(Received for publication, October 1, 1996, and in revised form, December 9, 1996)
From the The Clayton Foundation Laboratories for
Peptide Biology, The Salk Institute, La Jolla, California 92037, the
§ Departments of Biology and
Psychiatry University of
Utah, Salt Lake City, Utah 84112, and the ¶ Marine Science
Institute, University of the Philippines, Diliman, Quezon
City, 1101, Philippines
We report a novel post-translational modification involving halogenation of tryptophan in peptides recovered from the venom of carnivorous marine cone snails (Conus). The residue, L-6-bromotryptophan, was identified in the sequence of a heptapeptide, isolated from Conus imperialis, a worm-hunting cone. This peptide does not elicit gross behavioral symptoms when injected centrally or peripherally in mice. L-6-Bromotryptophan was also identified in a 33-amino acid peptide from Conus radiatus; this peptide has been shown to induce a sleep-like state in mice of all ages and is referred to as bromosleeper peptide. The sequences of the two peptides
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Polypeptides encoded by genes are primarily made up of the 20 common amino acids that are directly translated using the genetic code. However, many of these amino acids can be further modified post-translationally to yield a set of additional amino acids that contribute to the function of the mature protein. Together the 20 primary amino acids and these "secondary" amino acids which are found in proteins comprise the set of proteinogenous amino acids.
These modified amino acids include amino acid conjugates where the side
chain is linked to a glycosyl, phosphate, or sulfate group and amino
acids such as 5-hydroxylysine, 4-hydroxyproline, and
-carboxyglutamate. One notable set of modified amino acids are
halogenated derivatives of tyrosine and histidine. Naturally occurring
halogenated tyrosine and histidine residues have previously been
identified from proteins (1-4). A particularly well documented example
of in vivo post-translational halogenation of an amino acid
residue in a protein is afforded by thyroglobulin (5). After iodination
of several tyrosine residues, selective cleavages release the iodinated
thyroid hormones thyroxine (3,5,3
,5
-tetraiodothyronine or
T4)1; 3,5,3
-triiodothyronine
(T3), and 3,3
-di-iodothyronine. The presence of free
T3 and T4 has also been shown in
protochordates, suggesting a primitive thyroid function exists in
tunicates (2).
Of the 20 common amino acids, alanine, glycine, isoleucine, leucine,
and valine, which lack side chain functional groups, have not been
implicated in post-translational modifications (6). In 1907 it was
proposed that hydroxytryptophan was a proteinogenous amino acid (7),
but this proposal has not been verified (1), and chemical oxidation of
tryptophan is likely to be responsible for the observed modification.
More recently, Takai and Hayaishi (8) have described tryptophan side
chain oxidases in Pseudomonas, while McIntire et al.
(9) have described a redox co-factor which is covalently linked to
2 tryptophan residues in Methylobacterium extorquens and
Thiobacillus versutus. In this report, we establish, using
accepted criteria (10-12), that 6-bromotryptophan is a secondary amino
acid and establish its presence in two peptides purified from the
venoms of two Conus species, the imperial cone, Conus imperialis, and the radial cone, Conus radiatus (Fig.
1).
Most conotoxins are small, highly constrained and specialized
polypeptides present in the venom produced by marine cone snails (Conus) (13). A distinctive characteristic of the conotoxins is the high percentage of cysteine residues mediating disulfide bridges
in many of the peptides. The disulfide bridges are responsible for the
highly constrained conformations of these toxins enabling the molecules
to block a variety of different receptors with high binding affinity
and selectivity. These peptides also have high levels of other modified
amino acids including hydroxy proline and -carboxyglutamic acid
(14). To this list we now add 6-bromotryptophan.
Reagents
The following reagents were used: DIC (Chem-Impex International,
Wood Dale, IL); DCM (Fisher); Boc-Ala-OH, Boc-Cys(Mob)-OH, Boc-Gln(Xnt)-OH, Boc-Gly-OH, pGlu-OH, Boc-Thr(OBzl)-OH, and Boc-Ala-OH (Bachem, Torrance, CA); DL-6-bromotryptophan
(Biosynth A.G., Staad, Switzerland);
DL-5-bromotryptophan (synthesized as described
elsewhere (15)); acetyl chloride (99+%), anisole, ascorbic acid, hexyl alcohol (98%), HOBt, iodine, and piperidine (Aldrich); DIEA (Fisher); TBTU and N-methylpyrrolidone (Advanced Chemtech, Louisville,
KY); HF (Matheson Gas Products, Cucamonga, CA); trifluoroacetic acid (Halocarbon Products Corp., River Edge, NJ); ether, acetonitrile, and
acetic acid (Mallincrodt Baker Inc., Paris, KY); methanol (Burdick and
Jackson Division, Muskegon, MI); TCEP (synthesized by the method of
Burns et al. (16)); iodoacetamide, EDTA, guanidine hydrochloride, Hepes, sodium carbonate, 4-vinyl pyridine, Tris-HCl, and
Tris base (Sigma); -mercaptoethanol (Pierce);
-chymotrypsin, aminopeptidase-M, carboxypeptidase-Y,
endoproteinase Lys-C, endoproteinase Asp-N, and pyroglutamate
aminopeptidase (Boehringer Mannheim).
