of homogenous sample. It is usually expressed as the standard deviation and the relative standard deviation.
Prepare six individual sample of same batch and analyze as per Methodology.
Analysis sequence
| Sample | Type | Injections |
| System suitability solution | Standard | 1 |
| Blank solution | Unknown | 1 |
| System suitability solution | Standard | 1 |
| Reference solution | Standard | 6 |
| Sample 1 | Unknown | 1 |
| Sample 2 | Unknown | 1 |
| Sample 3 | Unknown | 1 |
| Sample 4 | Unknown | 1 |
| Sample 5 | Unknown | 1 |
| Sample 6 | Unknown | 1 |
| Blank solution | Unknown | 1 |
| System suitability solution (Bracketing) | Validate | 1 |
| Reference solution (Bracketing) | Validate | 1 |
Acceptance criteria
For known and unknown impurities in related substances method, relative standard deviation of six analyses shall be not more than 10 %.
- Ruggedness (Intermediate Precision):
Intermediate precision expresses within laboratory variation with different analysts or equipment or different column on different days using same batch of drug product as per Methodology
Test Procedure:
The analysis of the same batch will be done in six replicate analyses by using different columns by different analyst, by different system on different day. The mean, standard deviation and relative standard deviation will be calculated.
Analysis sequence
| Sample | Type | Injections |
| System suitability solution | Standard | 1 |
| Blank solution | Unknown | 1 |
| System suitability solution | Standard | 1 |
| Reference solution | Standard | 6 |
| Sample 1 | Unknown | 1 |
| Sample 2 | Unknown | 1 |
| Sample 3 | Unknown | 1 |
| Sample 4 | Unknown | 1 |
| Sample 5 | Unknown | 1 |
| Sample 6 | Unknown | 1 |
| Blank solution | Unknown | 1 |
| System suitability solution (Bracketing) | Validate | 1 |
| Reference solution (Bracketing) | Validate | 1 |
Acceptance criteria
For known and unknown impurities in related substances method, relative standard deviation of six analyses shall be not more than 10 %.
- Linearity
The linearity of an analytical procedure is its ability (within a given range) to obtained test results which are directly proportional to the concentration (amount) of analyte in the sample.
Determine the linearity by preparing the solution (standard and impurity standard solution) at different levels (six labels) over a specified range from LOQ to 200 % of the specification limit. Each level inject in duplicate. Calculate correlation co-efficient.
Test Procedure:
Prepare and inject the known impurities solution and standard solution in the range of LOQ to 200 % concentration level calculate the correlation coefficient.
Preparation of linearity solution
| Level | Level % to the limit concentration | Linearity standard solution | Make up to diluent (ml) |
| 1 | LOQ | ||
| 2 | 50% | ||
| 4 | 100 % | ||
| 6 | 150 % | ||
| 7 | 200 % |
Analysis sequence
| Sample | Type | Injections |
| System Suitability | Standard | 1 |
| Blank | Unknown | 1 |
| System Suitability | Standard | 1 |
| Reference solution | Standard | 6 |
| Linearity solution-LOQ% level | Standard | 2 |
| Linearity solution-50% level | Standard | 2 |
| Linearity solution-100 % level | Standard | 2 |
| Linearity solution-150% level | Standard | 2 |
| Linearity solution-200 % level | Standard | 2 |
| System suitability solution (Bracketing) | Validate | 1 |
| Reference solution (Bracketing) | Validate | 1 |
Acceptance criteria
Plot the calibration curve of peak area v/s concentration for the studied peak. The correlation coefficient (r), after the regression analysis of the results should not be less than 0.99.
Limit of Detection (LOD):
Limit of detection is the lowest concentration of analyte in a sample that can be detected but not necessarily quantified under the stated experimental condition. To determine the lowest amount of analyte in a sample which the analytical method can:
Detect but not necessarily quantitate as an exact value (LOD)
System suitability was performed.
