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An Introduction To Analytical Method Development For Pharmaceutical Formulations
Submitted by Rashmin on Tue, 07/22/2008 - 17:19
Analytical methods development and validation play important roles in the discovery,
development, and manufacture of pharmaceuticals.
Pharmaceutical products formulated with more than one drug, typically referred to as
combination products, are intended to meet previously unmet patients need by combining thetherapeutic effects of two or more drugs in one product. These combination products can
present daunting challenges to the analytical chemist responsible for the developmentand validation of analytical methods. This presentation will discuss the development and
validation of analytical method (Spectrophotometric, High performance liquidchromatography (HPLC), & High performance thin layer chromatography (HPTLC)) for
drug products containing more than one active ingredient. The official test methods that resultfrom these processes are used by quality control laboratories to ensure the identity, purity,
potency, and performance of drug products.
Introduction
The number of drugs introduced into the market is increasing every year. These drugs may be
either new entities or partial structural modification of the existing one. Very often there is a
time lag from the date of introduction of a drug into the market to the date of its inclusion in
pharmacopoeias. This happens because of the possible uncertainties in the continuous and
wider usage of these drugs, reports of new toxicities (resulting in their withdrawal from the
market), development of patient resistance and introduction of better drugs by competitors.
Under these conditions, standards and analytical procedures for these drugs may not beavailable in the pharmacopoeias. It becomes necessary, therefore to develop newer analytical
methods for such drugs.
Basic criteria for new method development of drug analysis:
y The drug or drug combination may not be official in any pharmacopoeias,y A proper analytical procedure for the drug may not be available in the literature due to
patent regulations,
y Analytical methods may not be available for the drug in the form of a formulation due tothe interference caused by the formulation excipients,
y Analytical methods for the quantitation of the drug in biological fluids may not beavailable,
y Analytical methods for a drug in combination with other drugs may not be available,y The existing analytical procedures may require expensive reagents and solvents. It may
also involve cumbersome extraction and separation procedures and these may not be
reliable.
Introduction To Spectrophotometric Methods Of Analysis For Drugs In Combination2
Simultaneous estimation of drug combination is generally done by separation usingchromatographic methods like HPLC, GC and HPTLC etc. These methods are accurate and
precise with good reproducibility, but the cost of analysis is quite high owing to expensive
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instrumentation, reagent and expertise. Hence it is worthwhile to develop simpler and costeffective method for simultaneous estimation of drugs for routine analysis of formulation.
Spectrophotometric analysis fulfils such requirement where the simultaneous estimation ofthe drug combination can be done with similar effectiveness as that of chromatographic
methods.
The spectrophotometric assay of drugs rarely involves the measurement of absorbance of
samples containing only one absorbing component. The pharmaceutical analyst frequentlyencounters the situation where the concentration of one or more substances is required in
samples known to contain other absorbing substances, which potentially interfere in theassay. If the formula of the samples is known, the identity and concentration of the interfering
substance are known and the extent of interference in the assay may be determined.
A number of modifications to the simple spectrophotometric procedure are available to the
analyst, which may eliminate certain sources of interference and permit the accurate
determination of all of the absorbing components. Each modification of the basic procedure
may be applied if certain criteria are satisfied.
The basis of all the spectrophotometric techniques for multicomponent samples is the
property that at all wavelengths:y the absorbance of a solution is the sum of absorbance of the individual components ory the measured absorbance is the difference between the total absorbance of the solution
in the sample cell and that of the solution in the reference cell.
There are various spectrophotometric methods are available which can be used for the
analysis of a combination samples. Following methods can be used
y Simultaneous equation methody Derivative spectrophotometric methody Absorbance ratio method ( Q-Absorbance method)y Difference spectrophotometryy Solvent extraction method
Simultaneous Equation Method2
If a sample contains two absorbing drugs (X and Y) each of which absorbs at the lmax of the
other (as shown in figure 1. 1 and2), it may be possible to determine both drugs by
the technique of simultaneous equation (Vierodts method) provided that certain criteria
apply.
The informations required are:
y the absorptivities of X at 1 and 2, ax1 and ax2 respectivelyy the absorptivities of Y at 1 and2, ay1 and ay2 respectivelyy the absorbance of the diluted sample at 1 and 2, A1 and A2 respectively.
Let Cx and Cy be the concentration of X and Y respectively in the diluted samples.
Two equations are constructed based upon the fact that at 1 and2, the absorbance of the
mixture is the sum of the individual absorbance of X and Y.
At 1
A1 = ax1bCx + ay1bCy . (1)
At2
A2 = ax2bCx + ay2bCy . (2)
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For measurements in 1 cm cells, b =1.
Rearrange equation (2)
Cy = (A2 - ax2 Cx) / ay2
Substituting for Cy in eq. (1) and rearranging gives
Cx = (A2 ay1 - A1 ay2) / (ax2 ay1 - ax1 ay2)Cy = (A1 ax2 - A2 ax1) / (ax2 ay1 - ax1 ay2)
Fig. 1: The overlain spectra of substance X and Y, showing the wavelength for the
assay of X and Y in admixture by the method of simultaneous equation.
Criteria for obtaining maximum precision have been suggested by Glenn3. According to him
absorbance ratio place limits on the relative concentrations of the components of the mixture.
(A2/A1) / (ax2/ax1) and (ay2/ay1)/ (A2/A1)
The criteria are that the ratios should lie outside the range 0.1- 2.0 for the precise
determination of Y and X respectively. These criteria are satisfied only when the max of the
two components are reasonably dissimilar. An additional criterion is that the two components
do not interact chemically, thereby negating the initial assumption that the total absorbance is
the sum of the individual absorbance. The additive of the absorbance should always be
confirmed in the development of a new application of this technique.
Simultaneous equation method using Matrices and Cramer's Rule can be explained as
follows:
Consider a binary mixture of component X and Y for which the absorption spectra ofindividual components and mixture are shown in figure 1.
-1 is the max of component X
-2 is the max of component Y
the total absorbance of a solution at a given wavelength is equal to the sum of the absorbance
of the individual components at the wavelength. Thus the absorbance of mixture at the
wavelength 1 and 2 may be expressed as follows:
At 1
A1 = ax1bCx + ay1bCy (1)
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At 2
A2 = ax2bCx + ay2bCy . (2)
Such equation can be solved using matrices.
From equation (1) and (2),
A1 = kx1 Cx + ky1Cy . (3)A2 = kx2 Cx + ky2Cy . (4)
Where k = a x b
Let A, be a column matrix with 'i' elements [i, is the number of wavelength at which
measurements are done; here two wavelength 1 and 2 are taken in to consideration, so i=2].Let C, be a column matrix with 'j' elements [j, is the number of components, in this case X
and Y are present, so j = 2]. Let k, be a matrix with i x j values so that it has number of rowsequals to number of wavelength and number of columns equal to number of components ( in
this case it has two rows and two columns). Hence we have
A = k x C . (5)
Since the number of wavelength equal to number of components, the equation (5) has a
unique solution.
C = k-1
x A .(6)
However, it will be faster to solve the equation (3) and (4) by means of cramer's rule. And
unknown concentration Cj of component j is found by replacing' j column of matrix A. The
determinant of the new matrix is divided by determinant of 'k' matrix.
Cx = (A1 ky2 - A2 ky1) / (kx1 ky2 - kx2 ky1) . (7)
Cy = (kx1A2 - kx2A1) / ( kx1 ky2 - kx2 ky1) .. (8)
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Therefore
Cx = (A1 ay2 - A2 ay1) / ( ax1 ay2 - ax2 ay1) (9)
Cy = (ax1A2 - ax2A1) / ( ax1 ay2 - ax2 ay1) ..(10)
In British Pharmacopoeia the assay of quinine-related alkaloids and Cinchonine related
alkaloids are based on this technique.