Crude Venom
The crude venom was obtained from C. imperialis and
C. radiatus by dissection of the venom duct gland and was
stored at 70 °C.
Peptide Purification
Pooled venom was diluted with 0.1% aqueous trifluoroacetic acid and injected onto a reverse phase high performance liquid chromatography (HPLC) using a Vydak C18 column (10 × 250 mm, 5 µm particle size, Rainin Instruments, Woburn, MA) and eluted with a linear gradient of acetonitrile in 0.085% trifluoroacetic acid at 5 mL/min. The HPLC apparatus consisted of HPXL pumps and either a Dynamax model UVI or UV-DII detector (Rainin Instruments). Subsequent purification steps utilized a C18 Microsorb or C18 Vydac column, 4.6 × 250 mm, 5 µm particle size (Rainin Instruments). The effluents were monitored at 220 nm. Peaks were collected, and aliquots were assayed for activity.
Bioassays
Biological activity of both the heptapeptide and the bromosleeper peptide was assayed by intracranial and intraperitoneal injection in mice (9-22 days old) as described previously (17). Aliquots of peptide samples were lyophilized and suspended in normal saline solution, then injected into mice using a 0.3-ml syringe with a 29-gauge needle. Twenty-microliter volumes were injected intracranially, and 50-µl volumes were injected intraperitoneally. Each control mouse was injected with an equal volume of normal saline solution containing dissolved residue of lyophilized column buffer. After injections, the mice were placed in cages for observation.
Enzyme Hydrolysis
PAP HydrolysisThe bromoheptapeptide was incubated in a 0.1 M Na2CO3 solution with pyroglutamate aminopeptidase (1:1, enzyme:substrate) at 37 °C for 17 h.
Endoproteinase Lys-C HydrolysisFragments of the pyridylethylated sleeper peptide were generated by digestion with endoproteinase Lys-C. The peptide was incubated with the enzyme in a total volume of 50 µl (25 mM sodium bicarbonate buffer, pH 8.5, 10% acetonitrile) at 37 °C for 16 h. The reaction was stopped by addition of 25 µl of acetonitrile and 5 µl of 10% trifluoroacetic acid and the digest purified with HPLC.
Endoproteinase Asp-N HydrolysisFragments of the pyridylethylated sleeper peptide were generated by digestion with endoproteinase Asp-N. The peptide was incubated with the enzyme in a total volume of 50 µl (25 mM potassium phosphate buffer, pH 8, 10% acetonitrile) at 37 °C for 19 h. The reaction was stopped by addition of 25 µl of acetonitrile and 5 µl of 10% trifluoroacetic acid and the digest purified with HPLC.
Aminopeptidase-M HydrolysisThe synthetic 1-4 bromosleeper N-terminal fragment (100 pmol) was incubated in 100 µl of 100 mM Hepes solution with 20 milliunits of aminopeptidase-M at 24 °C and the reaction monitored with HPLC at 24-h and 4-day time points.
Chemical Modifications
EsterificationEsterification of the N-terminal (1-4) fragment of the bromosleeper peptide with acidic hexanol, prepared from acetyl chloride and hexyl alcohol, was carried out as outlined elsewhere (18).
Reduction and AlkylationThe bromoheptapeptide was reduced
with 10 mM TCEP in 200 mM sodium acetate
buffer, pH 5, and alkylated with iodoacetamide in 30 mM
Tris base, pH 10, containing 2 mM EDTA at room temperature as described elsewhere (19). The bromosleeper peptide was reduced and
alkylated by either of two methods. In method 1, the peptide was
dissolved in 250 mM Tris-HCl, 6 M guanidine
hydrochloride, and 2 mM EDTA, pH 7.5, reduced with a 10%
solution of -mercaptoethanol in deionized H2O at room
temperature and alkylated in the dark with a 20% solution of 4-vinyl
pyridine in ethanol. With method 2 the peptide was reduced with TCEP
and alkylated with 4-vinyl pyridine as described previously (20).
Chemical Sequence and Amino Acid Analyses
Automated chemical sequence analysis was performed on a 477A Protein Sequencer (Applied Biosystems, Foster City, CA). Amino acid analysis was carried out using pre-column derivatization. Approximately 500 pmol of the bromoheptapeptide was sealed under vacuum with conc. HCl, hydrolyzed at 110 °C for 24 h, lyophilized and then derivatized with o-phthalaldehyde. The derivatized amino acids were then analyzed with HPLC.
