From the Institute for Molecular Bioscience, Australian Research Council Centre for Functional and Applied Genomics, University of Queensland, Brisbane, 4072 Queensland, Australia
Received for publication, October 13, 2002, and in revised form, December 9, 2002
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ABSTRACT |
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The plant cyclotides are a fascinating family of
circular proteins that contain a cyclic cystine knot motif. The
knotted topology and cyclic nature of the cyclotides pose interesting
questions about folding mechanisms and how the knotted arrangement of
disulfide bonds is formed. In the current study we have examined the
oxidative refolding and reductive unfolding of the prototypic
cyclotide, kalata B1. A stable two-disulfide intermediate accumulated
during oxidative refolding but not in reductive unfolding. Mass
spectrometry and NMR spectroscopy were used to show that the
intermediate contained a native-like structure with two native
disulfide bonds topologically similar to the intermediate isolated for
the related cystine knot protein EETI-II (Le-Nguyen, D., Heitz, A.,
Chiche, L., El Hajji, M., and Castro B. (1993) Protein Sci.
2, 165-174). However, the folding intermediate observed for kalata B1
is not the immediate precursor of the three-disulfide native peptide
and does not accumulate in the reductive unfolding process, in contrast
to the intermediate observed for EETI-II. These alternative pathways of
linear and cyclic cystine knot proteins appear to be related to the
constraints imposed by the cyclic backbone of kalata B1 and the
different ring size of the cystine knot. The three-dimensional
structure of a synthetic version of the two-disulfide intermediate of
kalata B1 in which Ala residues replace the reduced Cys residues
provides a structural insight into why the two-disulfide intermediate
is a kinetic trap on the folding pathway.
The cyclotide family comprises macrocyclic peptides that are ~30
residues in length and incorporate a knotted topology of disulfide
bonds formed between six conserved cysteine residues (1, 2). They are
interesting both structurally and functionally as they represent the
largest family of naturally occurring circular proteins (3). Further, a
diverse range of biological functions have been reported for these
peptides, including uterotonic activity (4), inhibition of neurotensin
binding (5), hemolytic (6, 7), anti-HIV (8), anti-microbial (7) and
insecticidal activity (9), as well as trypsin inhibitory activity
(10).
Cyclotides have been isolated from various species in the Rubiaceae,
Violaceae, and Cucurbitaceae plant families. The three-dimensional structures of four members of the family (kalata B1, Ref. 11; circulin
A, Ref. 12; cycloviolacin O1, Ref. 1; and MCoTI-II, Refs. 13 and 14),
have been elucidated using NMR spectroscopy and have revealed the
presence of a motif termed the cyclic cystine knot
(CCK)1 (1). The major
structural features of the motif are a cyclic backbone, a distorted
triple stranded The first cyclotides discovered fell into two distinct subfamilies
based on sequence similarities within, but not between, the
subfamilies. These were termed the Möbius and bracelet
subfamilies based on topological considerations (1), and comprised
peptides isolated from the Rubiaceae and Violaceae plant families. A
third subfamily has now been proposed based on a determination of the three-dimensional structure of MCoTI-II (13). This macrocyclic trypsin
inhibitor was discovered in the seeds of a plant from the
Cucurbitaceae, or squash, family (10), and its structure contains the
CCK motif (13, 14) seen in the previously reported cyclotides despite
having no sequence homology except for the six cysteine residues.
Acyclic forms of squash trypsin inhibitors have been known for many
years and include EETI-II (17) and CMTI-I (18). The structures (19, 20)
of these molecules are very similar to that determined for MCoTI-II,
apart from the cyclic backbone. Interestingly, no acyclic forms of the
cyclotides from the Rubiaceae and Violaceae plant families have been
found. A sequence comparison of kalata B1, MCoTI-II, and EETI-II is
given in Fig. 1 and illustrates the common cystine knot motif in the
three molecules. Fig. 1 also defines and highlights the diversity of
the backbone loops, defined as the regions between successive Cys
residues in these peptides. Owing to their cyclic nature kalata B1 and
MCoTI-II have six loops while the acyclic homologue EETI-II has five
loops. In the current study it was of interest to compare the oxidative
folding of kalata B1 with those of linear cystine knot peptides such as
EETI-II because they have some interesting topological similarities and differences.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-sheet and a cystine knot arrangement of the three
disulfide bonds. The cystine knot comprises an embedded ring formed by
disulfide bonds I-IV and II-V that is threaded by the III-VI
disulfide bond. This knotted topology was originally determined for
kalata B1 using NMR data (11) but the corresponding disulfide
connectivity of other members of the cyclotide family has since been
confirmed by synthetic methods involving directed disulfide bond
formation (7, 15). Despite this, a recent study based primarily on
analysis of local NOE patterns (16) suggested that an alternative,
non-knotted disulfide bonding pattern may be possible for kalata B1.
