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Determination of active hydrogen content by fast atom bombardment mass spectrometry following hydrogen-deuterium exchange
Vol. 112, No. 1, 1983 April
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
15, 1983
Pages
DETERMINATION
OF ACTIVE
MASS
SPECTROMETRY
Satinder
K.
February
CONTENT
FOLLOWING
Sethi,
Departments University
Received
HYDROGEN
David
of
Medicinal Utah,
of
BY FAST
ATOM
HYDROGEN-DEUTERIUM
L.
Smith
and
Salt
Chemistry Lake
BOMBARDMENT
EXCHANGE
James and
126-131
A.
McCloskey
Biochemistry Utah 84112
City,
25, 1983
Fast atom bombardyent mass spectroyetry following hydrogen - deuterium H20 has been studied as a means of exchanqe in [hydroxyH31glyCWOl and establ;shing active hydrogen content in molecules of unknown structure. one peptide and complex antibiotics, in the mass Nucleotides, carbohydrates, region to 1500 daltons and 29 exchangeable hydrogens were examined, with a correct hydrogen count unambiguously measured in every case. The Imethod is experimentally simple and applicable on a microgram scale, to salts and a variety of polar compounds of biological origin. Knowledge structure This
knowledge
of
an
the
a useful
tization,
or
nuclear
magnetic
methods
become
content
increases.
from
beyond
conditions exchange
Abbreviations
0006-291X/83
is of
4-6 in
atoms
are
principle
FAB, have
useful
hydrogens fast been
atom
groups,
H2
chemical (l),
deriva-
proton -
Unfortunately, the
often
limited
by
active
hydrogen because
back-exchange,
serious
deutethese
favorable
exchange
and
functional
hydrogen
as
but
of by
of
to
under
chemical
errors
bombardment; by
$1.50
126
M, 'H.
molecule
in
of
which
can
ioniresult
(6,7).
exchanged
Copyright 13 1983 bv Academic Press, Inc. All rights of reproduction in any form reserved.
inferred
are
(3-5)
strucand
functional
(2).
Gas-phase
unknown
overall
arrangement
ambiguous
usually
of
following
methods
hydrogens.
non-labile
used: hydrogen
but
be
system
results
spectrometric
sensitivity,
or and
often
of
composition,
liberation
inlet
the
deduction
spectrometry
or
and
Mass
severe
active
source
a molecule
elemental
chemical
mass
the
identity can
by or
inaccurate
microgram-level
zation
directly
of
subunits
the content
resonance,
to
structural
determining
ion
in
complementary
hydrogen
the
content
constraint
of
in
measured
in
hydrogen
important
identities
active
exchange
active
is
role
The
becomes
exact
information
groups.
rium
the
provides
ture.
plays
of
which
all
Vol.
112,
No.
The having
1, 1983
Irecent
development
a major
and
natural
impact
tent
for
molecules
imp-ovemellt
over
spectrome.try
for
been
active
in
of
this
region
The
the in
et
al.
the
have
was
ion were
--Materials. *H20
examined
FAB
not
the
to
were
salt;
several
of
active
would
up from
mass
to
biochemistry thousand
dal-
hydroqen
con-
constitute use
1500
the to
of
a major FAB
mass - *H20
daltons,
and
standpoint
of
a variety
quanosine
spectrum
of
sulfate;
29
applic-
compounds
of
University Utah.
Utah;
A Imixture Blenoxane
glycerol
*H20
of
the
reexchange Mass
at dry
to
rinsed mass
with An
modifications
tip
probe
MSD
of
labeling
and
C-perdeuterioqlycerol,
Isotopes,
St.
uridine
melibiose;
Louis,
MO.
5'-phosphate,
melezitose;
was
The Na
streptomycin
provided
a qift
from
by
W. R.
A*-demethyl,
Dr. and
Dr.
M.
P.
Gray,
B2 were
described
FAB
in
solution
per
Schweizer,
University
purchased
in
2 ul.
*H20.
a 10 ~1
was
adsorbed
pg
rinsed
using
probe
of locally
Prior
Two
syringe
immediately
[hydroxy-*H3!--
~1
that
of
were
application solution
had
transferred
precautions
to the
been to
necessary
pre-
the to
vacuum
avoid
H20.
spectra
magnetic
by
1-5
These by
Tech
prepared
was
tip
The
Mass either
Ion
% *H)
sources:
were
spectrometer.
deuterium
inr,trument,
atom
a concentration
*D20.
spectrometry.
potential.