Mass Spectrometry
Matrix-assisted laser desorption (MALD) (21) mass spectra were
measured using a "Bruker REFLEX" (Bruker Instruments Inc., Bremen,
Germany) time-of-flight (22) mass spectrometer fitted with a gridless
reflectron and a N2 laser and a 100-MHz digitizer. An
accelerating voltage of +31 kV and a reflector voltage of between 1.16 and 30 kV were employed for the post source decay FAST (23) measurements. The sample (in 0.1% aqueous trifluoroacetic acid) was
applied with -cyano-4-hydroxycinnamic acid. Liquid secondary ionization (LSI) (24) mass spectra were measured using a Jeol HX110
(Jeol, Tokyo, Japan) double focusing mass spectrometer operated at
10-kV accelerating voltage. The sample (in 0.1% aqueous
trifluoroacetic acid and 25% acetonitrile) was mixed in a glycerol,
3-nitrobenzyl alcohol matrix (1:1) and analyzed with either magnetic or
electric field scans. The spectra were calibrated using
[Cs(CsI)n]+ cluster ions. The LSIMS spectra were measured
at nominal resolutions of either 1000 or 3000. Electrospray mass
spectra were measured using an LCQ (Finnigan MAT, San Jose, CA) ion
trap mass spectrometer. The samples (in 0.1% aqueous trifluoroacetic
acid) were analyzed by direct infusion with (bromoheptapeptide) or
without (N-terminal 1-4 fragment of the bromosleeper peptide) the
addition of 20% acetic acid (6:1) solution. The mass accuracy was
typically better than: 1000 ppm for the time-of-flight instrument in
the linear mode, 200 ppm for the time-of-flight instrument in the
reflectron mode and the ion trap instrument, and 50 ppm for the double
focusing mass spectrometer. We note that when analyzing Gla-containing peptides with time-of-flight mass spectrometers, decarboxylation can
significantly reduce the mass accuracy below these levels (25).
Synthesis of the Bromoheptapeptide
The synthesis was carried out manually on a 4-methylbenzhydrylamine resin using DIC as coupling reagent with the Boc protection strategy in DCM with the exception of the introduction of the Fmoc (9-fluorenylmethoxycarbonyl)-DL-6-bromotryptophan or Fmoc-DL-5-bromotryptophan. The 4-methylbenzhydrylamine resin was prepared at The Salk Institute, with a substitution of 0.5 mmol/g. The DL-6-bromotryptophan and DL-5-bromotryptophan were derivatized to Fmoc-DL-6-bromotryptophan and Fmoc-DL-5-bromotryptophan, respectively. In the case of the Fmoc-DL-6-bromotryptophan-mediated coupling, HOBt/DIEA was used with TBTU in N-methylpyrrolidone (NMP) followed by the deprotection of the Fmoc group with 20% piperidine in NMP. Four-fold excess of amino acid derivatives were used in the coupling reactions with the exception of the DL-6-bromotryptophan where a 10% excess was used. The efficiency of the coupling reactions was checked using the Kaiser-ninhydrin test. The dried peptide-resin (1.28 g) was treated with 15 ml of HF in the presence of 1.5 ml of anisole at 0 °C for 1.5 h. After the evaporation of HF, a first extraction was carried out with ether (3 × 100 ml) and a second extraction with 0.1% aqueous trifluoroacetic acid and 60% acetonitrile (3 × 50 ml). Purification of the crude reduced product on analytical HPLC indicated two major components whose measured mass (MALD-MS) were consistent with the calculated peptide mass. The extract of the crude peptide (approximately 150 ml) was diluted with 500 ml of acetic acid, mixed vigorously, and titrated with iodine in methanol (1%) until the color of the solution remained amber for 10 min. The excess of iodine was eliminated with a 5% ascorbic acid solution. The volume was reduced by evaporation to 70 ml and the residue diluted with 430 ml of triethylamine phosphate, pH 2.25, buffer. Acetonitrile was added (approximately 20 ml) until the opalescent liquid turned clear.
The crude bromoheptapeptide solution was clarified by the addition of acetonitrile (50 ml) and loaded on a 45 × 320-mm column packed with Vydac C18 15-20-µm particles and eluted with a Waters PrepLC/System 500A equipped with gradient controller, Waters model 450 variable wavelength detector and Waters 1000 PrepPack cartridge chamber in 0.1% aqueous trifluoroacetic acid, using a gradient of 60% acetonitrile in 0.1% aqueous trifluoroacetic acid. Fractions (50 ml) were collected manually. Two components were isolated, one of them at approximately 16% acetonitrile, the other at approximately 22% acetonitrile. The collected fractions of the first component (1300 ml) were diluted with the same volume of 0.1% aqueous trifluoroacetic acid and reloaded onto the equilibrated preparative HPLC column. One major component was collected at approximately 22% acetonitrile and lyophilized (34.8 mg, purity based on HPLC 99%, based on CZE 97%). The collected fractions of the second component (700 ml) were purified as above. The major component was collected at approximately 26% acetonitrile and lyophilized (28.9 mg, purity based on HPLC 99%, based on CZE 97%). LSI-MS measurement of both components resulted in an intense species at m/z 852.2 consistent with the calculated monoisotopic [M + H]+ mass of 852.17 Da.
Synthesis of Bromosleeper N-terminal (1-4) Fragment
The synthesis was initiated on Boc-Ile-CM-resin (300 mg), prepared at The Salk Institute (1% cross-link, 200-400 mesh, substitution 0.71 mmol/g). The coupling reactions were carried out manually using the Boc/trifluoroacetic acid protocol with DIC in the case of coupling Boc-Thr(OBzl)-OH and Boc-Ala-OH (3 equivalents) in DCM. The N-terminal residue DL-6-bromotryptophan was introduced as the N-Fmoc-DL-6-bromotryptophan derivative (2 equivalents). The coupling was mediated with DIEA/HOBt, and TBTU was used as a condensing agent in NMP. Each coupling reaction was completed within 2 h and checked using the Kaiser-ninhydrin test. The N-terminal Fmoc group was removed with 20% piperidine/NMP in 2 × 10 min. The weight of the washed and dried resin was 390 mg (weight gain 90 mg). The dried deprotected peptide-resin (390 mg) was treated with 4 ml of HF in the presence of 0.4 ml of anisole at 0 °C for 1.5 h. After the evaporation of HF, a first extraction was carried out with ether 3 × 25 ml) and a second extraction with 0.1% trifluoroacetic acid and 60% acetonitrile (3 × 15 ml) in water. The fingerprint of the crude product on analytical HPLC indicated two major components (diastereomer of the L- or D-6-bromotryptophan tetrapeptide) with observed masses (MALDI-MS) which were consistent with the calculated peptide mass.