The present study provides additional evidence in favor of the
originally proposed knotted topology.
View larger version (19K):
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Fig. 1.
Amino acid sequences of kalata B1, MCoTI-II,
and EETI-II. The first two are cyclic cystine knot peptides while
the latter is a linear cystine knot. The disulfide connectivity of all
three is similar. Loops in the peptide backbone between successive
cysteines are numbered for reference in the text.
The cyclotides have recently been shown to be translated gene products (9) that are processed from linear precursor proteins; however, the mechanism of cyclization, and the folding pathways required to achieve the correct three-dimensional shape and disulfide bond connectivity are yet to be elucidated. Examination of the gene sequence suggests that loop 6 is where cyclization occurs and this is consistent with expectations based on a sequence comparison of cyclotides with acyclic cystine knot proteins such as EETI-II (Fig. 1). Effectively, loop 6 may be regarded as the linker region that is clasped together to form the cyclic peptide backbone.
The cyclic nature and knotted topology of the cyclotides gives them remarkable stability and there is much interest in determining how the unique knotted fold is formed. We have previously shown that prior cyclization of kalata B1 appears to facilitate oxidative folding into the native conformation (6). An acyclic form of kalata B1 required a hydrophobic solution environment to produce significant amounts of the correctly folded form, whereas the cyclic form folded efficiently into the native isomer in aqueous solution. We have also explored the importance of the cyclic backbone in the folding of cyclotides by synthesizing all of the topologically distinct acyclic permutants (21). This is equivalent to opening the backbone of kalata B1 in each of the six loops between successive Cys residues. We found that four of six permutants folded into native-like conformations, but two did not; these were precisely the two that involved breaking the embedded ring of the cystine knot. That study showed that a native-like fold can be produced without the cyclic backbone, but highlighted the importance of the cystine knot in forming the native conformation.
In the current study we have examined the oxidative refolding and
reductive unfolding of kalata B1 and characterized a major folding
intermediate. The properties of this intermediate, when compared with a
topologically similar intermediate characterized for EETI-II (22),
reveal fundamental differences in the folding pathways of cystine knot
proteins with cyclic backbones relative to those with conventional,
acyclic, backbones. Part of the study required the synthesis of a
mutant in which a single disulfide bond is removed and we show that
this adopts a native-like fold, consistent with expectations from the
identified folding intermediate.
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EXPERIMENTAL PROCEDURES |
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Isolation of Kalata B1-- Kalata B1 was extracted from the above ground parts of Oldenlandia affinis with dichloromethane/methanol (1:1; v/v) overnight at room temperature. The extract was partitioned with chloroform and water and the water/methanol layer concentrated on a rotary evaporator prior to lyophilization. The dried product was re-dissolved in H2O and purified using preparative RP-HPLC on a C18 column (Vydac) at 8 ml/min. Masses were analyzed using an ES-TOF Micromass LCT mass spectrometer.
Reductive Unfolding-- Kalata B1 (0.5 mg/ml) was dissolved in 0.1 M ammonium bicarbonate, pH 8.5, containing varying concentrations of dithiothreitol (DTT) or TCEP (0.5-300 mM). To monitor the unfolding, aliquots were removed at various time intervals and quenched with 4% aqueous trifluoroacetic acid. Samples were analyzed using RP-HPLC and LCMS. A large-scale reduction was performed for the subsequent oxidative refolding experiments. Kalata B1 was reduced with an excess of DTT (1 M) in ammonium bicarbonate (pH 8.5) at room temperature for 2 h. The reduced material was purified on semi-preparative RP-HPLC at 3 ml/min.
