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An internal standard should be used when performing MS quantitation.
An appropriate internal standard will control for extraction, HPLC
injection and ionization variability. In a complex matrix it is not
uncommon for two different standard levels in SRM integrated plots, at
the lower end of the standard curve, to give nearly an identical
response. It is only when an internal standard is used that the two points
can be differentiated. Some researchers attempt to prepare standard
curves and run samples without an internal standard and find moderate
success. Often without an internal standard % RSDs of replicates can be
as high as 20%. Using an internal standard the % RSDs can be brought
down to approximately 2%. We run triplicates at each level of our
standard curve.
How do I choose an internal standard?
The best internal standard is an isotopically labeled version of the
molecule you want to quantify. An isotopically labeled internal
standard will have a similar extraction recovery, ionization response in
ESI mass spectrometry, and a similar chromatographic retention time. If
you are performing non-clinical PK quantitation it may be difficult to
justify such a standard since a special synthesis of an isotopically
labeled standard can be expensive and time consuming. Often if you
are working with medicinal chemists they will have a library of
compound analogs that can be used as internal standards. These
.专业
.
analogs were made in the evolution of the compound to be tested and
will be similar to the compound to be quantified and more importantly
will be slightly different by parent mass. Try to avoid using
de-methylated (-14) or hydroxylated (+16) analogs as internal standards
since these are the most common mass shifts observed in natu
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