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PART – I
Laboratory Errors
Pharma Uptoday

pharmauptoday@gmail.com
ERROR

Error is the difference between the true result (or
accepted true result) and the measured result.
If the error in an analysis is large, serious
consequences may result.
A patient may undergo expensive and even
dangerous medical treatment based on an incorrect
laboratory result may implement costly and incorrect
modifications to a plant or process because of an
analytical error.
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Types of Errors

There are two principal types of error in analysis
determinate or systematic error
indeterminate or random error

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Determinate Error

Determinate errors are caused by faults in the
analytical procedure or the instruments used in the
analysis.
The name determinate error implies that the cause of
this type of error may be found out and then either
avoided or corrected.
Determinate errors are systematic errors; that is, they
are not random.
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Determinate Error

A particular determinate error may cause the
analytical results produced by the method to be
always too high;
Another determinate error may render all results too
low.
Sometimes the error is constant;
All results are too high (or too low) by the same
amount.
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Determinate Error

Sometimes the determinate error is proportional to
the true result, giving rise to proportional errors.
Other determinate errors may be variable in both sign
and magnitude, such as the change in the volume of a
solution as the temperature changes. Although this
variation can be positive or negative, it can be
identified and accounted for.

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Determinate Error

Determinate errors can be additive or they can be
multiplicative. It depends on the error and how it
enters into the calculation of the final result.
This determinate error could be the result of an
incorrectly calibrated balance.

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Determinate Error

If the balance is set so that the zero point is actually 0.5 mg
too high, all masses determined with this balance will be
0.5 mg too high.
If this balance was used to weigh any standard solution
used in the laboratory, the standard concentration will be
erroneously high, and all of the results obtained using this
standard will be erroneously low.
The error is reported as the absolute error, the absolute
value of the difference between the true and measured
values.
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Determinate Error

Determinate errors arise from some faulty step in the
analytical process.
The faulty step is repeated every time the
determination is performed. Whether a sample is
analyzed 5 times or 50 times, the results may all agree
with each other (good precision) but differ widely
from the true answer (poor accuracy).
Although the replicate results are close to each
other, that tells us nothing about their accuracy.
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Determinate Error
Systematic error is under the control of the analyst. It is the analyst’s
responsibility to recognize and correct for these systematic errors that cause
results to be biased, that is, offset in the average measured value from the
true value.
How are determinate errors identified and corrected?
Two methods are commonly used to identify the existence of systematic
errors.
One is to analyze the sample by a completely different analytical procedure
that is known to involve no systematic errors. Such methods are often called
“standard methods”; they have been evaluated extensively by many
laboratories and shown to be accurate and precise.
If the results from the two analytical methods agree, it is reasonable to
assume that both analytical procedures are free of determinate errors.
The second method is to run several analyses of a reference material of
known, accepted concentration of analyte. The difference between the
known (true) concentration and that measured by analysis should reveal the
error. If the results of analysis of a known reference standard are
consistently high (or consistently low), then a determinate error is involved
in the method.
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Determinate Error
The cause of the error must be identified and either
eliminated or controlled if the analytical procedure is to
give accurate results.
Many clinical and analytical laboratories participate in
proficiency testing programs, where “unknown”
standard samples are sent to the laboratory on a regular
basis.
The results of these samples are sent to the government
or professional agency running the program. The
unknowns are of course known to the agency that sent
the test samples; the laboratory receives a report on the
accuracy and precision of its performance.
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Determinate Error

Determinate errors can arise from uncalibrated
balances, improperly calibrated volumetric flasks or
pipettes, malfunctioning instrumentation, impure
chemicals, incorrect analytical procedures or
techniques, and analyst error.

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Determinate Error
Analyst error : The person performing the analysis causes
these errors.
They may be the result of inexperience, insufficient
training, or being “in a hurry”.
An analyst may use the instrument incorrectly,
perhaps by placing the sample in the instrument incorrectly
each time.
Setting the instrument to the wrong conditions for analysis.
Consistently misreading a meniscus in a volumetric flask as
high (or low)
Improper use of pipettes, such as “blowing out” the liquid
from a volumetric pipette.
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Determinate Error
Operational and personal errors
These are due to factors for which the individual analyst is responsible
and are not connected with the method or procedure: they form part of
the 'personal equation' of an observer.
The errors are mostly physical in nature and occur when sound analytical
technique is not followed.
Examples are:






mechanical loss of materials in various steps of an analysis
underwashing or overwashing of precipitates
ignition of precipitates at incorrect temperatures
insufficient cooling of crucibles before weighing
allowing hygroscopic materials to absorb moisture before or during
weighing
 use of reagents containing harmful impurities.