Oxidative Refolding--
Large scale refolding reactions were
performed in 50% isopropyl alcohol (v/v) in 0.1 M ammonium
bicarbonate, pH 8.5 and 1 mM reduced glutathione. To
isolate the folding intermediate the refolding reaction was allowed to
proceed for 15 min and then immediately purified on a semi-preparative
reverse phase column. Following purification the fractions were
lyophilized and stored at 20 °C. Small scale reactions were
performed under various solution conditions and analyzed by RP-HPLC and
mass spectrometry.
Synthesis of [Ala1,15]Kalata B1-- [Ala1,15]Kalata B1 was synthesized using a native chemical ligation strategy. This methodology requires the synthesis of a linear precursor peptide containing an N-terminal Cys residue. This forms a thioester with a functionalized C terminus and subsequently undergoes an S,N acyl migration to form a native peptide bond in the resultant circular protein. Of the four possible Cys residues in the di-Ala mutant peptide, Cys5 was chosen as the N-terminal residue. The linear precursor was synthesized using solid phase peptide synthesis with BOC/HBTU chemistry and cleaved from the resin with HF. The cyclization reaction was performed in 0.1 M sodium phosphate (pH 7.4) with an excess of TCEP over a period of ~30 min. The cyclic reduced precursor was then oxidized in 0.1 M ammonium bicarbonate, pH 8.5, 50% v/v isopropyl alcohol and 1 mM reduced glutathione at room temperature overnight. The peptide was purified as described above.
NMR Spectroscopy--
Samples for 1H NMR
measurements contained ~1 mM peptide in 90%
H2O/10% 2H2O (v/v) at ~pH 3. D2O (99.9% and 99.99%) was obtained from Cambridge Isotope Laboratories, Woburn, MA. Spectra were recorded at 290 and 298 K on a Bruker ARX-500 or Bruker DMX 750 spectrometer equipped with a
shielded gradient unit. two-dimensional NMR spectra were recorded in
phase-sensitive mode using time-proportional phase incrementation for
quadrature detection in the t1 dimension (23). The two-dimensional experiments consisted of a TOCSY (24) using a
MLEV-17 spin lock sequence (25) with a mixing time of 80 ms, DQF-COSY
(26), ECOSY (27), and NOESY (28) with mixing times of 100-250 ms.
Solvent suppression was achieved using a modified WATERGATE sequence
(29). Spectra were acquired over 6024 Hz with 4096 complex data points
in F2 and 512 increments in the F1 dimension.
3JNH-H coupling constants were measured from
a one-dimensional spectrum or from the DQF-COSY spectrum.
Spectra were processed on a Silicon Graphics Indigo work station using XWINNMR (Bruker) software. The t1 dimension was zero-filled to 2048 real data points, and 90° phase-shifted sine bell window functions were applied prior to Fourier transformation. Chemical shifts were referenced internal sodium 2,2-dimethyl-2-silapentane-5-sulponate.
Structure Calculations--
Preliminary structures of
[Ala1,15]kalata B1 were calculated using a torsion angle
simulated annealing protocol within the program DYANA (30). Final
structures were calculated using simulated annealing and energy
minimization protocols within CNS version 1.0 (31). The starting
structures were generated using random (,
) dihedral angles and
energy-minimized to produce structures with the correct local geometry.
A set of 50 structures was generated by a torsion angle
simulated-annealing protocol (32, 33). This protocol involves a
high-temperature phase comprising 4000 steps of 0.015 ps of torsion
angle dynamics, a cooling phase with 4000 steps of 0.015 ps of torsion
angle dynamics during which the temperature is lowered to 0 K, and
finally an energy minimization phase comprising 500 steps of Powell
minimization. Structures consistent with restraints were subjected to
further molecular dynamics and energy minimization in a water shell, as
described by Linge and Nilges (34). The refinement in explicit water
involves the following steps. First, heating to 500 K via steps of 100 K, each comprising 50 steps of 0.005 ps of Cartesian dynamics. Second,
2500 steps of 0.005 ps of Cartesian dynamics at 500 K before a cooling
phase where the temperature is lowered in steps of 100 K, each
comprising 2500 steps of 0.005 ps of Cartesian dynamics. Finally, the
structures were minimized with 2000 steps of Powell minimization.