Following drugs have been reported to be estimated simultaneously by the simultaneous
equation method.
- Estimation of Gliclazide and Metformin hydrochloride in combined dosage forms4.
- Estimation of Losartan potassium and Hydrochlorthiazide in tablets5.
- Estimation of Salbutamol and Theophylline from tablets6.
- Estimation ofAmlodipine besylate and Enalepril maleate from tablets7.
Drugs with large difference in the content in the combined dosage form have been estimated
simultaneously by Simultaneous equation method by standard addition technique. In whichknown amount of pure drug have been added to the sample drugs.
-Estimation of Ibuprofen and Pseudoephedrine hydrochloride from tablets8.
-Estimation of Salbutamol and Theophylline from tablets6.
Q-Absorbance Method (Absorbance Ratio Method)2
Q-Absorbance method depends on the property that, for a substance which obeys Beer's law
at all wavelength, the ratio of absorbances at any two wavelengths is a constant value
independent of concentration or pathlength. For example, two different dilution of the same
substance give the same absorbance ratio A1/A2. In the USP, this ratio is referred to as Q
value.
In the quantitative assay of two components in a mixture by the absorbance ratio method,absorbances are measured at two wavelengths. One being the max of one of the component
(2) and the other being a wavelength of equal absorptivities of the two components (Asshown in figure 2) i.e. an isoabsorptive point9.
Two equations are constructed as described for the method of simultaneous equation. Their
treatment is somewhat different, however, and uses the relationship ax1 = ay1 at 1. Assume b
= 1cm
A1 = ax1Cx + ax1Cy .. (1)
A2 /A1 = (ax2Cx + ay2Cy) / (ax1Cx + ax1Cy)
Divide each term by Cx + Cy and let Fx = Cx / (Cx + Cy) and Fy = Cy / (Cx + Cy) i.e. Fx and Fy
are the fraction of X and Y respectively in the mixture:
A2 /A
1 = (ax2 Fx + ay2Fy) / (ax1Fx + ax1Fy)But Fy = 1 - Fx
A2 /A1 = (ax2Fx - Fx ay2 + ay2) / ax1
A2 /A1 = (ax2 Fx)/ ax1 - (Fx ay2)/ ay1 + (ay2) / ay1
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Fig. 2: Wavelength for the assay of substances X and Y in admixture by the method of
absorbance ratio method.
Let QX = ax2 / ax1, QY = ay2/ ay1, and QM = A2 /A1
QM = Fx (QX - QY) + QY
Fx = (QM - QY) / (QX - QY) . (2)
Above equation gives fraction, rather than the concentration of X in the mixture in terms of
absorbance ratios. As these are independent of concentrations, only approximate, rater than
accurate, dilutions of X and Y and the sample mixture are required to determine Q X,QY, and
QM respectively.
For absolute concentration of X and Y, eq. (1) is rearranged
A1 = ax1 (Cx +CY)
Cx +Cy = A1 / ax1
From equation (2)
Cx / (Cx +Cy)= (QM - QY) / (QX - QY)
Cx / (A1 / ax1)= (QM - QY) / (QX - QY)
Cx = (QM - QY) A1 / (QX - QY) ax1
Above equation gives the concentration of X in terms of absorbance ratios, the absorbance ofmixture and the absorptivities of the compounds at the isoabsorptive wavelength.
The British Pharmacopoeia suggests the use of this method as the identification test for
Cyanocobalamin10
.
Following drugs have been reported to be estimated simultaneously by the Q- Absorbance
method.
- Estimation of Rifampicin and Isoniazide in pharmaceutical dosage forms 11.
- Estimation of Spiranolactone and hydroflumethiazide12
.
- Estimation of Nalidixic acid and Metronidazole from tablets13
.
- Estimation of Noscapine, Chlorpheniramine Maleate and Ephedrine hydrochloride from
tablets14
.
Derivative Spectroscopy 2
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For the purpose of spectral analysis in order to relate chemical structure to electronictransitions, and for analytical situations in which mixture contribute interfering absorption, a
method of manipulating the spectral data is called derivative spectroscopy15
.
Derivative spectrophotometry involves the conversions of a normal spectrum to its first,
second or higher derivative spectrum. (As shown in figure 3). In the context of derivative
spectrophotometry, the normal absorption spectrum is referred to as the fundamental, zero
order, orD0 spectrum.
The first derivative D1
spectrum is a plot of the rate of change of absorbance with wavelength
against wavelength i.e. a plot of the slope of the fundamental spectrum against wavelength or
a plot of dA/d vs. . . The maximum positive and maximum negative slope respectively in
the D spectrum correspond with a maximum and a minimum respectively in the D1
spectrum.
The max in D spectrum is a wavelength of zero slope and gives dA/d = 0 in the
D1
spectrum.
The second derivative D2
spectrum is a plot of the curvature of the D spectrum against
wavelength or a plot of d2A/ d
2vs. . The maximum negative curvature in the D spectrum
gives a minimum in the D2spectrum, and the maximum positive curvature in the D spectrum
gives two small maxima called satellite bands in theD
2
spectrum. The wavelength ofmaximum slope and zero curvature in the D spectrum correspond with cross-over points in
the D2 spectrum.
These spectral transformations confer two principal advantages on derivative
spectrophotometry. Firstly, an eve order spectrum is of narrower spectral bandwidth than itsfundamental spectrum. A derivative spectrum therefore shows better resolution of
overlapping bands than the fundamental spectrum and may permit the accurate determinationof the max of the individual bands. Secondly, derivative spectrophotometry discriminates in
favour of substances of narrow spectral bandwidth against broad bandwidth substances. All
the amplitudes in the derivative spectrum are proportional to the concentration of the analyte,
provided that Beer's law is obeyed by the fundamental spectrum.
Fig. 3: (b) First, (c) Second, (d) Third and (e)fourth derivative Spectrum of (a) Gaussian
peak.
The enhanced resolution and bandwidth discrimination increases with increasing derivativeorder. However, it is also found that the concomitant increase in electronic noise inherent in
the generation of the higher order spectra, and the consequent reduction of the signal-to-noise
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ratio, place serious practical limitations on the higher order spectra. For quantitativepurposes, second and fourth derivative spectra are the most frequently employed derivative
orders.
Derivative spectra may be generated by any of three techniques. The earliest derivative
spectra were obtained by modification of the optical system. Spectrophotometers with dual
monochromator set a small wavelength interval (, typically 1-3nm) apart, or with the
facility to oscillate the wavelength over a small range, are required. In either case the photodetector generates a signal with amplitude proportional to the slope of the spectrum
over the wavelength interval. Instruments of this type are expensive and are essentiallyrestricted to the recording of first derivative spectra only.
The second technique to generate derivative spectra is electronic differentiation of the
spectrophotometer analog signal. Resistance capacitance (RC) modules may be incorporated
in series between the spectrophotometer and recorder to provide differentiation of the
absorbance, not with respect to wavelength, but with respect to time, thereby producing the
signal dA/dt. If the wavelength scan rate is constant (d/dt = C), the derivative with respect to
wavelength is given by
dA
/ d = (dA
/dt) / (d /dt) = (dA
/dt)(1/C)Derivative spectra obtained by RC modules are highly dependent on instrumental parameters,
in particular the scan speed and the time constant. It is essential, therefore, to employ astandard solution of the analyte to calibrate the measured value the instrumental conditions
selected.