A2,
probe
the
with
of
(Y7.8 from
was
Samples
the
transferred
vic~usly
extent
a fragment
Laboratories).
(1:l)
sample,
of
labeling
N-[(9-6-D-ribofuranosylpurin-5-yl)-
MI
bleomycins
preparation. -
the
of (Bristol
Sample
METHODS
Na salt
conotoxin
formation
The
AND
y-cyclodextrin. 5'-phosphate,
of
for
on.
Na salt;
B-cyclodextrin;
glycerol of
(11).
commercial
5'-phosphate,
deuterated
mechanism
purchased
from
of
the
commented
purchased
carbamoyllthreonine
tht!
to
the
accuracy,
use
study
[Hydroxy-*H3]glycero1 ~ atom % *H) were
(9S+
followinq
lotk
in
is
[hydroxy-*H3]glycerol
region
high
employed TpT,
negative
matters
were
problems up
in
weight
with
spectrometry
and
exchanged
molecular
mass
a consequence,
MATERI4LS
of
region
attractive, As
technique
deoxynucleotide
related
as
structural
COMMUNICATIONS
importance. Sindona
and
bombardment
mass
is
directly
the
RESEARCH
determination
methods.
materials in
the
accurate
a microgram-scale,
0'1
ion
solution
of
existing
hytjrogens.
biological
of
atom
in
prospect
{explored
ability
the
BIOPHYSICAL
fast
chemistry
The
(B-10).
AND
of
on
products
ton5
has
BIOCHEMICAL
were or
electric
11N
ion
source
by
Biemann
and 127
using
dcquired
scanning was
a Varian at
installed,
co-workers
8 kV
731
accelerating
closely (12).
MAT
folloriny
A neutral
Xe beam
Vol.
112,
having data
No.
1, 1983
6 KeV
energy
were
Nicolet
taken
was
from
1170
Ion
BIOCHEMICAL
the
to
data
intense the
(Mt'H-1)'
replaced
by
protium.
teristic
of
FAB
for
1.
In
those In
from
Table
RESEARCH
desorption.
In
accumulated
RESULTS
AND
the
FAB
mass
are
given
in
within
each
exchanged
molecule
notation
Table
from
peak
fully
protonated
ion
spectra
exchange
[most
refers
for
BIOPHYSICAL
over
some
COMMUNICATIONS
cases
ion
(1024
scans)
2 min.
abundance using
a
averager.
abundance
the
mass
siqnal
hydroqen-deuterium to
used
AND
ion
Additional
every
(17,18),
case
the
of
Table
isotopic
compounds
Abundances
cluster.
in
a deuteron,
one
such
as
Nat
adducts,
were
also
observed,
but
extent
of
exchanqe
in
b,y
analoqy
FAB
to
(16).
has
which
these
(M+2H)+
in
deuterium
ions
normalized
notation
produced
which
following
are
The
to
usually
species
ten
1.
attached
(unexchanqed) to
spectra
spectra
molecule,
MHt
refers
DISCUSSION
The
been
are
charac-
are
not
listed
ions
was
the
in same
as
reported. every
the
case
mass
1.
examined
shift
Sull~nlary
the
between
of
the
Molecular
active
spectrum
hydroqen
of
Weight-Related
Molecular Weight., Unlabeled
Compound
correct
the
Ions
Number of Active Hydrogen8
Percent Exchange
content
unlabeled
was
material
Following
established (data
Hydrogen-Deuterium
nl/z
(relative
not
Exchange
intensity)"
(M+'H-3)+
(M+~H-~)+
(M+'H-l)+
(M+?H)+
90
345(O)
350(19)
351(55)
352(100)
512
390(13)
391(26)
392(60)
393(100)
514
93
520(11)
521(1Y)
522(56)
523(100)
Melibiose
342
90
349jiO)
350(41)
351(94)
352(100)
Melezitose!