The purification of bromosleeper N-terminal (1-4) fragment involved evaporation of 25% of the aqueous extract (rotavap 38 °C water bath). The solid residue was redissolved in 3.0 ml of 0.1% aqueous trifluoroacetic acid, 20% acetonitrile buffer and loaded in 0.5 ml portions to a semipreparative column. The fractions were collected manually and checked by analytical HPLC. The first pooled and lyophilized fractions resulted in an 8.8-mg peptide that was 99.9% pure by CZE, and the second fraction resulted in a 7.8-mg pure optical isomer tetrapeptide with 98% purity by CZE. LSI-MS measurement of both fractions resulted in an intense species at m/z 568.2, which compared closely with calculated [M + H]+ monoisotopic mass of 568.18 Da.
Peptide Characterization
Co-elution of Natural and Synthetic BromoheptapeptideReverse phase HPLC co-elution experiments of natural and synthetic bromoheptapeptide were carried out with a Vydac C18 (5 µm, 300 Å particle size) 2.1 × 150-mm column at a flow rate of 200 µl/min. Volatile buffers (0.055% aqueous trifluoroacetic acid and acetonitrile) were used and the effluent was monitored at 210, 254, and 280 nm with a HP1090 (Hewlett-Packard, Wilmington, DE).
Determination of L- Versus D-6-Bromotryptophan-containing BromoheptapeptideThe
two purified peptides (corresponding with either the D- or
L-isomers of 6-bromotryptophan) were reduced and alkylated. The HPLC-purified reduced and alkylated peptides were lyophilized and
redissolved in 250 mM Tris base, pH 8.5, and incubated with -chymotrypsin (1:40, 1:10, and 1:5; enzyme:substrate) for up to 9 days. The progress of the reaction was monitored with HPLC and
MALD-MS.
Approximately equal amounts of the endoproteinase Asp-N-digested N-terminal fragment of the bromosleeper peptide and the synthetic peptide Trp*-Ala-Thr-Ile-OH were mixed (where Trp* = bromotryptophan). The mixture was applied onto a C18 analytical column and eluted at 1 ml/min using a gradient of acetonitrile in 0.085% trifluoroacetic acid. A similar amount of the synthetic peptide was analyzed on HPLC under the same conditions.
Determination of L- Versus D-6-Bromotryptophan in the Bromosleeper Peptide N-terminal (1-4) FragmentAn aliquot (10 µl) of each synthetic peptide (1 mM) was lyophilized, redissolved in 100 mM Hepes, pH 7.5, and incubated with aminopeptidase-M (1:40; enzyme:substrate) for up to 4 days. The progress of the reaction was monitored with HPLC. The product of the aminopeptidase-M reaction was co-injected with the racemic mixture of 6-bromotryptophan or with the racemic mixture of 5-bromotryptophan.
Two peptides containing
L-6-bromotryptophan were isolated from the venom of
predatory Conus species. The first was a bromoheptapeptide from C. imperialis, purified from a side fraction isolated
during the purification of another unrelated peptide -conotoxin IMI (26) (see Fig. 2). Our interest in this sample was
initially stimulated after scanning fractions present in the crude
venom for novel peptides based on the intact mass (27), rather than biological activity. MALD-MS analysis of the purified fraction indicated species at m/z 853, 855, 875, and 879 (data not
shown). In order to obtain higher mass resolution without sacrificing sensitivity, this sample was analyzed with electrospray ionization and
an ion trap mass spectrometer (see Fig. 3A).
Several relatively intense species were observed with 2-Da separation
at m/z 835.9 and 837.9, m/z 853.1 and 855.1, and
m/z 875.2 and 877.2, which are referred to as doublets.
These doublets could be clearly resolved using a zoom scan (e.g.
