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Quantitative amino acid analysis by mass spectrometry
Vol. 2, No.2
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Feb. 1960
QUANTITATIVEAMINCACIDANAIXSIS BYMASS SBECTRCMETBY K. Biemann and W. Vetter Department of Chemistry, Massachusetts Institute Cambridge, Mass.
of Technoloa
Received February 1, 1960
The methods commonlyused for amino acid analysis employ an unspecific calorimetric
assay of the individual
ration by chromatography.
componentsafter a very careful sepa-
This latter
step makes such a procedure very
time-consuming and even with the elegant, almost fully
automatic method of
Spachan, Stein and Moore (1958) only one sample per day can be analyzed. Since a much faster but still
accurate method would be advantageous for
studies of peptide structures, vestigated the possibility
amino acid metabolism, etc.,
we have in-
of massspectrometric analysis of mixtures of
amino acids, which was expected to be speedy and accurate because prior separation into the componentswould not be necessary. The spectra of ethyJ. esters of amino acicls exhibit very intense peaks which are strictly
relatively
related to the structure
few, but
of the individual
amino acid (Biemann, Seibl and Gapp, 1959); and even the spectra of isomers, like the esters of leucine and isoleucine,
are sufficiently
the branching of the side chains to permit quantitative the massspectrometric
quantitative
different
discrimination.
because of Thus,
analysis of such mixtures should be pos-
sible in much the sameway as the hydrocarbon analysis which is now widely used in the petroleum industry
(for a review see Dibeler,
However, the extension of this principle
to the analysis of free amino
acids is complicated by the necessity to esterify reproducibly)
1956).
quantitatively
(or at least
the very small amount of the mixture commonlyavailable
a determination,
for such
to convert it to the free esters and to introduce these into 93
Vol. 2, No. 2
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
the mass spectrometer without fractionation
in any one of these steps.
We have now achieved this in the following way: milligram)
is refluxed
Feb. 1960
with 2 ml. anhydrous ethanolic
The mixture (about one hydrochloric
acid (5-l@)
for three hours, the solvent evaporated in a vacuum desiccator and the residue dissolved (or susperidedin 2 ml. dichloromethane.
The hydrochlorides
are con-
verted to the free esters by passing anhydrous ammoniathrough the solution for a few seconds; the solution
is then filtered
into a small, long-necked bulb type distilling is distilled to -60°,
off.
tube and most of the solvent
The tube is then connected to the massspectrometer, cooled
and the remaining dichloromethane is pumpedoff through the oil dif-
fusion pump of the inlet into the inlet to 160°,
from the ammoniumchloride
system. The mixture of esters is then introduced
system of the mass spectrometeti by rapidly
heating the tube
and the spectrum is scanned from mass25 to 200.
Calibratirm
spectra of each individual
the samemanner, using an authentic
amino acid have been obtained in
sample. The relative
peaks used for the measurementof the individual
intensities
amino acids (its massnumber
is given in column 2, Fig. 1) were determined from synthetic
mixtures of known
caaposition containing aspartic acid or phenylalanine as internal The calculation
of the results is facilitated
amino esters exhibit
standard.
by the fact that marry of the
a strong peak with little
and thus can be subtracted one after
of the
or no interference
from others
the other from the spectrum.
The few
remaining ones are obtained by one or two successive approximations or by the use of simultaneous equations. Table I gives the results of somepreliminary mtitures
of amino acids, presented as the relative
rather than the absolute amount, are of interest the necessity of quantitative
transfer
determinations on synthetic molar ratios
in most cases, eliminating
of the sample during the preparation.
However, this could be done without major changes, if essential. found deviate l-5$ *
since these,
from the calculated
The values
ones; as can be seen from Table I, the
A c3c 21-103~ mass spectrometer, equipped with a heated inlet operated at 140°, was.used in these experiments. 94
system,
vol.