504
53
514(13)
515(34)
516(80)
517(100)
581
93
59607)
597(59)
59X(100)
599(51)
u-Cyclodextrin
972
Y3
989145)
990(X3)
991(100)
y-Cyclodext&
1296
93
1319(66)
1320(87)
1321(100)
132L(3uj
Bleolilycins~ AL I cation< dwethyl-AZ G:
1414 1399 1424
93 93 93
1436(83) 1423(71) 1452(87)
1437(95) 1424(88) 1453(9Y)
1438(100) 1425(100) 1454(100)
1439(9X) 14X(96) 1455(90)
Conotaxin
1492
92
1518(79)
1519(95)
1520(100)
1521(x')
Uridlne-5'.phosphate, nlonosodlum salt
346
Guanosine-5'-phosphate,
385
id-[(9-6-U-ribofuranosylpurine 6-yl)carbomyl]threonine phosphate, ,monosodium
Streptomycin
sulfate
MIC
6
5'. salt
27
d Each isotopic cluster is normalized to the largest peak in the cluster. p FAB amass spectrum of unlabeled compound, ref. 13. d FA6 mass specttul of unlabeled cwlpound, ref. 14. Ion m/z 1439 IS fully exchanged M+; lower amass peaks dlie to bath exchange. c Tetradecapeptide, witn 2 disulfide bonds. ref. 15.
128
Y92(&5)
Vol
112, No. 1, 1983
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
(Mt2H)+ 517
m/z Fig.
1.
Fast 2
atom
bombardment
H3]glycerol
(G)
mass
and
spectrum
'H20.
The
of
m/z
meleritose
517
ion
in
[bdroxy-
contains
12 deuterium
atoms.
shown),
and
derlce thl?
was
extent
can
visual
required
be
if
the
the
established
as
The
observed for
29
the
hydroqens.
glycerol
judged
No evi-
skeleton
from
spectra
ranged
frolrl
from
illustrated
by
intensity
into deter-
heavy
simply
can
the
unambiguously
the
spectrum
be is
mass
129
518
spectrum
and
is
fewer
than
the
18
2Hlll-
accounted
can of
into
[hydroxy-
mainly
or
the
established of
calculated
known
as
of
introduction
lUO0
isotopes,
composition from
before m/z
m/z
90-Y%
decrease
was
of
contributions
elemental
(below
content
natural
steadily
times
cases
deuterium
relative
to
longer
simpler
as
isotope the
from
ions,
was
stand
inspection,
heavy (19)
to In
contribution
natural
of
[hydroxy-'H3]glycero1
value
allowed
1).
hydrogen
fragment
frown
This
was
(Fig.
also
any
exchange
h,ydrogens),
melezitose
equations
of
a maximum
matrix.
spectrometer.
simple
tice,
or
possible.
exchangeable
the
incorporation
of
sample mass
up to
C-perdeuterioglycerol
maximum
la.)eled
by
for
exchanqe,
tnolecule
us*ng The
th?
following
found
protonated
~mined
th?
that
13C .
for In
by
standard
be
estimated;
unlabled
by prac-
it coin-
Vol.
112,
pound.
No.
1, 1983
The
lower
incomplete
from
deuterium
peaks
are
Recause at
the
time
of
glycerol
ions
exchange
of
sample number
of and
572
the
(*HI,)
(20) from
If,
functional
the
isotopic
be
qained
by
lower
isotope
in
ohtdi
ned.
ble,
particularly
glycerol
(Kf
or
Na+)
micrograms
of
sample
cases
Reduction
conventional
in
1.
Fig.
21%
pattern
of
very
may
appear
pattern,
sample to
accu-
whether
levels
of and
other.
The
comparison
of
ions
(e.g.,
visually
effect m/z
517
the
confusing.
heavy
usinq
used
= 3,4,5...)
large
natural
the
of
each by
For
for
peak
(n
illustrated
an of
for ions from
isotopes,
deuterium
intense
and
by
levels
averager scanninq
was
size
in
of
several
to
their
suspected, to
the
sodium from
acidic
acidification establish
or
this
present
study
minutes
duration
submicrogram over Some
(Fiq.
tormation
used
weights
used
salt
(12,lH)
signal
scan.
as
fact
can
tip.
minimized. to
examined
were
were
molecular
scan
were
structure,
probe
sample
is
1)
experilnents
the
a signal
is
of
regardless
ions
having
(20).
be
the
cases
isotope
content
Thus,
be within
ions
lower
can
to
some
content
clusters sample,
mainly
in
second
deuterium
interest.
pattern
due
For
deuterium
the
carboxylate)
on
most
to
are
possible
and
the
of
be
first
isotopic
unknown
directly
encountered
by
of
(phosphate,
cluster
content,
overall
(Table
a molecule
out
In
in
correcting
mononucleotides
Several ience.
the
in
1)
ions.
replacement
carried
the
l),
the
may
cluster
clusters
groups
cation
region
found
glycerol
three
salts.
mass
Fig.