m/z 853.1 and 855.1; see Fig. 3A, inset). The
separation of approximately 22 Da between m/z 853.1 and
875.2 (and also between m/z 855.1 and 877.2) suggested
competitive [M + H]+ and [M + Na]+
formation (M = 852). Accordingly, the m/z 835.9 and
837.9 doublets were attributed to loss of NH3 from the
protonated molecule ion. The presence of the doublets was
characteristic of a molecule containing a single 79Br or
81Br atom. This pattern of isotopomers is quite
distinctive, since these isotopes are separated by 2 Da and have
approximately equal natural abundance, and this characteristic doublet
was observed from both the synthetic 5- and 6-bromotryptophan amino
acids (data not shown). Accurate mass analysis using LSI on a magnetic
sector instrument was used to determine masses of m/z 853.19 and 855.20 for the [M + H]+ doublets (data not shown). It
was deduced that the peptide was N-terminally blocked with pyroglutamic
acid from initial chemical sequencing measurements and the shift in
chromatographic retention time following treatment with pyroglutamate
aminopeptidase. Automated Edman degradation analysis after
pyroglutamate aminopeptidase treatment resulted in the sequence:
Cys-Gly-Gln-Ala-X-Cys, where X indicates a blank
cycle. Amino acid analysis confirmed the presence of 1 mole ratio of
glycine and alanine to 2 mole ratios of glutamate and cysteine. A major
component of the hydrolysate eluted 0.7 min after the expected
retention time of derivatized tryptophan, but 2.2 min before the
expected retention time of derivatized arginine. After reduction and
alkylation of the sample with iodoacetamide (to form the Cys(Cam)
derivative which has a residue mass of 160 Da) MALD-MS analysis
revealed two sets of doublets at m/z 991 and 993 and
m/z 1007 and 1009 (see Fig. 3B) separated by 16 Da. We interpreted these species as the [M
+ Na]+ and
[M
+ K]+ of the reduced and alkylated peptide (M
= 968 Da). The shift in mass after reduction and alkylation (M
M = 968-852 = 116 Da) was consistent with the presence of two
cysteine residues. Other species observed in Fig. 3B were
interpreted as fragment ions (e.g. m/z 788 corresponds with
the post source decay b6 fragment ion).2 The post-source decay FAST spectrum
of the reduced and alkylated product, measured at low, medium, and high
laser power fluences, are shown in Fig. 3C. In Fig.
3C, the position of the monoisotopic [M
+ H]+ = 969 is indicated, although only the cationized intact ions were
observed. Three fragment ions, which were observed above the background
noise level in the low power spectrum at m/z 793.1, 528.1, and 456.6, were also observed at varying intensities at medium and high
laser power. Based on the mass differences between the parent and the
successive fragments (176.9, 265.0, and 71.5 Da), we interpreted these
ions as corresponding to N-terminal fragments differing in mass by
Cys(Cam), X, and Ala where X = 265 Da. We
conclude that these three fragment ions (b6,
b5, and b4) encompass the blank observed in the
chemical sequence data. Based on these results we deduced that the 6th
amino acid, was hydrophobic, absorbed intensely at 280 nm, and had a
mass of 265 Da. We proposed the sequence:
Pca-Cys-Gly-Gln-Ala-Trp*-Cys-NH2 (where Pca = pyroglutamic acid and Trp* = bromotryptophan). The calculated [M + H]+ for the monoisotopic mass of the bromoheptapeptide
(853.176 Da) was consistent with the measured m/z of 853.19 (see Fig. 3A).
Assignment of bromotryptophan was confirmed by total chemical synthesis
of the bromoheptapeptide. The synthesis of bromoheptapeptide using a
racemic mixture of the D and L forms of
6-bromotryptophan resulted in two diastereomeric peptides, one
containing the D configuration 6-bromotryptophan at
position 6, while the other containing the L configuration
6-bromotryptophan at position 6. HPLC purification of the crude
synthesis product indicated the presence of a hydrophobic and a
hydrophilic species (see Fig. 4A), both of
which contained the characteristic doublet at m/z 853.2 and
855.2 consistent with the native bromoheptapeptide based on LSI-MS
analysis (data not shown). The separation of the peptides containing a
D versus an L amino acid by reverse
phase HPLC exploits structural differences that attend chiral inversion
at the C atom. The hydrophilic isomer co-eluted with the natural
peptide on HPLC (see Fig. 4B). The susceptibility of the
modified tryptophan residue toward enzymatic hydrolysis after reduction
and alkylation of the cysteine residues was determined by incubation of
the synthetic peptide with
-chymotrypsin. The hydrophilic isomer was
observed to hydrolyze when incubated with a 1:10 enzyme to substrate
ratio within 2 days (see Fig. 4C), whereas the hydrophobic
isomer underwent no hydrolysis at this enzyme to substrate ratio when
incubated for 9 days (data not shown). The intact mass and isotopomer
distribution for the chymotrypsin-hydrolyzed fragment analyzed with
LSI-MS corresponded with the calculated mass for the reduced and
alkylated 1-6 bromoheptapeptide fragment
(Pca-Cys(Cam)-Gly-Gln-Ala-Trp*-OH; calculated monoisotopic mass
for the [M + H]+ is 810.19 Da, observed m/z
810.2 (data not shown)).
Although bromine is typically incorporated at position 6 in marine products, in order to unambiguously resolve the question of the stereochemistry of this modified amino acid, we synthesized the bromoheptapeptide with the racemic mixture of D- and L-5-bromotryptophan. This peptide did not co-elute on HPLC with the natural bromoheptapeptide (data not shown).
Insufficient native bromoheptapeptide was available for testing biological activity. Synthetic bromoheptapeptide was assayed for biological activity by injecting 20 nmol of peptide either intracranially or intraperitoneally into mice. No gross behavioral changes in activity were observed, and this peptide was not further tested for biological activity.
Bromosleeper PeptideConcurrent with the investigation of the
bromoheptapeptide we also characterized a novel "sleeper" peptide,
which induces a sleep-like state in mice; this peptide was purified
from C. radiatus venom (peak BS of Fig.