2, NO. 2
BIOCHEMICAL
Feb. 1960
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABIJ-3I Amino Acid
Mass Number' L
zl-Y ala abu val leu ileu
Mixture A Calcd. Foundh 2.64Q 2.63 1.73 1.85 1.87
1.30
v-0 ser thr
1.75 1.84 1.83
Mixture B Calcd. Foundi 2.16 2.09 1.28 1.31
Mixture C Calcd. Foundj
1.32
1.41
opr0 met
1.40
Me tyr asp glu orn
1.00
1.00
1.03 1.40
1.05 1.41
3.10
3.27
1.44
1.42
0.98 1.01
0.98 1.00
1.00
1.00
1.41 1.66 1.18
1.38 1.68 1.17
1.43
1.44
1.00
Mixture D Calcd. Foundj
1.02
1.60
1.65
1.00 0.80
1.03 0.76 1.21
1.19
(a) m/e of peak used for calculation. (b) (R-CR-NHa)+fragment of (c) originates through further fragmentation of (b). R-CR(NHH2)C0aCaH . 5 . (e) (H~-c?H~)+. (f) fragment of orn-lactam. (d) (CHs-S-C&.) (g) values represent molar ratios. (j) average of 3 determinations.
(h) average of 2, (i) average of 4,
accuracy varies somewhatfor the different
amino acids and also depends on the
particular
At present, we are trying
composition of the mixture.
accuracy obtained with ornithine
and tyrosine
the more commonamino acids not listed
to improve the
and to extend the method to someof
in the table,
like tryptophan,
histidine,
cysteine and, if possible, arginine. Webelieve the main advantage of this new approach to be the speed of the analysis;
each determination requires only 30-40 minutes instrument time, thus
allowing the analysis of a larger number of samples than hitherto following
possible.
the total
This
may be an important factor
in many studies, e.g.,
hydrolysis
of a peptide, multiplicate
analysis of mixtures to increase the confidence in the
results obtained, determination of the amino acid composition of the large number of small peptides obtained in the partial 95
hydrolysis
of proteins,
etc.
Further-
Vol. 2, No. 2
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
more, new amino acids can be analyzed accordingly, calibration
Feb. 1960
once a small, pure sample for
is available.
This investigation National Institutes
was supported by a research grant (RG-5472) from the
of Health, Public Health Service.
References K. Biemann, J. Seibl and F. Gapp, Biochem. Biophys. Res. Comm.,1, 307 (1959). V. H. Dibeler in "Organic Analysis,"
Vol. III,
Interscience
Pub., NewYork, 1956,
P. 387 ff. D. H. Spackman, W. H. stein and S. Moore, Anal. Chem., z(l, 1190 (1.958).
96
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Feb. 1960
QUANTITATIVEAMINCACIDANAIXSIS BYMASS SBECTRCMETBY K. Biemann and W. Vetter Department of Chemistry, Massachusetts Institute Cambridge, Mass.
of Technoloa
Received February 1, 1960
The methods commonlyused for amino acid analysis employ an unspecific calorimetric
assay of the individual
ration by chromatography.
componentsafter a very careful sepa-
This latter
step makes such a procedure very
time-consuming and even with the elegant, almost fully
automatic method of
Spachan, Stein and Moore (1958) only one sample per day can be analyzed. Since a much faster but still
accurate method would be advantageous for
studies of peptide structures, vestigated the possibility
amino acid metabolism, etc.,
we have in-
of massspectrometric analysis of mixtures of
amino acids, which was expected to be speedy and accurate because prior separation into the componentswould not be necessary. The spectra of ethyJ. esters of amino acicls exhibit very intense peaks which are strictly
relatively
related to the structure
few, but
of the individual
amino acid (Biemann, Seibl and Gapp, 1959); and even the spectra of isomers, like the esters of leucine and isoleucine,
are sufficiently
the branching of the side chains to permit quantitative the massspectrometric
quantitative
different
discrimination.
because of Thus,
analysis of such mixtures should be pos-
sible in much the sameway as the hydrocarbon analysis which is now widely used in the petroleum industry
(for a review see Dibeler,
However, the extension of this principle
to the analysis of free amino
acids is complicated by the necessity to esterify reproducibly)
1956).
quantitatively
(or at least
the very small amount of the mixture commonlyavailable
a determination,
for such
to convert it to the free esters and to introduce these into 93
Vol. 2, No. 2
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
the mass spectrometer without fractionation
in any one of these steps.
We have now achieved this in the following way: milligram)
is refluxed
Feb. 1960
with 2 ml. anhydrous ethanolic
The mixture (about one hydrochloric
acid (5-l@)
for three hours, the solvent evaporated in a vacuum desiccator and the residue dissolved (or susperidedin 2 ml. dichloromethane.