Some analysts are unable to judge colour changes sharply in visual
titrations, which may result in a slight overstepping of the end point.
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Determinate Error
Some other analyst-related errors are
Carelessness, which is not as common as is generally
believed
Transcription errors, that is, copying the wrong
information into a lab notebook or onto a label
Calculation errors.

Proper training, experience, and attention to detail on
the part of the analyst can correct these types of
errors.

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Determinate Error
Reagents and instrumentation:
Contaminated or decomposed reagents can cause
determinate errors.
Impurities in the reagents may interfere with the
determination of the analyte, especially at the ppm
level or below.
Prepared reagents may also be improperly labeled.
The suspect reagent may be tested for purity using a
known procedure or the analysis should be redone
using a different set of reagents and the results
compared.
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Determinate Error
Numerous errors involving instrumentation are possible, including
faulty construction of balances,
use of uncalibrated or improperly calibrated weights,
incorrect instrument alignment,
incorrect wavelength settings,
incorrect reading of values, and
incorrect settings of the readout (i.e., zero signal should read zero).
Any variation in proper instrument settings can lead to errors.

These problems can be eliminated by a systematic procedure to
check the instrument settings and operation before use. Such
procedures are called standard operating procedures (SOPs) in
many labs.
There should be a written SOP for each instrument and each
analytical method used in the laboratory.
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Determinate Error
In instrumental analysis, electrical line voltage fluctuations are
a particular problem. This is especially true for automated
instruments running unattended overnight.
Instruments are often calibrated during the day, when
electrical power is in high demand.
At night, when power demand is lower, line voltage may
increase substantially, completely changing the relationship
between concentration of analyte and measured signal.
Regulated power supplies are highly recommended for
analytical instruments. The procedure for unattended analysis
should include sufficient calibration checks during the
analytical run to identify such problems.
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Determinate Error
Analytical method
The most serious errors are those in the method itself.
Examples of method errors include
incorrect sampling
incomplete reaction for chemical methods,
unexpected interferences from the sample itself or reagents used
having the analyte in the wrong oxidation state for the measurement
loss of analyte during sample preparation by volatilization or precipitation
an error in calculation based on incorrect assumptions in the procedure
(errors can evolve from assignment of an incorrect formula or molecular
weight to the sample).

In titrimetric analysis errors may occur
owing to failure of reactions to proceed to completion,
occurrence of induced and side reactions,
reaction of substances other than the constituent being determined,
difference between the observed end point and the stoichiometric
equivalence point of a reaction.
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Determinate Error
Contamination
Contamination of samples by external sources can be a
serious source of error and may be extremely variable.
Aluminum levels in the dust in a normal laboratory are so
high that dust prohibits the determination of low ppb levels
of aluminum in samples.
A special dust-free “clean lab” or “clean bench” with a filter
to remove small dust particles may be required, for
determination of traces of aluminum, silicon, and other
common elements such as iron.
When trace (< ppm level) or ultratrace (< ppb level) organic
and inorganic analysis is required, the laboratory
environment can be a significant source of contamination.
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Determinate Error
Contamination
Another major source of contamination in an analysis can be the
analyst. It depends on what kind of analytes are being measured, but
when trace or ultratrace levels of elements or molecules are being
determined, the analyst can be a part of the analytical problem.
Many
personal
care
items,
such
as
hand
creams, shampoos, powders, and cosmetics, contain significant
amounts of chemicals that may be analytes.
The problem can be severe for volatile organic compounds in
aftershave, perfume, and many other scented products and for
silicone polymers, used in many health and beauty products.
Powdered gloves may contain a variety of trace elements and should
not be used by analysts performing trace element determinations.
Hair, skin, and clothing can shed cells or fibers that can contaminate a
sample.