The LOD was determined for Citalopram, Impurity-A, Impurity-B, Impurity-C, Impurity-D & Impurity-G Calculated the concentration at which the signal to noise ratio is about 3:1.Prepare the LOD Solution using blank, placebo spiked with known impurities at determined LOD level and inject in six replicates. Calculate % RSD for six replicates of known impurities.
Analysis sequence
| Sample | Type | Injections |
| System suitability solution | Standard | 1 |
| Standard solution (0.1%) | Unknown | 1 |
| Blank solution | Unknown | 1 |
| System Suitability | Standard | 1 |
| Reference solution | Standard | 6 |
| LOD-Initial | Unknown | 1 |
| LOD-I/1 | Unknown | 1 |
| LOD-I/2 | Unknown | 1 |
| LOD-I/3 | Unknown | 1 |
| LOD-I/4 | Unknown | 1 |
| LOD-I/5 | Unknown | 1 |
| LOD-I/6 | Unknown | 1 |
| System suitability solution (Bracketing) | Validate | 1 |
| Reference solution (Bracketing) | Validate | 1 |
Acceptance criteria:
% RSD for six replicates response of known impurities shall be not more than 30.0%. The signal to noise ratio should be more than 3:1
.Limit of Quantitation (LOQ):
Limit of Quantitation is the lowest concentration of analyte in a sample that can be quantitate with acceptable precision under the stated experimental condition.
To determine the lowest amount of analyte in a sample which the analytical method can:
Quantitate with suitable precision and accuracy (LOQ)
The LOQ determined Citalopram, Impurity-A, Impurity-B, Impurity-A, Impurity-B, Impurity-C, Impurity-D & Impurity-G. Calculated the concentration at which the signal to noise ratio is about 10:1. Prepare the LOQ Solution using blank, placebo spiked with known impurities at determined LOQ level and inject in six replicates. Calculate % RSD for six replicates of known impurities.
Analysis sequence
| Sample | Type | Injections |
| System suitability solution | Standard | 1 |
| Blank solution | Unknown | 1 |
| System Suitability | Standard | 1 |
| Reference solution | Standard | 6 |
| LOQ-Initial | Unknown | 1 |
| LOQ-I/1 | Unknown | 1 |
| LOQ-I/2 | Unknown | 1 |
| LOQ-I/3 | Unknown | 1 |
| LOQ-I/4 | Unknown | 1 |
| LOQ-I/5 | Unknown | 1 |
| LOQ-I/6 | Unknown | 1 |
| System suitability solution (Bracketing) | Validate | 1 |
| Reference solution (Bracketing) | Validate | 1 |
Acceptance criteria:
% RSD for six replicates response of known impurities shall be not more than 10.
The signal to noise ratio should be more than 10:1.
- Solution Stability:
It is essential when validating an analytical method to confirm that the analyte has adequate stability in both the standard and sample solution during analytical measurement stages of the testing.
Test Procedure:
Prepare the standard solution and sample solution spiked with known impurities at the specification level as per Methodology. Analyze the standard solution and sample solution at the different time intervals and calculate the % cumulative RSD of peak area for known impurities and main peak.
Analysis sequence
| Sample | Type | Injections |
| System suitability solution | Standard | 1 |
| Blank solution | Unknown | 1 |
| Placebo solution | Unknown | 1 |
| System suitability solution | Standard | 1 |
| Reference solution | Standard | 6 |
| Test Solution | Unknown | 1 |
| System suitability solution (Bracketing) | Validate | 1 |
| Reference solution (Bracketing) | Validate | 1 |
Acceptance criteria:
Cumulative %RSD of peak area for known impurities and main peak shall not be more than10%.
Deviation /Incident
Any deviation during validation exercise shall be reported and justified. Raw data and chromatograms of all non-satisfactory results shall be kept along with validation report.
Validation summary
Data obtained through validation exercise shall be analyzed with regard to various parameters of validation and their acceptance criteria. A validation report shall be prepared summarizing all data. All prints, chromatograms and calculations shall be captured in this report.
Final Conclusion/Recommendation
Based on finding of data analysis conclusion shall be drawn.
Revision History:
| Revision No. | Details of changes | Reason for change |
| 00 | Nil | New Document |