The hydrochlorides
are con-
verted to the free esters by passing anhydrous ammoniathrough the solution for a few seconds; the solution
is then filtered
into a small, long-necked bulb type distilling is distilled to -60°,
off.
tube and most of the solvent
The tube is then connected to the massspectrometer, cooled
and the remaining dichloromethane is pumpedoff through the oil dif-
fusion pump of the inlet into the inlet to 160°,
from the ammoniumchloride
system. The mixture of esters is then introduced
system of the mass spectrometeti by rapidly
heating the tube
and the spectrum is scanned from mass25 to 200.
Calibratirm
spectra of each individual
the samemanner, using an authentic
amino acid have been obtained in
sample. The relative
peaks used for the measurementof the individual
intensities
amino acids (its massnumber
is given in column 2, Fig. 1) were determined from synthetic
mixtures of known
caaposition containing aspartic acid or phenylalanine as internal The calculation
of the results is facilitated
amino esters exhibit
standard.
by the fact that marry of the
a strong peak with little
and thus can be subtracted one after
of the
or no interference
from others
the other from the spectrum.
The few
remaining ones are obtained by one or two successive approximations or by the use of simultaneous equations. Table I gives the results of somepreliminary mtitures
of amino acids, presented as the relative
rather than the absolute amount, are of interest the necessity of quantitative
transfer
determinations on synthetic molar ratios
in most cases, eliminating
of the sample during the preparation.
However, this could be done without major changes, if essential. found deviate l-5$ *
since these,
from the calculated
The values
ones; as can be seen from Table I, the
A c3c 21-103~ mass spectrometer, equipped with a heated inlet operated at 140°, was.used in these experiments. 94
system,
vol.
2, NO. 2
BIOCHEMICAL
Feb. 1960
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABIJ-3I Amino Acid
Mass Number' L
zl-Y ala abu val leu ileu
Mixture A Calcd. Foundh 2.64Q 2.63 1.73 1.85 1.87
1.30
v-0 ser thr
1.75 1.84 1.83
Mixture B Calcd. Foundi 2.16 2.09 1.28 1.31
Mixture C Calcd. Foundj
1.32
1.41
opr0 met
1.40
Me tyr asp glu orn
1.00
1.00
1.03 1.40
1.05 1.41
3.10
3.27
1.44
1.42
0.98 1.01
0.98 1.00
1.00
1.00
1.41 1.66 1.18
1.38 1.68 1.17
1.43
1.44
1.00
Mixture D Calcd. Foundj
1.02
1.60
1.65
1.00 0.80
1.03 0.76 1.21
1.19
(a) m/e of peak used for calculation. (b) (R-CR-NHa)+fragment of (c) originates through further fragmentation of (b). R-CR(NHH2)C0aCaH . 5 . (e) (H~-c?H~)+. (f) fragment of orn-lactam. (d) (CHs-S-C&.) (g) values represent molar ratios. (j) average of 3 determinations.
(h) average of 2, (i) average of 4,
accuracy varies somewhatfor the different
amino acids and also depends on the
particular
At present, we are trying
composition of the mixture.
accuracy obtained with ornithine
and tyrosine
the more commonamino acids not listed
to improve the
and to extend the method to someof
in the table,
like tryptophan,
histidine,
cysteine and, if possible, arginine. Webelieve the main advantage of this new approach to be the speed of the analysis;
each determination requires only 30-40 minutes instrument time, thus
allowing the analysis of a larger number of samples than hitherto following
possible.
the total
This
may be an important factor
in many studies, e.g.,
hydrolysis
of a peptide, multiplicate
analysis of mixtures to increase the confidence in the
results obtained, determination of the amino acid composition of the large number of small peptides obtained in the partial 95
hydrolysis
of proteins,
etc.
Further-
Vol. 2, No. 2
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
more, new amino acids can be analyzed accordingly, calibration
Feb. 1960
once a small, pure sample for
is available.
This investigation National Institutes
was supported by a research grant (RG-5472) from the
of Health, Public Health Service.
References K. Biemann, J. Seibl and F. Gapp, Biochem. Biophys. Res. Comm.,1, 307 (1959). V. H. Dibeler in "Organic Analysis,"
Vol. III,
Interscience
Pub., NewYork, 1956,
P. 387 ff. D. H. Spackman, W. H. stein and S. Moore, Anal. Chem., z(l, 1190 (1.958).
96