COMMUNICATIONS
material).
of
glycerol exchange
on
Mt
represent
of
typically
can
The
the
RESEARCH
in
unlabeled
changes ions
extent
Table
measured
of
abundances
matrix
515
from
spectrum
small
deuteriums
calculating
taken
to
were
Clarification
&as
the
appear
515,
([hydroxy-2H31glycerol)n.zHt
bleom,ycins,
be
atoms,
the
ions,
6$*)
mass
ionization,
measure
(m/z
BIOPHYSICAL
contributions
the
glycerol
AND
peaks
but
sensitive the
rately
of
isotope
exchange,
(recognized many
BIOCHEMICAL
For
n/z
cases,
will
also
I30
in
although suffice.
is
where
ITIeaSlJrWWflt
some I)
600,
fluctuation
accurate
in
levels
ion
for
convenwas
therefore
possi-
interference
from
beam of multiple
intensity deuterium scans
Vol. 112, No. 1, 1983
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
ACKNOWLEDGMENTS This work was supported by the National Institute of General Medical Sciences (GM 21584). The authors are grateful to Dr. W. R. Gray for advice and assistance in calculation of isotopic abundances, and to Mr. S. A. Martin in the laboratory of Dr. K. Biemann for advice concerning ion source installation. REFERENCES 1. 2.
3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17. 18. 19. 20.
Ma, -r. s.,
and Ladas, A. S. (1976) Organic Functional Group Analysis by Gas Chromatography, pp. 138-145, Academic Press, New York. Budzikiewicz, H., Djerassi, C., and Williams, D. H. (1964) Structure Elucidation of Natural Products by Mass Spectrometry, Vol. 1, pp. 17-40, Holden-Day, San Francisco. Hunt, D. F., McEwen, C. N., and Upham, R. A. (1972) Anal. Chem. 44, 12921294., Blum, W., Schlumpf, E., Liehr, J. G., and Richter, W. J. (1976) Tetrahedron Lett. 565-568. and Smith, L. L. (1979) Biomed. Mass Spectrom. 6, 15-18. Lin, Y. Y., and Sethi, S. K. (1980) J. Am. Chem. Sot. 102, 6953-6963. Hunt, D. F., Martinson, 0. P., and Buttrill, Jr., S. E. (1976) Org. Mass Spectrom. 11, 762-772. Rinehart, Jr., K. L. (1982) Science 218, 254-260. Dell, A., and Morris, H. R. 11982)Biochem. Biophys. Res. Commun. 106, 1456-1462. Barber, M., Bordoli, R. S., Sedgwick, R. D., Tyler, A. N., and Green, B. N. (1982) J. C. S. Res. Commun. 936-938. Sindona, G., Uccella, N., and Weclawek, K. (1982) J. Chem. Res. 184-185. Martin, S. A., Costello, C. E., and Biemann, K. (1982) Anal. Chem. 54, 2362-2368. Kambara, H., Ogawa, Y., Mochizuki, K., and Hishida, S. (1982) Mass Spectrosc. (Tokyo) 30, 169-181. Barber, M., Bordoli, R. S., Sedgwick, R. D., and Tyler, A. N. (1981) Biochem. Biophys. Res. Commun. 101, 632-638. McIntosh, M., Cruz, 1. J., Hunkapiller, M. W., Gray, W. R., and Olivera, B. M. (1982) Arch. Biochem. Biophys. 218, 329-334. Barber, M., Bordoli, R. S., Sedgwick, R. D., and Tyler, A. N. (1981) 293, 270-275. --Nature Bordoli, R. S., Garner, G. V., Gordon, D. B., Sedgwick, R. Barber, M., D ., Tetler, L. W., and Tyler, A. N. (1981) Biochem. J. 197, 401-404. Barb'er, M., Bordoli, R. S., Elliott, G. J., Sedgwick, R. D., and Tyler, A. N. (1982) Anal. Chem. 54, 645A-657A. Beynon, J. H. (1960) Mass Spectrometry and its Applications to Organic Chemistry, pp. 294-302, Elsevier, Amsterdam. and McCloskey, J. A. (1977) Anal. Chem. 49, 281-283. Yamamoto, H.,
131
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
15, 1983
Pages
DETERMINATION
OF ACTIVE
MASS
SPECTROMETRY
Satinder
K.