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Indeterminate Error
Indeterminate errors are not constant or biased.
They are random in nature and are the cause of slight
variations in results of replicate samples made by the same
analyst under the same conditions.
Sources of random error include the limitations of reading
balances, scales such as rulers or dials, and electrical “noise” in
instruments. For example, a balance that is capable of
measuring only to 0.001 g cannot distinguish between two
samples with masses of 1.0151 and 1.0149 g. In one case the
measured mass is low, in the other case it is high.
pharmauptoday@gmail.com
Indeterminate Error
Indeterminate errors are not constant or biased.
They are random in nature and are the cause of slight
variations in results of replicate samples made by the same
analyst under the same conditions.
Sources of random error include the limitations of reading
balances, scales such as rulers or dials, and electrical “noise”
in instruments. For example, a balance that is capable of
measuring only to 0.001 g cannot distinguish between two
samples with masses of 1.0151 and 1.0149 g. In one case the
measured mass is low, in the other case it is high.
pharmauptoday@gmail.com
Indeterminate Error
These random errors cause variation in results, some of which may
be too high and some too low.
The average of the replicate determinations is accurate, but each
individual determination may vary slightly from the true value.
Indeterminate errors arise from sources that cannot be
corrected, avoided, or even identified, in some cases.
All analytical procedures are subject to indeterminate error.
However, because indeterminate error is random, the errors will
follow a random distribution.
This distribution can be understood using the laws of probability
and basic statistics. The extent of indeterminate error can be
calculated mathematically.
pharmauptoday@gmail.com
Gross Error
Gross errors differ from indeterminate and determinate errors.
They usually occur only occasionally, are often large, and may cause
a result to be either high or low.
They are often the product of human errors.
For example,
if part of a precipitate is lost before weighing, analytical results will be
low.
Touching a weighing bottle with your fingers after its empty mass is
determined will cause a high mass reading for a solid weighed in the
contaminated bottle.

Gross errors lead to outliers, results that appear to differ markedly
from all other data in a set of replicate measurements.
pharmauptoday@gmail.com
Absolute & Relative errors
An absolute error is the numerical difference between a
measured value and a true or accepted value.
A relative error is the absolute error divided by the true or
accepted value.

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Common identified error
Concentration errors
Labeling errors
Calculation errors
Manual calculation
Using wrong formula

Computational calculation
Using wrong formula in excel
Using different location (wrong cell) in the excel sheet
Improper use of $, () symbols.

Rounding off errors
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Rejection of Results
When a set of replicate results is obtained it may be the case that
one of the results appears to be “out of line”; such a result is called
an outlier.
While it is tempting to discard data that does not “look good” in
order to make the analysis seem more precise, it is never a good
practice unless there is justification for discarding the result.
If it is known that an error was made,
such as spillage of the sample,
use of the wrong size pipet,
incorrect dilution, or
allowing the sample to boil to dryness when it should not have done

so, the result should be rejected and not used in any compilation of
results.
In practice, if something of this sort is suspected, a good analyst will
discard the sample and start over if possible.
pharmauptoday@gmail.com
PART – II
UNDERSTAND THE IMPORTANCE
OF EACH STEP TO MINIMISE
ERRORS

pharmauptoday@gmail.com
References
Text book of Quantitative Chemical Analysis- 5th Edition –Vogel.
Pharmaceutical Analysis : A Textbook for Pharmacy Students &
Pharmaceutical Chemists – David G. Watson
Handbook of instrumental techniques for analytical chemistry –
Frank Settle.
Instant Notes in Analytical Chemistry – D. Kealey & P.J. Haines.
Analytical Chemistry for Technicians 3rd edition (CRC, 2003) –
Kenkel.
pharmaceutical-drug-analysis book 2nd edition – Ashutoshkar.
Fundamentals of Analytical Chemistry 8th edition HQ
(Thomson, 2004) – Douglas A. Skoog.
Undergraduate instrumental analysis 6th edition – James W.
Robinson.
pharmauptoday@gmail.com

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Laboratory Errors: Causes and Corrections