5A). In the subsequent purification steps
using an analytical HPLC column, the sleeper activity coincided with
the major peaks shown in Fig. 5, B and C.
A family of peptides which elicit a sleep-like state in mice, the conantokins, have been described previously from Conus venoms. The peptide isolated from C. radiatus was very different from the conantokins with respect to activity profile; whereas the conantokins cause sleep when injected intracranially in very young mice (<2 weeks old) and hyperactivity in older mice (>3 weeks old), the new peptide induced sleep in mice of both age groups. A summary of the in vivo effect of the purified peptide is shown in Table I. It is obviously more potent in 9-day-old mice than in the older mice; the effective dose is lower, the onset time is shorter, and the duration of sleep is longer in younger mice.
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MALD-MS analysis of the purified fraction measured in the linear mode
indicated a broad species at m/z 3884 in contrast to the
measurement in the reflectron mode of m/z 3729. LSI-MS
analysis of the same sample indicated a species at m/z
3916.4 (data not shown). These results suggested that the peptide
contained a number of Gla residues (25). Chemical sequencing after
reduction and pyridylethylation of the cysteine residues gave no
regular phenylthiohydantoid derivative of an amino acid at cycle one
but an intense signal for alanine at cycle two followed by normal
repetitive recovery. Weak signals were also observed at positions 6, 8, and 9. Endoproteinase Asp-N hydrolysis of the bromosleeper peptide
generated three major fractions, which when submitted to chemical
sequence analysis revealed the following sequences: (i)
X-Ala-Thr-Ile; (ii)
Asp-X-Cys-X-X-Thr-Cys-Asn-Val-Thr-Phe-Lys-Thr-Cys-Cys-Gly-Hyp-Hyp-Gly, and (iii) Asp-Trp-Gln-Cys-Val-X-Ala-Cys-Pro-Val; where
X indicates a blank cycle. Endoproteinase Lys-C hydrolysis
generated two fragments that after mass spectrometry and chemical
sequence analysis could be used to deduce the connectivity of the three
Asp-N fragments as (i) 1-4, (ii) 5-23, and (iii) 24-33. Based on
mass spectrometric analysis of the Asp-N fragments 5-23 and 24-33,
the weak signals at 6, 8, 9, and 29 were interpreted as Gla residues.
The accurate mass of the 24-33 fragment indicated that the C terminus
of the peptide was in the free acid form (data not shown). We noted a strong UV absorption at 280 nm for both the intact peptide and the
N-terminal fragment characteristic of an indole group. Although it was
reasonable to expect such absorption from the intact peptide that
contains tryptophan, in the case of the 1-4 fragment this adsorption
was attributed to the residue in position 1. Electrospray ionization
ion trap mass spectral analysis of the N-terminal 1-4 fragment
revealed a weak (but constant) signal which when accumulated over
several minutes resulted in a doublet of peaks at m/z 568.1 and 570.1; the zoom scan of which is shown in Fig. 6.
LSI-MS analysis of the N-terminal 1-4 fragment (after esterification
with hexanol to optimize the sensitivity of LSI analysis; resulting in
addition of 84 Da) also resulted in a weak signal where a doublet at
m/z 652.27 and 654.26 could be observed which was not
present when the matrix alone was analyzed (data not shown). We noted
the similarity between the isotopomer intensities of the doublet
observed in Fig. 6 and that observed for the bromoheptapeptide (see
Fig. 3A, inset) and the synthetic bromotryptophan amino
acids. The properties of the modified amino acid were consistent with
the presence of bromotryptophan; e.g. the observed
m/z of 652.27 was consistent with the calculated
monoisotopic mass for the [M + H]+ of the 1-4 fragment
Trp*-A-T-I-C6H12 (652.271 Da). We therefore proposed the sequence
Trp*-Ala-Thr-Ile-Asp-Gla-Cys-Gla-Gla-Thr-Cys-Asn-Val-Thr-Phe-Lys-Thr-Cys-Cys-Gly-Hyp-Hyp-Gly-Asp-Trp-Gln-Cys-Val-Gla-Ala-Cys-Pro-Val-OH (where Hyp = hydroxyproline, Gla = -carboxy glutamate,
and Trp* = bromotryptophan).
After synthesis of the bromosleeper peptide 1-4 N-terminal fragment
with a racemic mixture of the D and L forms of
6-bromotryptophan, a hydrophobic and a hydrophilic peptide isomer were
purified (see Fig. 7A). LSI-MS analysis of
both the hydrophobic and the hydrophilic peptide isomer resulted in
mass spectra consistent with that of the native 1-4 bromosleeper
fragment (data not shown). The hydrophilic isomer was found to co-elute
with the natural peptide on HPLC (see Fig. 7B). The
susceptibility of the bromotryptophan residue toward enzymatic
hydrolysis was determined by incubation of the synthetic peptide with
aminopeptidase-M. The hydrophilic isomer was observed to hydrolyze
within 24 h (see Fig. 7C), whereas the hydrophobic
isomer underwent no hydrolysis under the same conditions or when
incubated for 4 days. The bromotryptophan amino acid released from the
hydrophilic isomer co-eluted on HPLC with the racemic mixture of
6-bromotryptophan but did not co-elute with the racemic mixture of
5-bromotryptophan (data not shown).