February
CONTENT
FOLLOWING
Sethi,
Departments University
Received
HYDROGEN
David
of
Medicinal Utah,
of
BY FAST
ATOM
HYDROGEN-DEUTERIUM
L.
Smith
and
Salt
Chemistry Lake
BOMBARDMENT
EXCHANGE
James and
126-131
A.
McCloskey
Biochemistry Utah 84112
City,
25, 1983
Fast atom bombardyent mass spectroyetry following hydrogen - deuterium H20 has been studied as a means of exchanqe in [hydroxyH31glyCWOl and establ;shing active hydrogen content in molecules of unknown structure. one peptide and complex antibiotics, in the mass Nucleotides, carbohydrates, region to 1500 daltons and 29 exchangeable hydrogens were examined, with a correct hydrogen count unambiguously measured in every case. The Imethod is experimentally simple and applicable on a microgram scale, to salts and a variety of polar compounds of biological origin. Knowledge structure This
knowledge
of
an
the
a useful
tization,
or
nuclear
magnetic
methods
become
content
increases.
from
beyond
conditions exchange
Abbreviations
0006-291X/83
is of
4-6 in
atoms
are
principle
FAB, have
useful
hydrogens fast been
atom
groups,
H2
chemical (l),
deriva-
proton -
Unfortunately, the
often
limited
by
active
hydrogen because
back-exchange,
serious
deutethese
favorable
exchange
and
functional
hydrogen
as
but
of by
of
to
under
chemical
errors
bombardment; by
$1.50
126
M, 'H.
molecule
in
of
which
can
ioniresult
(6,7).
exchanged
Copyright 13 1983 bv Academic Press, Inc. All rights of reproduction in any form reserved.
inferred
are
(3-5)
strucand
functional
(2).
Gas-phase
unknown
overall
arrangement
ambiguous
usually
of
following
methods
hydrogens.
non-labile
used: hydrogen
but
be
system
results
spectrometric
sensitivity,
or and
often
of
composition,
liberation
inlet
the
deduction
spectrometry
or
and
Mass
severe
active
source
a molecule
elemental
chemical
mass
the
identity can
by or
inaccurate
microgram-level
zation
directly
of
subunits
the content
resonance,
to
structural
determining
ion
in
complementary
hydrogen
the
content
constraint
of
in
measured
in
hydrogen
important
identities
active
exchange
active
is
role
The
becomes
exact
information
groups.
rium
the
provides
ture.
plays
of
which
all
Vol.
112,
No.
The having
1, 1983
Irecent
development
a major
and
natural
impact
tent
for
molecules
imp-ovemellt
over
spectrome.try
for
been
active
in
of
this
region
The
the in
et
al.
the
have
was
ion were
--Materials. *H20
examined
FAB
not
the
to
were
salt;
several
of
active
would
up from
mass
to
biochemistry thousand
dal-
hydroqen
con-
constitute use
1500
the to
of
a major FAB
mass - *H20
daltons,
and
standpoint
of
a variety
quanosine
spectrum
of
sulfate;
29
applic-
compounds
of
University Utah.
Utah;
A Imixture Blenoxane
glycerol
*H20
of
the
reexchange Mass
at dry
to
rinsed mass
with An
modifications
tip
probe
MSD
of
labeling
and
C-perdeuterioqlycerol,
Isotopes,
St.
uridine
melibiose;
Louis,
MO.
5'-phosphate,
melezitose;
was
The Na
streptomycin
provided
a qift
from
by
W. R.
A*-demethyl,
Dr. and
Dr.
M.
P.
Gray,
B2 were
described
FAB
in
solution
per
Schweizer,
University
purchased
in
2 ul.
*H20.
a 10 ~1
was
adsorbed
pg
rinsed
using
probe
of locally
Prior
Two
syringe
immediately
[hydroxy-*H3!--
~1
that
of
were
application solution
had
transferred
precautions
to the
been to
necessary
pre-
the to
vacuum
avoid
H20.
spectra
magnetic
by
1-5
These by
Tech
prepared
was
tip
The
Mass either
Ion
% *H)
sources:
were
spectrometer.
deuterium
inr,trument,
atom
a concentration
*D20.
spectrometry.
potential.