  • 1. PART – I Laboratory Errors Pharma Uptoday pharmauptoday@gmail.com
  • 2. ERROR Error is the difference between the true result (or accepted true result) and the measured result. If the error in an analysis is large, serious consequences may result. A patient may undergo expensive and even dangerous medical treatment based on an incorrect laboratory result may implement costly and incorrect modifications to a plant or process because of an analytical error. pharmauptoday@gmail.com
  • 3. Types of Errors There are two principal types of error in analysis determinate or systematic error indeterminate or random error pharmauptoday@gmail.com
  • 4. Determinate Error Determinate errors are caused by faults in the analytical procedure or the instruments used in the analysis. The name determinate error implies that the cause of this type of error may be found out and then either avoided or corrected. Determinate errors are systematic errors; that is, they are not random. pharmauptoday@gmail.com
  • 5. Determinate Error A particular determinate error may cause the analytical results produced by the method to be always too high; Another determinate error may render all results too low. Sometimes the error is constant; All results are too high (or too low) by the same amount. pharmauptoday@gmail.com
  • 6. Determinate Error Sometimes the determinate error is proportional to the true result, giving rise to proportional errors. Other determinate errors may be variable in both sign and magnitude, such as the change in the volume of a solution as the temperature changes. Although this variation can be positive or negative, it can be identified and accounted for. pharmauptoday@gmail.com
  • 7. Determinate Error Determinate errors can be additive or they can be multiplicative. It depends on the error and how it enters into the calculation of the final result. This determinate error could be the result of an incorrectly calibrated balance. pharmauptoday@gmail.com
  • 8. Determinate Error If the balance is set so that the zero point is actually 0.5 mg too high, all masses determined with this balance will be 0.5 mg too high. If this balance was used to weigh any standard solution used in the laboratory, the standard concentration will be erroneously high, and all of the results obtained using this standard will be erroneously low. The error is reported as the absolute error, the absolute value of the difference between the true and measured values. pharmauptoday@gmail.com
  • 9. Determinate Error Determinate errors arise from some faulty step in the analytical process. The faulty step is repeated every time the determination is performed. Whether a sample is analyzed 5 times or 50 times, the results may all agree with each other (good precision) but differ widely from the true answer (poor accuracy). Although the replicate results are close to each other, that tells us nothing about their accuracy. pharmauptoday@gmail.com
  • 10. Determinate Error Systematic error is under the control of the analyst. It is the analyst’s responsibility to recognize and correct for these systematic errors that cause results to be biased, that is, offset in the average measured value from the true value. How are determinate errors identified and corrected? Two methods are commonly used to identify the existence of systematic errors. One is to analyze the sample by a completely different analytical procedure that is known to involve no systematic errors. Such methods are often called “standard methods”; they have been evaluated extensively by many laboratories and shown to be accurate and precise. If the results from the two analytical methods agree, it is reasonable to assume that both analytical procedures are free of determinate errors. The second method is to run several analyses of a reference material of known, accepted concentration of analyte. The difference between the known (true) concentration and that measured by analysis should reveal the error. If the results of analysis of a known reference standard are consistently high (or consistently low), then a determinate error is involved in the method. pharmauptoday@gmail.com
  • 11. Determinate Error The cause of the error must be identified and either eliminated or controlled if the analytical procedure is to give accurate results. Many clinical and analytical laboratories participate in proficiency testing programs, where “unknown” standard samples are sent to the laboratory on a regular basis. The results of these samples are sent to the government or professional agency running the program. The unknowns are of course known to the agency that sent the test samples; the laboratory receives a report on the accuracy and precision of its performance. pharmauptoday@gmail.com
  • 12. Determinate Error Determinate errors can arise from uncalibrated balances, improperly calibrated volumetric flasks or pipettes, malfunctioning instrumentation, impure chemicals, incorrect analytical procedures or techniques, and analyst error. pharmauptoday@gmail.com