The third technique is based upon microcomputer differentiation. Microcomputers
incorporated into or interfaced with the spectrophotometer may be programmed to provide
derivative spectra during or after the scan, to measure derivative amplitudes between
specified wavelengths and to calculate concentrations and associated statistics from the
measured amplitude.
For the estimation of drugs in combinations, simultaneous use of derivative spectroscopy
along with simultaneous equation has been reported in the literature16.
Following drugs have been reported to be estimated simultaneously by the Derivativespectroscopy method.
-Estimation of Propranolol and Hydrochlorthiazide17
.
-Estimation of Phenylpropanolamine, chlorpheniramine and Bromhexine18.
-Estimation of Naphazoline hydrochloride and Chlorpheniramine maleate19
.
Drugs with large difference in the content in the combined dosage form have been estimated
simultaneously by Simultaneous equation method by standard addition technique. In which
known amount of pure drug have been added to the sample drugs.
-Estimation of Ibuprofen and Pseudoephedrine hydrochloride from tablets20
.
-Estimation of Salbutamol and Theophylline from tablets21
.
Solvent Extraction Method2
In solvent extraction method quantitation of individual drugs in combinations has been
performed by separation of individual drugs based on their selective solubility followed by
spectrophotometric measurement22
.
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If the interference from the other absorbing substances is large, it may be possible to separatethe absorbing interferent from the analyte by solvent extraction procedure. These are
particularly appropriate for acidic or basic drugs whose state of ionisation determines theirsolvent partitioning behavior. The judicious choice of pH of the aqueous medium may effect
the complete separation of the interferents from the analyte, the concentration of which may
be obtained by a simple measurement of absorbance of the extract containing the analyte.
Following drugs have been reported to be estimated by the Solvent extraction method.
-Estimation of Probenecid and Ampicillin from tablets22
.
-Estimation of Probenecid and Cephalexine from tablets22
.
-Estimation of Caffeine from Aspirin and Caffeine tablets23
.
-Estimation of Paracetamol and Diclofenac sodium from tablets24
.
Introduction To Hplc Methods Of Analysis For Drugs In Combination25 - 27
Most of the drugs in multicomponent dosage forms can be analyzed by HPLC methodbecause of the several advantages like rapidity, specificity, accuracy, precision and ease of
automation in this method. HPLC method eliminates tedious extraction and isolation
procedures. Some of the advantages are:
speed (analysis can be accomplished in 20 minutes or less),
greater sensitivity (various detectors can be employed),
improved resolution (wide variety of stationary phases),
reusable columns (expensive columns but can be used for many analysis),
ideal for the substances of low volatility,
easy sample recovery, handling and maintenance,
instrumentation tends itself to automation and quantitation (less time and less labour),
precise and reproducible,
calculations are done by integrator itself,
suitable for preparative liquid chromatography on a much larger scale.
There are different modes of separation in HPLC. They are normal phase mode, reversed
phase mode, reverse phase ion pair chromatography, affinity chromatography and size
exclusion chromatography.
In the normal phase mode, the stationary phase is polar and the mobile phase is nonpolar in
nature. In this technique, nonpolar compounds travel faster and are eluted first. This is because of the lower affinity between the nonpolar compounds and the stationary phase.
Polar compounds are retained for longer times because of their higher affinity with the
stationary phase. These compounds, therefore take more times to elute. Normal phase modeof separation is therefore, not generally used for pharmaceutical applications because most of
the drug molecules are polar in nature and hence take longer time to elute.
Reversed phase mode is the most popular mode for analytical and preparative separations ofcompound of interest in chemical, biological, pharmaceutical, food and biomedical sciences.
In this mode, the stationary phase is nonpolar hydrophobic packing with octyl or octa decylfunctional group bonded to silica gel and the mobile phase is polar solvent. An aqueous
mobile phase allows the use of secondary solute chemical equilibrium (such as ionization
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control, ion suppression, ion pairing and complexation) to control retention and selectivity.The polar compound gets eluted first in this mode and nonpolar compounds are retained for
longer time. As most of the drugs and pharmaceuticals are polar in nature, they are notretained for longer times and hence elute faster. The different columns used are octa decyl
silane (ODS) or C18, C8, C4, etc., (in the order of increasing polarity of the stationary phase).
In ion exchange chromatography, the stationary phase contains ionic groups like NR3+
or
SO3- , which interact with the ionic groups of the sample molecules. This is suitable for the
separation of charged molecules only. Changing the pH and salt concentration can modulate
the retention.
Ion pair chromatography may be used for the separation of ionic compounds and this method
can also substitute for ion exchange chromatography. Strong acidic and basic compounds
may be separated by reversed phase mode by forming ion pairs (coulumbic association
species formed between two ions of opposite electric charge) with suitable counter ions. This
technique is referred to as reversed phase ion pair chromatography or soap chromatography.
Affinity chromatography uses highly specific biochemical interactions for separation. The
stationary phase contains specific groups of molecules which can adsorb the sample if certain
steric and charge related conditions are satisfied. This technique can be used to isolateproteins, enzymes as well as antibodies from complex mixtures.
Size exclusion chromatography separates molecules according to their molecular mass.Largest molecules are eluted first and the smallest molecules last. This method is generally
used when a mixture contains compounds with a molecular mass difference of at least 10%.This mode can be further subdivided into gel permeation chromatography (with organic
solvents) and gel filtration chromatography (with aqueous solvents).
A schematic diagram of HPLC equipment is given in Fig.4.28
Fig. 4: A schematic diagram of HPLC equipment.
Various components of HPLC are:29-33
A solvent delivery system, including pump,
Sample injection system,
A chromatographic column,
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A detector,
A strip chart recorder,
Data handling device and microprocessor control.
a) Solvent delivery system:
A mobile phase is pumped under pressure from one or several reservoir and flows throughthe column at a constant rate. For normal phase separation eluting power increases with
increasing polarity of the solvent but for reversed phase separation, eluting power decreases
with increasing polarity.
A degasser is needed to remove dissolved air and other gases from the solvent. Special gradesof solvents are available for HPLC and these have been purified carefully in order to remove
absorbing impurities and particulate matter to prevent these particles from damaging thepumping or injection system or clogging the column.
Pumps:
The pump is one of the most important component of HPLC, since its performance directly
affects retention time, reproducibility and detector sensitivity.
Three main types of pumps are used in HPLC to propel the liquid mobile phase through the
system.
1. Displacement pump: It produces a flow that tends to independent of viscosity and back
pressure and also output is pulse free. But it possesses limited capacity (250 ml).
2. Reciprocating pump: It has small internal volume (35 to 400 l), their high output pressure
(upto 10,000 psi) and their constant flow rates. But it produces a pulsed flow.
3. Pneumatic or constant pressure pump: They are pulse free; suffer from limited capacity as
well as a dependence of flow rate on solvent viscosity and column back pressure. They are
limited to pressure less than 2000 psi.
(b) Sample injection system:Insertion of the sample onto the pressurized column must be as a narrow plug so that the peak
broadening attributable to this step is negligible. The injection system itself should have nodead (void) volume.
There are three important ways of introducing the sample into injection port.
Loop injection: In which, a fixed amount of volume is introduced by making use of
fixed volume loop injector.
Valve injection: In which, a variable volume is introduced by making use of an injection
valve.
On column injection: In which, a variable volume is introduced by means of a syringe
through a septum.
(c) Chromatographic column:
The column is usually made up of heavy glass or stainless steel tubing to withstand high
pressure. The columns are usually 10-30 cm long and 4-10 mm inside diameter containing
stationary phase at particle diameter of 25 m or less.