We report the purification of two peptides from venoms of two species of cone snails that are divergent from each other, both in their morphology and the feeding biology. The two peptides from these disparate venoms are not homologous to each other, but unexpectedly, we have found that they share one novel biochemical feature, the presence of L-6-bromotryptophan.
The first peptide characterized was a heptapeptide isolated from the venom of the imperial cone, C. imperialis, which hunts polychaete worms. The bromoheptapeptide exhibited no gross peripheral or central symptoms when injected into mice; its biological activity in marine annelid systems has yet to be assessed. The bromoheptapeptide incorporates three post-translational modifications other than bromotryptophan (pyroglutamic acid, disulfide bridge, and amidated C terminus). We know of only a few other peptides that contain pyroglutamic acid, a disulfide bridge, and an amidated C terminus (e.g. tunicate gonadotropin releasing hormone II from Cheylosoma productum (28)), emphasizing the highly modified nature of the bromoheptapeptide.
In contrast to the worm-hunting C. imperialis, the radial cone, C. radiatus, is a deep water Indo-Pacific fish-hunting cone snail. The 33-residue bromosleeper peptide isolated from C. radiatus venom induces a sleep-like state when injected centrally into mice, symptomatology reminiscent of the biological effects of the conantokins, a well characterized Conus peptide family which inhibits the N-methyl-D-aspartic acid receptors (29-33). However, the bromosleeper peptide differs from the conantokins in that it induces a sleep-like state in mice of all ages (conantokins cause sleep in young mice under 2 weeks of age; mice older than 3 weeks exhibit a climbing syndrome). For the bromosleeper peptide, no climbing syndrome is observed at any age.
The number of post-translational modifications in the bromosleeper
peptide is also noteworthy: in addition to having bromotryptophan, the
bromosleeper peptide has three disulfide bridges, 4 residues of
-carboxyglutamate (formed by the vitamin K-dependent
post-translational carboxylation of glutamate residues) and 2 hydroxyproline residues. Furthermore, there clearly is selectivity with
respect to the bromination reaction; only Trp (1) is brominated, while
Trp (25) is unmodified. This selectivity in bromination suggests a
Trp-bromination signaling site to direct the modification enzyme to a
specific tryptophan residue.
To our knowledge, L-6-bromotryptophan has neither been reported among the numerous peptides previously characterized from a variety of species of Conus venoms nor from any other natural peptides/proteins. Thus, the discovery of this amino acid residue in Conus peptides both establishes L-6-bromotryptophan as a proteinogenous amino acid and unequivocally demonstrates that tryptophan can be a precursor for a secondary amino acid in eukaryotic systems.
In order to minimize the erroneous labeling of modified amino acids as
proteinogenous, guidelines with specific criteria have been proposed
(10) for acceptance of new proteinogenous amino acids. Unfortunately,
these guidelines are not always infallible and have not circumvented
the inappropriate acceptance and subsequent withdrawal of residues such
as -hydroxyglutamic acid and norleucine as proteinogenous amino
acids. The submission and subsequent withdrawal of modified amino acids
as proteinogenous highlights the difficulties that may be encountered
in determining the nature of modified amino acids. MS techniques have
been used previously to reduce possible ambiguities in the
determination of a new amino acid (12). In contrast to the
proteinogenous amino acids that were identified after using acid or
base hydrolysis to liberate the amino acid, orthogonal techniques for
sequence determination of peptides (34, 35) have allowed the
unambiguous identification of the bromotryptophan amino acid residue.
In particular, the MS sequence experiment provided sequence
information encompassing the modified amino acid. As a result, we
can exclude the possibility of hydrolysis introducing some chemical
modification.
Previously proposed criteria (11), which have been fulfilled for classification of this modified amino acid as proteinogenous, are as follows.
(i) The complete sequences of two peptides that contain this post-translationally modified amino acid have been characterized. In addition, the sequence of a third novel bromotryptophan-containing peptide, bromocontryphan,3 has been determined.
(ii) The complete synthesis of the bromoheptapeptide and the synthesis of the N-terminal tetrapeptide fragment of the bromosleeper peptide have been carried out using a racemic mixture of 6-bromotryptophan. After synthesis of the peptides, it has been possible to resolve and thereby purify each 6-bromotryptophan-containing peptide (see Figs. 4A and 7A). The purified synthetic hydrophilic isomer of the bromoheptapeptide has been shown to co-elute with the natural bromoheptapeptide (see Fig. 4B). The purified synthetic hydrophilic isomer of the N-terminal 1-4 fragment of the bromosleeper peptide has been shown to co-elute with the natural bromosleeper peptide 1-4 fragment (see Fig. 7B).
(iii) The purified hydrophilic synthetic isomer of the
bromoheptapeptide has been identified as the L conformation
on the basis of the ability of -chymotrypsin to cleave the
peptide (see Fig. 4C). The purified synthetic hydrophilic
isomer of the N-terminal 1-4 fragment of the bromosleeper peptide has
been identified as the L conformation on the basis of the
ability of aminopeptidase-M to cleave the N-terminal residue from the
tetrapeptide (see Fig. 7C), and the fragment was observed to
co-elute with the racemic mixture of 6-bromotryptophan under
conditions that distinguish this amino acid from 5-bromotryptophan.