  • 13. Determinate Error Analyst error : The person performing the analysis causes these errors. They may be the result of inexperience, insufficient training, or being “in a hurry”. An analyst may use the instrument incorrectly, perhaps by placing the sample in the instrument incorrectly each time. Setting the instrument to the wrong conditions for analysis. Consistently misreading a meniscus in a volumetric flask as high (or low) Improper use of pipettes, such as “blowing out” the liquid from a volumetric pipette. pharmauptoday@gmail.com
  • 14. Determinate Error Operational and personal errors These are due to factors for which the individual analyst is responsible and are not connected with the method or procedure: they form part of the 'personal equation' of an observer. The errors are mostly physical in nature and occur when sound analytical technique is not followed. Examples are:      mechanical loss of materials in various steps of an analysis underwashing or overwashing of precipitates ignition of precipitates at incorrect temperatures insufficient cooling of crucibles before weighing allowing hygroscopic materials to absorb moisture before or during weighing  use of reagents containing harmful impurities. Some analysts are unable to judge colour changes sharply in visual titrations, which may result in a slight overstepping of the end point. pharmauptoday@gmail.com
  • 15. Determinate Error Some other analyst-related errors are Carelessness, which is not as common as is generally believed Transcription errors, that is, copying the wrong information into a lab notebook or onto a label Calculation errors. Proper training, experience, and attention to detail on the part of the analyst can correct these types of errors. pharmauptoday@gmail.com
  • 16. Determinate Error Reagents and instrumentation: Contaminated or decomposed reagents can cause determinate errors. Impurities in the reagents may interfere with the determination of the analyte, especially at the ppm level or below. Prepared reagents may also be improperly labeled. The suspect reagent may be tested for purity using a known procedure or the analysis should be redone using a different set of reagents and the results compared. pharmauptoday@gmail.com
  • 17. Determinate Error Numerous errors involving instrumentation are possible, including faulty construction of balances, use of uncalibrated or improperly calibrated weights, incorrect instrument alignment, incorrect wavelength settings, incorrect reading of values, and incorrect settings of the readout (i.e., zero signal should read zero). Any variation in proper instrument settings can lead to errors. These problems can be eliminated by a systematic procedure to check the instrument settings and operation before use. Such procedures are called standard operating procedures (SOPs) in many labs. There should be a written SOP for each instrument and each analytical method used in the laboratory. pharmauptoday@gmail.com
  • 18. Determinate Error In instrumental analysis, electrical line voltage fluctuations are a particular problem. This is especially true for automated instruments running unattended overnight. Instruments are often calibrated during the day, when electrical power is in high demand. At night, when power demand is lower, line voltage may increase substantially, completely changing the relationship between concentration of analyte and measured signal. Regulated power supplies are highly recommended for analytical instruments. The procedure for unattended analysis should include sufficient calibration checks during the analytical run to identify such problems. pharmauptoday@gmail.com
  • 19. Determinate Error Analytical method The most serious errors are those in the method itself. Examples of method errors include incorrect sampling incomplete reaction for chemical methods, unexpected interferences from the sample itself or reagents used having the analyte in the wrong oxidation state for the measurement loss of analyte during sample preparation by volatilization or precipitation an error in calculation based on incorrect assumptions in the procedure (errors can evolve from assignment of an incorrect formula or molecular weight to the sample). In titrimetric analysis errors may occur owing to failure of reactions to proceed to completion, occurrence of induced and side reactions, reaction of substances other than the constituent being determined, difference between the observed end point and the stoichiometric equivalence point of a reaction. pharmauptoday@gmail.com
  • 20. Determinate Error Contamination Contamination of samples by external sources can be a serious source of error and may be extremely variable. Aluminum levels in the dust in a normal laboratory are so high that dust prohibits the determination of low ppb levels of aluminum in samples. A special dust-free “clean lab” or “clean bench” with a filter to remove small dust particles may be required, for determination of traces of aluminum, silicon, and other common elements such as iron. When trace (< ppm level) or ultratrace (< ppb level) organic and inorganic analysis is required, the laboratory environment can be a significant source of contamination. pharmauptoday@gmail.com