Columns with an internal diameter of 5 mm give good results because of compromise
between efficiency, sample capacity, and the amount of packing and solvent required.
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Column packing:
The packing used in modern HPLC consist of small, rigid particles having a narrow particle
size distribution. There are three main types of column packing in HPLC.
1. Porous, polymeric beds: Porous, polymeric beds based on styrene divinyl benzene co-
polymers used doe ion exchange and size exclusion chromatography. For analytical purpose
these have now been replaced by silica based, packing which are more efficient and morestable.
2. Porous layer beds: Consisting of a thin shell (1-3 m) of silica or modified silica on an
spherical inert core (e.g. Glass). After the development of totally porous micro particulatepackings, these have not been used in HPLC.
3. Totally Porous silica particles (dia. 20 m are usually dry packed. While
particles of diameter
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d. It must be added at a concentration that will produce a peak area or peak height ratio ofabout unity with the compound,
e. It must not be present in the original sample,
f. It must be stable, unreactive with sample components, column packing and the mobile
phase and
g. It is desirable that this compound is commercially available in high purity.
The internal standard should be added to the sample prior to sample preparation procedure
and homogenized with it. To be able to recalculate the concentration of a sample component
in the original sample, we have to demonstrate first the response factor. The response factor
(RF) is the ratio of peak areas of sample component (Ax) and the internal standard (AISTD)
obtained by injecting the same quantity. It can be calculated by using the formula,
RF =Ax / AISTD
On the basis of the response factor and strength of the internal standard (NISTD), the amount
of the analyte in the original sample can be calculated using the
formula,
X =AS / RF * AISTDX NISTD
The calculations described above can be used after proving the linearity of the calibrationcurve for the internal standard and the analytical reference standard of the compound of
interest. When more than one component is to be analyzed from the sample, the responsefactor of each component should be determined in the calculations using similar formula.
3. Standard addition method: In the standard addition method, a known amount of the
standard compound is added to the sample solution to be estimated. This method is suitable if
sufficient amount of the sample is available and is more realistic in the sense that it allows
calibration in the presence ofexcipients or other components.
As gradient elution can be a source of additional error in quantitative analysis. It is also
necessary to keep the flow rate and the mobile phase composition constant. The sampleshould be dissolved in the mobile phase. If the solvent used in the preparing the sample
solution and the mobile phase are not identical, the analysis can become less accurate and it is
also possible that the detector response is more dependent on the sample.
Design And Development And Of Separation Method
Methods for analyzing drugs in multicomponent dosage forms can be developed, provided
one has knowledge about the nature of the sample, namely, its molecular weight, polarity,
ionic character and the solubility parameter. An exact recipe for HPLC, however, cannot be
provided because method development involves considerable trial and error procedures. The
most difficult problem usually is where to start, what type of column is worth trying with
what kind of mobile phase. In general one begins with reversed phase chromatography, when
the compounds are hydrophilic in nature with many polar groups and are water soluble.
The organic phase concentration required for the mobile phase can be estimated by gradient
elution method. For aqueous sample mixtures, the best way to start is with gradient reversed
phase chromatography. Gradient can be started with 5-10% organic phase in the mobile phase
and the organic phase concentration (methanol or acetonitrile) can be increased up to 100%
within 30-45min. Separation can then be optimized by changing the initial mobile phase
composition and the slope of the gradient according to the chromatogram obtained from the
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preliminary run. The initial mobile phase composition can be estimated on the basis of wherethe compounds of interest were eluted, namely, at what mobile phase composition.
Changing the polarity of mobile phase can alter elution of drug molecules. The elution
strength of a mobile phase depends upon its polarity, the stronger the polarity, higher is the
elution. Ionic samples (acidic or basic) can be separated, if they are present in undissociated
form. Dissociation of ionic samples may be suppressed by the proper selection of pH.
The pH of the mobile phase has to be selected in such a way that the compounds are not
ionized. If the retention times are too short, the decrease of the organic phase concentration in
the mobile phase can be in steps of 5%. If the retention times are too long, an increase of the
organic phase concentration is needed.
In UV detection, good analytical results are obtained only when the wavelength is selectedcarefully. This requires knowledge of the UV spectra of the individual components present in
the sample. If analyte standards are available, their UV spectra can be measured prior toHPLC method development.
The molar absorbance at the detection wavelength is also an important parameter. When
peaks are not detected in the chromatograms, it is possible that the sample quantity is not
enough for the detection. An injection of volume of 20 l from a solution of 1 mg/mlconcentration normally provides good signals for UV active compounds around 220 nm.
Even if the compounds exhibit higher lmax, they absorb strongly at lower wavelength. It is notalways necessary to detect compounds at their maximum absorbance. It is, however,
advantageous to avoid the detection at the sloppy part of the UV spectrum for precisequantitation. When acceptable peaks are detected on the chromatogram, the investigation of
the peak shapes can help further method development.
The addition of peak modifiers to the mobile phase can affect the separation of ionic samples.
For examples, the retention of the basic compounds can be influenced by the addition of
small amounts of triethylamine (a peak modifier) to the mobile phase. Similarly for acidic
compounds small amounts of acids such as acetic acid can be used. This can lead to useful
changes in selectivity.When tailing or fronting is observed, it means that the mobile phase is not totally compatible
with the solutes. In most case the pH is not properly selected and hence partial dissociation or
protonation takes place. When the peak shape does not improve by lower (1-2) or higher (8-
9) pH, then ion-pair chromatography can be used. For acidic compounds, cationic ion pair
molecules at higher pH and for basic compounds, anionic ion-pair molecules at lower pH can
be used. For amphoteric solutes or a mixture of acidic and basic compounds, ion-pair
chromatography is the method of choice.
The low solubility of the sample in the mobile phase can also cause bad peak shapes. It is
always advisable to use the same solvents for the preparation of sample solution as the
mobile phase to avoid precipitation of the compounds in the column or injector.
Optimization can be started only after a reasonable chromatogram has been obtained. Areasonable chromatogram means that more or less symmetrical peaks on the chromatogram
detect all the compounds. By sight change of the mobile phase composition, the position ofthe peaks can be predicted within the range of investigated changes. An optimized
chromatogram is the one in which all the peaks are symmetrical and are well separated in lessrun time.
The peak resolution can be increased by using a more efficient column (column with higher
theoretical plate number, N) which can be achieved by using a column of smaller particle
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size, or a longer column. These factors, however, will increase the analysis time. Flow ratedoes not influence resolution, but it has a strong effect on the analysis time.
System Suitability Tests For Chromatographic Methods 36
System suitability is the checking of a system to ensure system performance before or during
the analysis of unknowns. Parameters such as plate count, tailing factors, resolution and
reproducibility (%RSD retention time and area for six repetitions) are determined andcompared against the specifications set for the method. These parameters are measured
during the analysis of a system suitability "sample" that is a mixture of main components and
expected by-products. Lists of the terms to be measured and their recommended limits
obtained from the analysis of the system suitability sample are given below.
Definition
The purpose of the system suitability test is to ensure that the complete testing system
(including instrument, reagents, columns, analysts) is suitable for the intended application.
The USPChromatography General Chapter states:
"System suitability tests are an integral part of gas and liquid chromatographic methods. Theyare used to verify that the resolution and reproducibility of the chromatographic system are
adequate for the analysis to be done. The tests are based on the concept that the equipment,electronics, analytical operations and samples to be analyzed constitute an integral system
that can be evaluated as such."
Evolution of System Suitability
Similar to the analytical method development, the system suitability test strategy should be
revised as the analysts develop more experience with the assay. In general, consistency of
system performance (e.g., replicate injections of the standard) and chromatographic
suitability (e.g. tailing factor, column efficiency and resolution of the critical pair) are the
main components of system suitability.