A2,
probe
the
with
of
(Y7.8 from
was
Samples
the
transferred
vic~usly
extent
a fragment
Laboratories).
(1:l)
sample,
of
labeling
N-[(9-6-D-ribofuranosylpurin-5-yl)-
MI
bleomycins
preparation. -
the
of (Bristol
Sample
METHODS
Na salt
conotoxin
formation
The
AND
y-cyclodextrin. 5'-phosphate,
of
for
on.
Na salt;
B-cyclodextrin;
glycerol of
(11).
commercial
5'-phosphate,
deuterated
mechanism
purchased
from
of
the
commented
purchased
carbamoyllthreonine
tht!
to
the
accuracy,
use
study
[Hydroxy-*H3]glycero1 ~ atom % *H) were
(9S+
followinq
lotk
in
is
[hydroxy-*H3]glycerol
region
high
employed TpT,
negative
matters
were
problems up
in
weight
with
spectrometry
and
exchanged
molecular
mass
a consequence,
MATERI4LS
of
region
attractive, As
technique
deoxynucleotide
related
as
structural
COMMUNICATIONS
importance. Sindona
and
bombardment
mass
is
directly
the
RESEARCH
determination
methods.
materials in
the
accurate
a microgram-scale,
0'1
ion
solution
of
existing
hytjrogens.
biological
of
atom
in
prospect
{explored
ability
the
BIOPHYSICAL
fast
chemistry
The
(B-10).
AND
of
on
products
ton5
has
BIOCHEMICAL
were or
electric
11N
ion
source
by
Biemann
and 127
using
dcquired
scanning was
a Varian at
installed,
co-workers
8 kV
731
accelerating
closely (12).
MAT
folloriny
A neutral
Xe beam
Vol.
112,
having data
No.
1, 1983
6 KeV
energy
were
Nicolet
taken
was
from
1170
Ion
BIOCHEMICAL
the
to
data
intense the
(Mt'H-1)'
replaced
by
protium.
teristic
of
FAB
for
1.
In
those In
from
Table
RESEARCH
desorption.
In
accumulated
RESULTS
AND
the
FAB
mass
are
given
in
within
each
exchanged
molecule
notation
Table
from
peak
fully
protonated
ion
spectra
exchange
[most
refers
for
BIOPHYSICAL
over
some
COMMUNICATIONS
cases
ion
(1024
scans)
2 min.
abundance using
a
averager.
abundance
the
mass
siqnal
hydroqen-deuterium to
used
AND
ion
Additional
every
(17,18),
case
the
of
Table
isotopic
compounds
Abundances
cluster.
in
a deuteron,
one
such
as
Nat
adducts,
were
also
observed,
but
extent
of
exchanqe
in
b,y
analoqy
FAB
to
(16).
has
which
these
(M+2H)+
in
deuterium
ions
normalized
notation
produced
which
following
are
The
to
usually
species
ten
1.
attached
(unexchanqed) to
spectra
spectra
molecule,
MHt
refers
DISCUSSION
The
been
are
charac-
are
not
listed
ions
was
the
in same
as
reported. every
the
case
mass
1.
examined
shift
Sull~nlary
the
between
of
the
Molecular
active
spectrum
hydroqen
of
Weight-Related
Molecular Weight., Unlabeled
Compound
correct
the
Ions
Number of Active Hydrogen8
Percent Exchange
content
unlabeled
was
material
Following
established (data
Hydrogen-Deuterium
nl/z
(relative
not
Exchange
intensity)"
(M+'H-3)+
(M+~H-~)+
(M+'H-l)+
(M+?H)+
90
345(O)
350(19)
351(55)
352(100)
512
390(13)
391(26)
392(60)
393(100)
514
93
520(11)
521(1Y)
522(56)
523(100)
Melibiose
342
90
349jiO)
350(41)
351(94)
352(100)
Melezitose!