  • 21. Determinate Error Contamination Another major source of contamination in an analysis can be the analyst. It depends on what kind of analytes are being measured, but when trace or ultratrace levels of elements or molecules are being determined, the analyst can be a part of the analytical problem. Many personal care items, such as hand creams, shampoos, powders, and cosmetics, contain significant amounts of chemicals that may be analytes. The problem can be severe for volatile organic compounds in aftershave, perfume, and many other scented products and for silicone polymers, used in many health and beauty products. Powdered gloves may contain a variety of trace elements and should not be used by analysts performing trace element determinations. Hair, skin, and clothing can shed cells or fibers that can contaminate a sample. pharmauptoday@gmail.com
  • 22. Indeterminate Error Indeterminate errors are not constant or biased. They are random in nature and are the cause of slight variations in results of replicate samples made by the same analyst under the same conditions. Sources of random error include the limitations of reading balances, scales such as rulers or dials, and electrical “noise” in instruments. For example, a balance that is capable of measuring only to 0.001 g cannot distinguish between two samples with masses of 1.0151 and 1.0149 g. In one case the measured mass is low, in the other case it is high. pharmauptoday@gmail.com
  • 23. Indeterminate Error Indeterminate errors are not constant or biased. They are random in nature and are the cause of slight variations in results of replicate samples made by the same analyst under the same conditions. Sources of random error include the limitations of reading balances, scales such as rulers or dials, and electrical “noise” in instruments. For example, a balance that is capable of measuring only to 0.001 g cannot distinguish between two samples with masses of 1.0151 and 1.0149 g. In one case the measured mass is low, in the other case it is high. pharmauptoday@gmail.com
  • 24. Indeterminate Error These random errors cause variation in results, some of which may be too high and some too low. The average of the replicate determinations is accurate, but each individual determination may vary slightly from the true value. Indeterminate errors arise from sources that cannot be corrected, avoided, or even identified, in some cases. All analytical procedures are subject to indeterminate error. However, because indeterminate error is random, the errors will follow a random distribution. This distribution can be understood using the laws of probability and basic statistics. The extent of indeterminate error can be calculated mathematically. pharmauptoday@gmail.com
  • 25. Gross Error Gross errors differ from indeterminate and determinate errors. They usually occur only occasionally, are often large, and may cause a result to be either high or low. They are often the product of human errors. For example, if part of a precipitate is lost before weighing, analytical results will be low. Touching a weighing bottle with your fingers after its empty mass is determined will cause a high mass reading for a solid weighed in the contaminated bottle. Gross errors lead to outliers, results that appear to differ markedly from all other data in a set of replicate measurements. pharmauptoday@gmail.com
  • 26. Absolute & Relative errors An absolute error is the numerical difference between a measured value and a true or accepted value. A relative error is the absolute error divided by the true or accepted value. pharmauptoday@gmail.com
  • 27. Common identified error Concentration errors Labeling errors Calculation errors Manual calculation Using wrong formula Computational calculation Using wrong formula in excel Using different location (wrong cell) in the excel sheet Improper use of $, () symbols. Rounding off errors pharmauptoday@gmail.com
  • 28. Rejection of Results When a set of replicate results is obtained it may be the case that one of the results appears to be “out of line”; such a result is called an outlier. While it is tempting to discard data that does not “look good” in order to make the analysis seem more precise, it is never a good practice unless there is justification for discarding the result. If it is known that an error was made, such as spillage of the sample, use of the wrong size pipet, incorrect dilution, or allowing the sample to boil to dryness when it should not have done so, the result should be rejected and not used in any compilation of results. In practice, if something of this sort is suspected, a good analyst will discard the sample and start over if possible. pharmauptoday@gmail.com
  • 29. PART – II UNDERSTAND THE IMPORTANCE OF EACH STEP TO MINIMISE ERRORS pharmauptoday@gmail.com
  • 30. References Text book of Quantitative Chemical Analysis- 5th Edition –Vogel. Pharmaceutical Analysis : A Textbook for Pharmacy Students & Pharmaceutical Chemists – David G. Watson Handbook of instrumental techniques for analytical chemistry – Frank Settle. Instant Notes in Analytical Chemistry – D. Kealey & P.J. Haines. Analytical Chemistry for Technicians 3rd edition (CRC, 2003) – Kenkel. pharmaceutical-drug-analysis book 2nd edition – Ashutoshkar. Fundamentals of Analytical Chemistry 8th edition HQ (Thomson, 2004) – Douglas A. Skoog. Undergraduate instrumental analysis 6th edition – James W. Robinson. pharmauptoday@gmail.com