Early Stage of Method Development
During the early stage of the method development process some of the more sophisticatedsystem suitability tests may not be practical due to the lack of experience with the method. In
this stage, usually a more "generic" approach is used. For example, evaluation of the tailingfactor to check chromatographic suitability, and replicate injections of the system suitability
solution to check injection precision may be sufficient for an HPLC impurities assay.
In the early method development, it may be useful to perform some additional system
suitability tests to evaluate the system performances under different method conditions. This
information will help to develop an appropriate system suitability test strategy in the future.
As The Method Matures
As more experience is acquired for this method, a more sophisticated system suitability test
may be necessary. For HPLC impurities method intended to be stability indicating, a critical pair for resolution determination should be identified. The critical pair is defined as the two
peaks with the least resolution in the chromatographic separation. Generally, a minimumresolution limit is defined for the critical pair to ensure that the separations of all other
impurities are acceptable. All critical factors that will significantly impact the method performance will need to be identified. Therefore, if the resolution test results exceed the
acceptance limit, the critical factors can be adjusted to optimize the system performance. If %organic in the mobile phase has a significant impact on the resolution of the critical pair,
organic composition in the mobile phase can be adjusted within a predetermined range to
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achieve the acceptable resolution. Therefore, system suitability strategy not only consists ofthe tests and limits, but also the approach used to optimize system performance when the
original test result exceeds the limit. In addition, if the method demands high methodsensitivity (e.g. to analyze very low impurity levels), a detector sensitivity solution may be
required to demonstrate suitable signal-to-noise from the HPLC system. These system
suitability tests, combined with the typical replicate injections of the standard solution, may
be used to demonstrate the system suitability for this method.
Long Term System Suitability Strategy
During the final stage of method development, there is a need to define the long-term strategy
for system suitability requirements, and the practicalities for all laboratories using this
method. If the system suitability test involves the use of any reference sample (i.e. isolated
and characterized impurity), the laboratory needs to have enough supply of this reference
sample to complete the system suitability test. However, maintaining the supply of this
reference sample in the long term is usually not an easy task. If the reference sample is a
degradation product of the drug substance, it is desirable to generate the reference sample in-
situby artificially degrading the drug substance in order to streamline the method. Therefore,
extensive investigations must be done to evaluate the best approach to generate the reference
sample, and to identify the critical factors needed to ensure that the degradation process isreproducible.
How to Set Limits
Numerous approaches can be used to set limits for system suitability tests. This depends onthe experience with the method, material available and personal preference. During method
development, it may be useful to perform some system suitability tests with no acceptancelimit. Firstly, it is premature to set any limit during the very early stage of method
development. Secondly, since experimental conditions will be varied intentionally during
method development, collecting system suitability data in these experiments will help the
analyst to evaluate the impact of results generated under different method conditions. This
information will be used to set appropriate system suitability limits in the future.
Default Values from Regulatory Guidelines
There are numerous guidelines which detail the expected limits for typical chromatographic
methods. In the current FDA guidelines on "Validation of Chromatographic Methods" , the
following acceptance limits are proposed as initial criteria:
These suggested limits may be used as a reference to set up the initial system suitabilitycriteria in the early method development process.
Method Validation Results
Making use of the method validation results is yet another approach. During the robustness
testing of method validation, critical method parameters such as mobile phase composition,
column temperature are varied to mimic the day-to-day variability. Therefore, the system
suitability results from these robustness experiments should reflect the expected range for the
system suitability results. As a result, the limits for system suitability tests can be determined
from these experiments. This is a very effective approach since the required system suitability
results can be generated during method validation, and no special study is required. However,
these results only reflect the expected performance of the system, but not necessarily the
minimum "performance standard" for acceptable results. For example, the minimum
resolution of the critical pair from method validation may be 3.5; however, a resolution of 2.0
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may still be acceptable as long as they are baseline resolved, and all other chromatographicparameters remain acceptable.
Simulated Conditions
Ideally the analyst should observe the results from a "deteriorating" system and determine the
situations under which the results are no longer acceptable. One way to simulate the
deterioration of the system is to use an old or artificially degraded column in the analysis.Typically, a column can be degraded artificially by numerous injections or heating at extreme
pH conditions. These old columns will provide the information about the changes
System Suitability Parameters and Recommendations
Parameter Recommendation
Capacity Factor (k) The peak should be well-resolved from other peaks and thevoid volume, generally k>2.0
Repeatability RSD /= 5 is desirable.
Relative retention Not essential as long as the resolution is stated.
Resolution (Rs) Rs of > 2 between the peak of interest and the closest elutingpotential interferent (impurity, excipient, degradation product, internal standard, etc.
Tailing Factor (T) T of 2000
If the results are adversely affected by the changes in column performance (e.g. unacceptable
precision of results due to overlapping peaks), the system suitability results from these
experiments will help to determine the limits for system suitability criteria.
This approach facilitates the investigation of the worst case scenario, which reflects minimum
performance standard used to ensure that the chromatography is not adversely affected.
The parameters that are affected by the changes in chromatographic conditions are:
Resolution (Rs),
Capacity factor (k),
Selectivity (a),
Column efficiency (N) and
Peak asymmetry factor (As).
1. Resolution (Rs): Resolution is the parameter describing the separation power of the
complete chromatographic system relative to the particular components of the mixture.
The resolution, Rs, of two neighboring peaks is defined as the ratio of the distance between
two peak maxima. It is the difference between the retention times of two solutes divided by
their average peak width. For baseline separation, the ideal value of Rs is 1.5. It is calculated
by using the formula,
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Fig. 5: Resolution between two peaks.
where, Rt1 and Rt2 are the retention times of components 1 and 2 and
W1 and W2 are peak width of components 1 and 2.
There are three fundamental parameters that influence the resolution of a chromatographicseparation:
capacity factor (k')
selectivity ()
column efficiency (N)
These parameters provide you with different means to achieve better resolution, as well as
defining different problem sources
2. Capacity Factor (k): Capacity factor is the ratio of the reduced retention volume to the
dead volume. Capacity factor, k, is defined as the ratio of the number of molecules of solutein the stationary phase to the number of molecules of the same in the mobile phase. Capacity
factor is a measure of how well the sample molecule is retained by a column during anisocratic separation. The ideal value of k ranges from 2-10. Capacity factor can be
determined by using the formula,
Fig. 6: Retention Factor
Where, tR=retention volume at the apex of the peak (solute) and
t0 = void volume of the system.
Capacity Factor (k') changes are typically due to:
Variations in mobile phase composition
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Changes in column surface chemistry (due to aging)
Changes in operating temperature.
In most chromatography modes, capacity factor (k') changes by 10 percent for a temperaturechange of 5 C.
Adjusting Capacity Factor (k')
Good isocratic methods usually have a capacity factor (k') in the range of 2 to 10 (typically
between 2 and 5). Lower values may give inadequate resolution. Higher values are usually
associated with excessively brood peaks and unacceptably long run times.
If the analytes fall outside their specified windows run the initial column test protocol tocompare the results obtained with a new column.
Capacity Factor (k') values are sensitive to:
solvent strength
composition
purity
temperature
column chemistry
sample
If the shift in Capacity Factor (k') value is observed with both analytes and the column test
solution, the problem is most likely due to change in the column, temperature or mobile
phase composition. This is particular ly true if the shift occurred gradually over a series of
runs. If, however the test mixture runs as expected, the problem is most likely sample-
related.