504
53
514(13)
515(34)
516(80)
517(100)
581
93
59607)
597(59)
59X(100)
599(51)
u-Cyclodextrin
972
Y3
989145)
990(X3)
991(100)
y-Cyclodext&
1296
93
1319(66)
1320(87)
1321(100)
132L(3uj
Bleolilycins~ AL I cation< dwethyl-AZ G:
1414 1399 1424
93 93 93
1436(83) 1423(71) 1452(87)
1437(95) 1424(88) 1453(9Y)
1438(100) 1425(100) 1454(100)
1439(9X) 14X(96) 1455(90)
Conotaxin
1492
92
1518(79)
1519(95)
1520(100)
1521(x')
Uridlne-5'.phosphate, nlonosodlum salt
346
Guanosine-5'-phosphate,
385
id-[(9-6-U-ribofuranosylpurine 6-yl)carbomyl]threonine phosphate, ,monosodium
Streptomycin
sulfate
MIC
6
5'. salt
27
d Each isotopic cluster is normalized to the largest peak in the cluster. p FAB amass spectrum of unlabeled compound, ref. 13. d FA6 mass specttul of unlabeled cwlpound, ref. 14. Ion m/z 1439 IS fully exchanged M+; lower amass peaks dlie to bath exchange. c Tetradecapeptide, witn 2 disulfide bonds. ref. 15.
128
Y92(&5)
Vol
112, No. 1, 1983
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
(Mt2H)+ 517
m/z Fig.
1.
Fast 2
atom
bombardment
H3]glycerol
(G)
mass
and
spectrum
'H20.
The
of
m/z
meleritose
517
ion
in
[bdroxy-
contains
12 deuterium
atoms.
shown),
and
derlce thl?
was
extent
can
visual
required
be
if
the
the
established
as
The
observed for
29
the
hydroqens.
glycerol
judged
No evi-
skeleton
from
spectra
ranged
frolrl
from
illustrated
by
intensity
into deter-
heavy
simply
can
the
unambiguously
the
spectrum
be is
mass
129
518
spectrum
and
is
fewer
than
the
18
2Hlll-
accounted
can of
into
[hydroxy-
mainly
or
the
established of
calculated
known
as
of
introduction
lUO0
isotopes,
composition from
before m/z
m/z
90-Y%
decrease
was
of
contributions
elemental
(below
content
natural
steadily
times
cases
deuterium
relative
to
longer
simpler
as
isotope the
from
ions,
was
stand
inspection,
heavy (19)
to In
contribution
natural
of
[hydroxy-'H3]glycero1
value
allowed
1).
hydrogen
fragment
frown
This
was
(Fig.
also
any
exchange
h,ydrogens),
melezitose
equations
of
a maximum
matrix.
spectrometer.
simple
tice,
or
possible.
exchangeable
the
incorporation
of
sample mass
up to
C-perdeuterioglycerol
maximum
la.)eled
by
for
exchanqe,
tnolecule
us*ng The
th?
following
found
protonated
~mined
th?
that
13C .
for In
by
standard
be
estimated;
unlabled
by prac-
it coin-
Vol.
112,
pound.
No.
1, 1983
The
lower
incomplete
from
deuterium
peaks
are
Recause at
the
time
of
glycerol
ions
exchange
of
sample number
of and
572
the
(*HI,)
(20) from
If,
functional
the
isotopic
be
qained
by
lower
isotope
in
ohtdi
ned.
ble,
particularly
glycerol
(Kf
or
Na+)
micrograms
of
sample
cases
Reduction
conventional
in
1.
Fig.
21%
pattern
of
very
may
appear
pattern,
sample to
accu-
whether
levels
of and
other.
The
comparison
of
ions
(e.g.,
visually
effect m/z
517
the
confusing.
heavy
usinq
used
= 3,4,5...)
large
natural
the
of
each by
For
for
peak
(n
illustrated
an of
for ions from
isotopes,
deuterium
intense
and
by
levels
averager scanninq
was
size
in
of
several
to
their
suspected, to
the
sodium from
acidic
acidification establish
or
this
present
study
minutes
duration
submicrogram over Some
(Fiq.
tormation
used
weights
used
salt
(12,lH)
signal
scan.
as
fact
can
tip.
minimized. to
examined
were
were
molecular
scan
were
structure,
probe
sample
is
1)
experilnents
the
a signal
is
of
regardless
ions
having
(20).
be
the
cases
isotope
content
Thus,
be within
ions
lower
can
to
some
content
clusters sample,
mainly
in
second
deuterium
interest.
pattern
due
For
deuterium
the
carboxylate)
on
most
to
are
possible
and
the
of
be
first
isotopic
unknown
directly
encountered
by
of
(phosphate,
cluster
content,
overall
(Table
a molecule
out
In
in
correcting
mononucleotides
Several ience.
the
in
1)
ions.
replacement
carried
the
l),
the
may
cluster
clusters
groups
cation
region
found
glycerol
three
salts.
mass
Fig.