It is also noteworthy that the sequence of a cDNA clone encoding the bromosleeper peptide from C. radiatus has been determined.4 The mature peptide purified from venom is encoded at the extreme C-terminal end of the predicted prepropeptide precursor. The bromotryptophan residue is encoded in the mRNA by the codon for tryptophan. We presume that the polypeptide precursor for the bromosleeper peptide has a normal L-tryptophan after the primary translation event. A modification system then specifically brominates Trp (1) of the bromosleeper peptide (most probably this modification takes place before the mature peptide is proteolytically cleaved from the precursor) resulting in a L-6-bromotryptophan residue.
Brominated Conus Peptides in the General Context of Brominated Amino Acids and Natural ProductsA wide variety of haloperoxidases are known that can brominate tyrosine residues in humans and animals, including myeloperoxidases and lactoperoxidases (4). In addition, bromoperoxidases have been isolated from several species of algae (4,36).
Post-translationally iodinated (1, 37-40, 41), chlorinated (42-44), and brominated (45,1 44) tyrosine residues have been isolated from a variety of marine specimens. Although it has been suggested that there must be other halogenated amino acid residues than tyrosine in sponges, none have been positively identified.
The bromination of tryptophan or its derivatives appears to occur widely in marine organisms. Brominated indole derivatives have been characterized in a wide variety of marine natural products over a broad phylogenetic range (from marine algae to vertebrate systems). The remarkable diversity of marine natural products containing indole derivatives is briefly summarized in Table II (see Ref. 46 for other brominated marine products). Of the brominated compounds isolated from marine products, only jaspamide (47), eusynstyelamide (48), halocyamine A, and halocyamine B (49) contain brominated indole groups within a peptidic framework. Jaspamide is a metabolite of mixed peptide polyketide biosynthetic origin which has been proposed as a cyclic depsipeptide made up of 3 amino acids and an octyl ketide group (47). Eusynstyelamide is an extremely polar molecule isolated after methanol extraction which has been proposed to be a highly modified peptide dimer where each monomer is made up of two modified amino acids and a guanidinyl-amide group (41). Halocyamine A and B are modified peptidic structures where both (A and B) contain three residues, 2 of which are common amino acids (49). The structure of the L-6-bromotryptophan amino acid observed in the bromoheptapeptide and the bromosleeper differs from the D-N-methyl-2-bromotryptophan in jaspinamide, the bromoindoyl group in eusynstyelamide and the modified bromodidehydrotryptamine found in the halocyamines. However, the major difference is that neither jaspinamide, eusynstyelamide, nor the halocyamines are purely peptidic structures. Although the cyclic structure of jaspinamide does incorporate one other common amino acid (alanine), it is better described as a hybrid polyketide/polypeptide. Eusynstyelamide is also not a true peptide structure, and although a case can be made that it incorporates a modified arginine amino acid and modified tryptophan, the structure is more correctly a bromoindoyl-succinic acid-guanidinyl-amide. The halocyamines A and B are closest in structure to peptidic, containing histidyl, threonyl, glycy, and dihydroxy phenylalanyl residues linked at the C terminus to the 6-bromo-8,9-didehydrotryptamine group. However, the bromodidehydrotryptamine is a C-terminal modification extending a tripeptide rather than a fourth amino acid. Thus, neither jaspinamide, eusynstyelamide, nor the halocyamines are the result of mRNA transcription, and therefore the resulting modified bromoindole groups present in these molecules cannot be considered as proteinogenous amino acids. With the exception of D-N-methyl-2-bromotryptophan, all of the molecules listed in Table II involve bromine substitution at position 6 (and in some cases at additional sites) of the indole ring. On the basis of these observations a general rule for incorporation of bromine at position 6 in marine organisms has been proposed (50).
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Some of the great diversity of marine natural products containing brominated indole derivatives are likely to be defensive compounds with strong pharmacological activity, particularly those from sessile marine organisms which rely strongly on their chemical defenses. Thus, although bromination has been reported from a very diverse group of biologically active compounds, it has not previously been demonstrated that a brominated tryptophan occurs in a regular polypeptide structure. However, given that the cone snails have developed an amazing brew of potent antagonists, it is perhaps not surprising that as marine organisms, they have recruited bromination as a means of increasing their peptidic repertoire. In effect, they may have recruited bromination in much the same way as other marine organisms have used bromination for generating pharmacologically active natural products.
Thus, if the cone snails have indeed evolved bromination of tryptophan as a novel adaptation in their venom ducts, it would not be difficult to see potential intermediate steps in the generation of such a system. The broad distribution of brominated natural products in the marine environment presumably arises through a broad spectrum of bromo- and lactoperoxidases in marine organisms. If a bromoperoxidase were recruited to become sequence-specific, it would become a post-translational modification enzyme, only catalyzing the bromination of specific tryptophan residues in a polypeptide structure, such as apparently occurs for the bromosleeper peptide. Thus the occurrence of L-6-bromotryptophan in Conus peptides could be due to an adaptation involving the recruitment of an enzymatic system already generally distributed among marine organisms; the cone snails have used this more general bromination chemistry evolved in marine ecosystems in a specialized way in their venom ducts.
We are grateful to Ferring Research Institute (San Diego, CA) for access to the electrospray mass spectrometer.