3. Selectivity(a): The selectivity (or separation factor), a, is a measure of relative retention of
two components in a mixture. Selectivity is the ratio of the capacity factors of both peaks, andthe ratio of its adjusted retention times. Selectivity represents the separation power of
particular adsorbent to the mixture of these particular components.
This parameter is independent of the column efficiency; it only depends on the nature of thecomponents, eluent type, and eluent composition, and adsorbent surface chemistry. In
general, if the selectivity of two components is equal to 1, then there is no way to separatethem by improving the column efficiency.
The ideal value of a is 2. It can be calculated by using formula,
a=V2 V1 / V1 V0 = k1/ k2
Where, V0 = the void volume of the column,
V1 and V2 =the retention volumes of the second and the first peakrespectively.
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Fig. 7: Selectivity
Adjusting selectivity ()
When troubleshooting changes in Selectivity (), the approach is similar to the approach used
to troubleshoot changes in Capacity Factor (k').
When Selectivity () is affected, the corrective action depends on whether the problem is
mobile phase or column related.Be sure to compare results obtained with the test solution to those observed when the column
was new. Use these results to distinguish column changes from problems with mobile phaseor other operating parameters.
Selectivity () values are sensitive to:
changes in mobile phase composition (pH ionic strength)
purity
temperature
4. Column Efficiency/ Band broadening: Efficiency, N, of a column is measured by the
number of theoretical plates per meter. It is a measure of band spreading of a peak. Similarthe band spread, higher is the number of theoretical plates, indicating good column andsystem performance. Columns with N ranging from 5,000 to 100,000 plates/meter are ideal
for a good system. Efficiency is calculated by using the formula,
Fig. 8: Number of Theoretical Plates
Where, tR is the retention time and
W is the peak width.
A decline in measured efficiency may be due to:
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age and history of the column
extra column band broadening (such as due to malfunctioning injector or improper tubing
ID)
inappropriate detector settings (for example, time constant)
change in flow rate and solvent viscosity.
You can recognize problems in your separation due to a loss of column efficiency when the
width and/or shape of all peaks are affected.
If the measured efficiency has degraded, either the column has degraded, or system
bandbroadening has increased. At this point, check system bandspreading against establishedbenchmarks.
Methods of measuring column efficiency (N)
Methods used for the measurement and calculation of column include (in order to sensitivity
to abnormal peak shape):
Asymmetry-based (Most sensitive to tailing or fronting)
5 sigma
4 sigma
Tangent
3 sigma
height
2 sigma (infection) (Least sensitive to tailing or fronting)
Choose the method that best suits your operating requirements. It is critical that the same
method always be used and executed reproducibly.
Figure above illustrates the use of the different peak widths of a Gaussian peak for thecalculation of column efficiency (N).
When measuring Column Efficiency, use test conditions identical to those used in the
established benchmark performance (such as test sample, flow rate, mobile phase
composition and so on). Measure the column efficiency against the established performance.
5. Peak asymmetry factor (Tf): Peak asymmetry factor, Tf, can be used as a criterion of
column performance. The peak half width, b, of a peak at 10% of the peak height, divided by
the corresponding front half width, a, gives the asymmetry factor.
Fig. 9A: Asymmetric Factor
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For a well packed column, an asymmetry factor of 0.9 to 1.1 should be achievable.
Fig. 9B: Asymmetric Factor
Introduction To Hptlc Methods Of Analysis For Drugs In Combination37
HPTLC (High Performance Thin Layer Chromatography) is a well known and versatileseparation method which shows a lot of advantages in comparison to other separation
techniques.
Layer of Sorbent 100m
Efficiency High due to smaller particle
Separations 3 - 5 cm
Analysis Time Shorter migration distance an
Solid support Wide choice of stationary ph
Development chamber New type that require less am
Sample spotting Auto sampler
Scanning Use of UV/ Visible/ Fluores
densitometer
Features of HPTLC
1. Simultaneous processing of sample and standard - better analytical precision andaccuracy less need for Internal Standard
2. Several analysts work simultaneously3. Lower analysis time and less cost per analysis4. Low maintenance cost5. Simple sample preparation - handle samples of divergent nature
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6. No prior treatment for solvents like filtration and degassing7. Low mobile phase consumption per sample8. No interference from previous analysis - fresh stationary and mobile phases for each
analysis - no contamination
9. Visual detection possible - open system10.Non UV absorbing compounds detected by post-chromatographic derivatization
Steps involved in HPTLC
1. Selection of chromatographic layer2. Sample and standard preparation3. Layer pre-washing4. Layer pre-conditioning5. Application of sample and standard6. Chromatographic development7. Detection of spots8. Scanning9. Documentation of chromatic plate
Selection of chromatographic layer
- Precoated plates - different support materials - different Sorbents available- 80% of analysis - silica gel GF Basic substances, alkaloids and steroids Aluminum oxide
- Amino acids, dipeptides, sugars and alkaloids - cellulose
- Non-polar substances, fatty acids, carotenoids, cholesterol - RP2, RP8 and RP18
- Preservatives, barbiturates, analgesic and phenothiazines- Hybrid plates-RPWF254s
Sample and Standard Preparation
- To avoid interference from impurities and water vapours.
- Low signal to noise ratio - Straight base line- Improvement of LOD
- Solvents used are Methanol, Chloroform: Methanol (1:1), Ethyl acetate: Methanol (1:1), - -
- Chloroform: Methanol: Ammonia (90:!0:1), Methylene chloride : Methanol (1:1), 1%
Ammonia or 1% Acetic acid- Dry the plates and store in dust free atmosphere
Activation of pre-coated plates
- Freshly open box of plates do not require activation
- Plates exposed to high humidity or kept on hand for long time to be activated
- By placing in an oven at 110-120c for 30 prior to spotting- Aluminum sheets should be kept in between two glass plates and placing in oven at 110-
120c for 15 minutes.
Application of sample and standard
- Usual concentration range is 0.1-1g / l
-A bove this causes poor separation- Linomat IV (automatic applicator) - nitrogen gas sprays sample and standard from syringe
on TLC plates as bands
- Band wise application - better separation - high response to densitometer
Selection of mobile phase
- Trial and error
- ones own experience and Literature
Normal phase
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- Stationary phase is polar- Mobile phase is non polar
- Non-polar compounds eluted first because of lower affinity with stationary phase- Polar compounds retained because of higher affinity with the stationary phase
Reversed phase
- Stationary phase is non polar
- Mobile phase is polar- Polar compounds eluted first because of lower affinity with stationary phase
- Non-Polar compounds retained because of higher affinity with the stationary phase
- 3 - 4 component mobile phase should be avoided
- Multi component mobile phase once used not recommended for further use and solvent
composition is expressed by volumes (v/v) and sum of volumes is usually 100
- Twin trough chambers are used only 10 -15 ml of mobile phase is required
- Components of mobile phase should be mixed introduced into the twin - trough chamber
Pre- conditioning (Chamber saturation)
- Un- saturated chamber causes high Rf values
- Saturated chamber by lining with filter paper for 30 minutes prior to development - uniform
distribution of solvent vapours - less solvent for the sample to travel - lower Rf values.