COMMUNICATIONS
material).
of
glycerol exchange
on
Mt
represent
of
typically
can
The
the
RESEARCH
in
unlabeled
changes ions
extent
Table
measured
of
abundances
matrix
515
from
spectrum
small
deuteriums
calculating
taken
to
were
Clarification
&as
the
appear
515,
([hydroxy-2H31glycerol)n.zHt
bleom,ycins,
be
atoms,
the
ions,
6$*)
mass
ionization,
measure
(m/z
BIOPHYSICAL
contributions
the
glycerol
AND
peaks
but
sensitive the
rately
of
isotope
exchange,
(recognized many
BIOCHEMICAL
For
n/z
cases,
will
also
I30
in
although suffice.
is
where
ITIeaSlJrWWflt
some I)
600,
fluctuation
accurate
in
levels
ion
for
convenwas
therefore
possi-
interference
from
beam of multiple
intensity deuterium scans
Vol. 112, No. 1, 1983
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
ACKNOWLEDGMENTS This work was supported by the National Institute of General Medical Sciences (GM 21584). The authors are grateful to Dr. W. R. Gray for advice and assistance in calculation of isotopic abundances, and to Mr. S. A. Martin in the laboratory of Dr. K. Biemann for advice concerning ion source installation. REFERENCES 1. 2.
3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16. 17. 18. 19. 20.
Ma, -r. s.,
and Ladas, A. S. (1976) Organic Functional Group Analysis by Gas Chromatography, pp. 138-145, Academic Press, New York. Budzikiewicz, H., Djerassi, C., and Williams, D. H. (1964) Structure Elucidation of Natural Products by Mass Spectrometry, Vol. 1, pp. 17-40, Holden-Day, San Francisco. Hunt, D. F., McEwen, C. N., and Upham, R. A. (1972) Anal. Chem. 44, 12921294., Blum, W., Schlumpf, E., Liehr, J. G., and Richter, W. J. (1976) Tetrahedron Lett. 565-568. and Smith, L. L. (1979) Biomed. Mass Spectrom. 6, 15-18. Lin, Y. Y., and Sethi, S. K. (1980) J. Am. Chem. Sot. 102, 6953-6963. Hunt, D. F., Martinson, 0. P., and Buttrill, Jr., S. E. (1976) Org. Mass Spectrom. 11, 762-772. Rinehart, Jr., K. L. (1982) Science 218, 254-260. Dell, A., and Morris, H. R. 11982)Biochem. Biophys. Res. Commun. 106, 1456-1462. Barber, M., Bordoli, R. S., Sedgwick, R. D., Tyler, A. N., and Green, B. N. (1982) J. C. S. Res. Commun. 936-938. Sindona, G., Uccella, N., and Weclawek, K. (1982) J. Chem. Res. 184-185. Martin, S. A., Costello, C. E., and Biemann, K. (1982) Anal. Chem. 54, 2362-2368. Kambara, H., Ogawa, Y., Mochizuki, K., and Hishida, S. (1982) Mass Spectrosc. (Tokyo) 30, 169-181. Barber, M., Bordoli, R. S., Sedgwick, R. D., and Tyler, A. N. (1981) Biochem. Biophys. Res. Commun. 101, 632-638. McIntosh, M., Cruz, 1. J., Hunkapiller, M. W., Gray, W. R., and Olivera, B. M. (1982) Arch. Biochem. Biophys. 218, 329-334. Barber, M., Bordoli, R. S., Sedgwick, R. D., and Tyler, A. N. (1981) 293, 270-275. --Nature Bordoli, R. S., Garner, G. V., Gordon, D. B., Sedgwick, R. Barber, M., D ., Tetler, L. W., and Tyler, A. N. (1981) Biochem. J. 197, 401-404. Barb'er, M., Bordoli, R. S., Elliott, G. J., Sedgwick, R. D., and Tyler, A. N. (1982) Anal. Chem. 54, 645A-657A. Beynon, J. H. (1960) Mass Spectrometry and its Applications to Organic Chemistry, pp. 294-302, Elsevier, Amsterdam. and McCloskey, J. A. (1977) Anal. Chem. 49, 281-283. Yamamoto, H.,
131