Chromatographic development and drying
- After development, remove the plate and mobile phase is removed from the plate - to avoid
contamination of lab atmosphere- Dry in vacuum desiccator - avoid hair drier - essential oil components may evaporate
Detection and visualization
- Detection under UV light is first choice - non destructive
- Spots of fluorescent compounds can be seen at 254 nm (short wave length) or at 366 nm
(long wave length)
- Spots of non fluorescent compounds can be seen - fluorescent stationary phase is used -
silica gel GF- Non UV absorbing compounds like ethambutol, dicylomine etc - dipping the plates in 0.1%
iodine solution
- When individual component does not respond to UV - derivatisation required for detection
Quantification
- Sample and standard should be chromatographed on same plate - after development
chromatogram is scanned
- Camag TLC scanner III scan the chromatogram in reflectance or in transmittance mode by
absorbance or by fluorescent mode - scanning speed is selectable up to 100 mm/s - spectra
recording is fast - 36 tracks with up to 100 peak windows can be evaluated
- Calibration of single and multiple levels with linear or non-linear regressions are possible
when target values are to be verified such as stability testing and dissolution profile singlelevel calibration is suitable
- Statistics such as RSD or CI report automatically- Concentration of analyte in the sample is calculated by considering the sample initially
taken and dilution factors.
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Fig. 10: Schematic procedure for HPTLC
38
HPTLC Method design and development
Set the analytical objective first that may be quantification or qualitative identification or
separation of two components/multicomponent mixtures or optimization of analysis time
before starting HPTLC. Method for analyzing drugs in multicomponent dosage forms by
HPTLC demands primary knowledge about the nature of the sample, namely, structure,
polarity, volatility, stability and the solubility parameter. An exact recipe for HPTLC,
however, also same like HPLC cannot be provided because method development involves
considerable trial and error procedures. The most difficult problem usually is where to start,
with what kind of mobile phase.
Selection of stationary phase is quite easy that is to start with silica gel which is reasonable
and nearly suits all kind of drugs. Mobile phase optimization is carried out by using three
level techniques. First level involves use of neat solvents and then by finding some such
solvents which can have average separation power for the desired drugs. Second level
involves decreasing or increasing solvent strength using hexane or water for respective
purposes. Third level involves trying of mixtures instead of neat solvents from the selected
solvents of first and second level which can further be optimized by the use of modifier like
acids or bases.
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Analytes are detected using fluorescence mode or absorbance mode. But if the analytes arenot detected perfectly than it need change of stationary phase or mobile phase or need the
help of pre or post chromatographic derivatization.
Optimization can be started only after a reasonable chromatogram which can be done by
slight change in mobile phase composition. This leads to a reasonable chromatogram which
has all the desired peaks in symmetry and well separated.
Parameters that are affected by the changes in chromatographic conditions are:
Retention factor (Rf) and
Peak purity
1. Retention factor (Rf): Retention factor (Rf) is defined as the amount of separation due to
the solvent migration through the sorbent layer as shown in the formula. It depends on timeof development and velocity coefficient or solvent front velocity.
Migration distance of substance
Rf = --------------------------------------------------------
Migration distance of solvent front from origin2. Peak purity: The null hypothesis these spectra are identical can in this case (purity) with
two sided significance. During the purity test the spectrum taken at the first peak slope is
correlated with the spectrum of peak maximum [r(s,m)] and the correlation of the spectra
taken at the peak maximum with the one from the down slope or peak end [r(m,e)] which is
used as a reference spectra for statistical calculation. An error probability of 1% only be
rejected if the test value is greater than or equal to 2.576.
Validation Of Analytical Method 39-41
Validation is an act of proving that any procedure, process, equipment, material, activity or
system performs as expected under given set of conditions and also give the required
accuracy, precision, sensitivity, ruggedness, etc.
When extended to an analytical procedure, depending upon the application, it means that a
method works reproducibly, when carried out by same or different persons, in same or
different laboratories, using different reagents, different equipments, etc.
The various validation parameters are:
accuracy,
precision(repeatability and reproducibility),
linearity and range,
limit of detection(LOD)/ limit of quantitation(LOQ),
selectivity/ specificity,
robustness/ ruggedness and
Stability and system suitability studies.
Advantages of Analytical method Validation:-
The biggest advantage of method validation is that it builds a degree of confidence, not only
for the developer but also to the user.
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Although the validation exercise may appear costly and time consuming, it resultsinexpensive, eliminates frustrating repetitions and leads to better time management in the
end.
Minor changes in the conditions such as reagent supplier or grade, analytical setup are
unavoidable due to obvious reasons but the method validation absorbs the shock of such
conditions and pays for more than invested on the process.
Analytical method validation: The Regulatory Perspective
In the US, there was no mention of the word validation in the cGMPs of 1971, and precision
and accuracy were stated as laboratory controls. It was only in the cGMP guideline of March1979 that the need for validation was implied. It was done in two sections: (1) Section
211.165, where the word validation was used and (2) section 211.194, in which the proof ofsuitability, accuracy and reliability was made compulsory for regulatory submissions.
Another guidance on validation of chromatographic methods was released by CDRE on1
stNov. 1994.
The WHO published a guidelines under the title, Validation of analytical procedures used in
the examination of pharmaceutical materials. It appeared in the 32nd
report of the WHO
expert committee on specifications for pharmaceutical preparations which was published in1992.
The international Conference on Harmonization (ICH), which has been on the forefront of
developing the harmonized tripartite guidelines for adoption in the US, Japan and EC , has
issued two guidelines under the titles- Text on validation ofAnalytical procedures(Q2A) and
validation ofAnalytical procedure Methodology (Q2B).
Among the pharmacopoeias, USP XXII 1225 (1995) carries a section which describesrequirements of validation of compendial methods. The British Pharmacopoeia includes the
definition of method validation in 15 latest editions, but the term is completely missing form
the Indian Pharmacopoeia. (1996).
K
ey parameters of the Analytical method validation:-
It is important for one to understand the parameters or characteristics involved in the
validation process. The various Performance parameters, which are addressed in a validation
exercise, are grouped as follows.
(1) Accuracy: -
The accuracy of an analytical method may be defined as the closeness of the test results
obtained by the method to the true value. It is the measure of the exactness of the analytical
method developed. Accuracy may often express as percent recovery by the assay of a known
amount of analyte added.
Accuracy may be determined by applying the method to samples or mixtures of excipients to
which known amount of analyte have been added both above and below the normal levels
expected in the samples. Accuracy is then calculated from the test results as the percentage of
the analyte recovered by the assay. Dosage form assays commonly provide accuracy within
3-5% of the true value.
The ICH documents recommend that accuracy should be assessed using a minimum of ninedeterminations over a minimum of three concentration levels, covering the specified range
(i.e. three concentrations and three replicated of each concentration).
(2) Precision: -
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The precision of an analytical method is the degree of agreement among individual testresults when the method is applied repeatedly to multiple samplings of homogenous samples.
This is usually expressed as the standard deviation or the relative standard deviation(coefficient of variation). Precision is a measure of the degree of reproducibility or of the
repeatability of the analytical method under normal operating circumstances.
Repeatability involves analysis of replicates by the analyst using the same equipment and
method and conducting the precision study over short period of time while reproducibilityinvolves precision study at
Different Occasions,
Different Laboratories,
Different Batch of Reagent,
Different Analysts,
Different Equipments.
Determination of Repeatability:- Repeatability can be defined as the precision of the
procedure when repeated by same analyst under the same operating conditions (same
reagents, equipments, settings and laboratory) over a short interval of time.
It is normally expected that at least six replicates be carried out and a table showing eachindividual result provided from which the mean, standard deviation and co-efficient of
variation should be calculated for set of n value. The RSD values are important for showingdegree of variation expected when the analytical procedure is repeated several time in a
standard situation. (RSD below 1% for built drugs, RSD below 2% for assays in finishedproduct).
The ICH documents recommend that repeatability should be assessed using a minimum of
nine determinations covering the specified range for the procedure (i.e. three concentrations
and three replicates of each concentration or using a minimum of six determinations at 100%
of the test concentration).
Determination of reproducibility:- Reproducibility means the precision of the procedure
when it is carried out under different conditions-usually in different laboratories-on separate,
putatively identical samples taken from the same homogenous batch of material.
Comparisions of results obtained by different analysts, by the use of different equipments, or
by carrying out the analysis at different times can also provide valuable information.
(3) Linearity and range:-
The linearity of an analytical method is its ability to elicit test results that are directly (or by a
well defined mathematical transformation) proportional to the analyte concentration in
samples within a given range. Linearity usually expressed in terms of the variance around the
slope of regression line calculated according to an established mathematical relationship from
test results obtained by the analysis of samples with varying concentrations of analyte.
The linear range of detectability that obeys Beers law is dependent on the compound
analyzed and the detector used. The working sample concentration and samples tested for
accuracy should be in the linear range. The claim that the method is linear is to be justified
with additional mention of zero intercept by processing data by linear least square regression.
Data is processed by linear least square regression declaring the regression co-efficient and b
of the linear equation y= ax + b together with the correlation coefficient of determination r.
For the method to be linear the r value should be close to1.
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The range of an analytical method is the interval between the upper and lower levels of theanalyte (including these levels) that have been demonstrated to be determined with precision,
accuracy and linearity using the method as written.
(4) Limit of Detection and limit ofQuantitation:-
Limit of detection:- The limit of detection is the parameter of limit tests. It is the lowest level
of analyte that can be detected, but not necessarily determined in a quantitative fashion, usinga specific method under the required experimental conditions. The limit test thus merely
substantiates that the analyte concentration is above or below a certain level.
The determination of the limit of detection of instrumental procedures is carried out bydetermining the signal-to-noise ratio by comparing test results from the samples with known
concentration of analyte with those of blank samples and establishing the minimum level atwhich the analyte can be reliably detected. A signal-to-noise ratio of 2:1 or 3:1 is generally
accepted.
The signal-to-noise ratio is determined by dividing the base peak by the standard deviation of
all data points below a set threshold. Limit of detection is calculated by taking the
concentration of the peak of interest divided by three times the signal-to-noise ratio.
For spectroscopic techniques or other methods that rely upon a calibration curve for
quantitative measurements, the IUPAC approach employs the standard deviation of the
intercept (Sa) which may be related to LOD and the slope of the calibration curve, b, by
LOD = 3 Sa / b
Limit of quantitation:- Limit of quantitation is a parameter of quantitative assays for low
levels of compounds in sample matrices such as impurities in bulk drugs and degradation
products in finished pharmaceuticals. The limit of quantitation is the lowest concentration of
analyte in a sample that may be determined with acceptable accuracy and precision when the
required procedure is applied.
It is measured by analyzing samples containing known quantities of the analyte and
determining the lowest level at which acceptable degrees of accuracy and precision areattainable. Where the final assessment is based on an instrumental reading, the magnitude of
background response by analyzing a number of blank samples and calculating the standard
deviation of this response. The standard deviation multiplied by a factor (usually 10) provides
an estimate of the limit of quantitation. In many cases, the limit of quantitation is
approximately twice the limit of detection.
(5) Selectivity and Specificity:-
The selectivity of an analytical method is its ability to measure accurately and specifically the
analyte of interest in the presence of components that may be expected to be present in the
sample matrix.
If an analytical procedure is able to separate and resolve the various components of a mixture
and detect the analyte qualitatively the method is called selective. On the other hand, if the
method determines or measures quantitatively the component of interest in the sample matrix
without separation, it is said to be specific.
Hence one basic difference in the selectivity and specificity is that, while the former isrestricted to qualitative detection of the components of a sample, the latter means quantitative
measurement of one or more analyte.
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Selectivity may be expressed in terms of the bias of the assay results obtained when the procedure is applied to the analyte in the presence of expected levels of other components,
compared the results obtained when the procedure is applied to the analyte in the presence ofexpected levels of other components, compared to the results obtained on the same analyte
without added substances. When the other components are all known and available,
selectivity may be determined by comparing the test results obtained on the analyte with and
without the addition of the potentially interfering materials. When such components are eitherunidentified or unavailable, a measure of selectivity can often be obtained by determining the
recovery of a standard addition of pure analyte to a material containing a constant level of the
other components.
(6) Robustness and Ruggedness:-
Robustness:- The robustness of an analytical method is a measure of its capacity to remain
unaffected by small but deliberate variation in method parameters and provides an indication
of its reliability during normal usage. The determination of robustness requires that methods
characteristic are assessed when one or more operating parameter varied.
Ruggedness:- The ruggedness of an analytical method is the degree of reproducibility of test
results obtained by the analysis of the same samples under a variety of normal test conditionssuch as different laboratories, different analysts, using operational and environmental
conditions that may differ but are still within the specified parameters of the assay. The
testing of ruggedness is normally suggested when the method is to be used in more than one
laboratory. Ruggedness is normally expressed as the lack of the influence on the test results
of operational and environmental variables of the analytical method.
For the determination of ruggedness, the degree of reproducibility of test result is determinedas function of the assay variable. This reproducibility may be compared to the precision of
the assay under normal condition to obtain a measure of the ruggedness of the analytical
method.
(7) Stability and System suitability tests:-
Stability of the sample, standard and reagents is required for a reasonable time to generatereproducible and reliable results. For example, 24 hour stability is desired for solutions and
reagents that need to be prepared for each analysis.
System suitability test provide the added assurance that on a specific occasion the method isgiving, accurate and precise results. System suitability test are run every time a method is
used either before or during analysis. The results of each system suitability test are comparedwith defined acceptance criteria and if they pass, the method is deemed satisfactory on that
occasion. The nature of the test and the acceptance criteria will be based upon data generated
during method development optimization and validation experiments.
Data Elements Required For Assay Validation34, 35
There are various analytical methods used for the examination of pharmaceutical materials. Not all the characteristics referred above will need to be considered in all cases. Analytical
methods may be broadly classified as Per WHO as follows:
Cla ss A: Tests designed to establish identity, whether of bulk drug substances or of aparticular ingredient in a finished dosage form.
Cla ss B: Methods designed to detect and quantitative impurities in a bulk drug substance or
finished dosage form.
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Class C: Methods used to determine quantitatively the concentration of a bulk drug substanceor of a major ingredient in a finished dosage form.
Class D: Methods used to assess the characteristic of finished dosage forms, such
as dissolution profiles and content uniformity.
Table: Characteristic that should be considered for different types of analytical
procedure:
Class A Class B
Quantitative tests
Accuracy X
Precision X
Robustness X X
Linearity and range X
Selectivity X X
Limit ofDetection X
Limit of Quantitation X
Where, X indicates the tests to be performed.
As per USP:
Category I: Analytical methods for quantitation of major components of bulk drug substances
or active ingredients including preservatives in finished pharmaceutical products.
Category II: Analytical methods for determination of impurities in bulk drugs or for
determination of degradation compounds in finished pharmaceutical products.
Category III: Analytical methods for determination of performance characteristics (e.g.
dissolution, drug release).
Category IV: Identification tests.
Table: Data Elements Required for Assay Validation:
Analytical Performance Characteristics Assay Assay Category II
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Category IQuantitative tests
Accuracy X X
Precision X X
Specificity X X
Limit ofDetection
Limit of Quantitation X
Linearity X X
Range X X
Where, X indicates the tests to be performed.
Conclusion:
The efficient development and validation of analytical methods are critical elements in the
development of pharmaceuticals. Success in these areas can be attributed to several important
factors, which in turn will contribute to regulatory compliance. Experience is one of these
factors both the experience level of the individual scientists and the collective experience
level of the development and validation department.
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