Structures were analyzed using PROMOTIF (35) and PROCHECK-NMR (36).
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RESULTS |
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The cyclotides provide a unique opportunity to examine the folding
of the cystine knot motif in the presence of a constrained backbone. In
the current study we chose the prototypic cyclotide kalata B1 to probe
oxidative refolding and reductive unfolding. We have previously shown
that reduced cyclic kalata B1 can be very efficiently refolded into the
native conformation (6) under appropriate conditions. Refolding was
performed in 50% isopropyl alcohol (v/v) in 0.1 M ammonium
bicarbonate, pH 8.5 and 1 mM reduced glutathione at room
temperature overnight, and essentially only one product was obtained
(6). In the current study the oxidative folding reaction was monitored
by removing aliquots at selected time points and analyzing them with
RP-HPLC. Fig. 2a shows the RP-HPLC traces for a time-course carried out over 10 h for kalata B1. In contrast to what is typically observed for the refolding of most
peptides native oxidized kalata B1 elutes significantly later than the
reduced peptide. This is most likely because of the patch of
hydrophobic residues that becomes surface exposed upon correct folding
(6), which provides a characteristic marker of the native folded
compound.
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In addition to the late eluting native peak, there are several peaks that elute with retention times close to that of the reduced cyclic peptide. LCMS confirmed that these peaks correspond to partially oxidized forms but peak overlap prevented their definitive characterization. Between the two extremes of the reduced and native forms there is an additional sharp, well-resolved peak that is detectable minutes after starting the refolding reaction (intermediate IIa in Fig. 2a). Its relatively late retention time suggests a conformation not dissimilar from the native form.
To determine if the presence of this well resolved folding intermediate was dependent on the refolding conditions several oxidation reactions were performed under various solution conditions (results not shown). Oxidation of reduced, cyclic kalata B1 in 0.1 M ammonium bicarbonate alone produces a small amount of the well-resolved intermediate and native peptide within 15 min. The percentage of the native product is markedly increased in the presence of reduced glutathione. Inclusion of guanidine hydrochloride in the buffer prevented folding into the native conformation and there was also no evidence for the folding intermediate. These results suggest that reduced glutathione aids refolding by allowing disulfide shuffling, while denaturing agents prevent native-like interactions that are required for folding to occur.
Isolation and Identification of the Major Folding Intermediate-- Folding intermediates for model disulfide-rich peptides such as BPTI and lysozyme have been extensively studied (37, 38). It has been shown that quenching oxidative folding reactions with acid does not result in significant intramolecular disulfide rearrangement even after delays of several hours (38). In accordance with these findings, we used an acid quench method in our studies to prevent disulfide rearrangement.
Large scale oxidative refolding reactions were used to purify the folding intermediate of kalata B1. Reactions were left for ~15 min, quenched with acid and then immediately purified using semi-preparative RP-HPLC. The early eluting intermediates were not purified to homogeneity and the main focus was on the well resolved intermediate. This intermediate was purified, and an accurate molecular mass (2894 ± 0.1 Da) was determined using electrospray mass spectrometry. The molecular mass was consistent with a peptide with two disulfide bonds intact and one bond reduced.
Reductive Unfolding of Kalata B1-- The reductive unfolding of kalata B1 was examined using both DTT and TCEP as reducing agents in the presence and absence of isopropyl alcohol. Isopropyl alcohol did not appear to influence the reactions. The reactions performed at various concentrations of DTT (5-100 mM) at pH 8.5 essentially show only reduced and fully oxidized species with no significant accumulation of any partially reduced species (Fig. 2b). However, lowering the pH to 4.5 and using TCEP (5-300 mM) as the reductant revealed the presence of minor components along the unfolding pathway (Fig. 2c). LCMS analysis allowed determination of the mass of the two most abundant intermediates shown in Fig. 2c, which correspond to a one-disulfide (Ia) and a two-disulfide (IIb) species. A very minor peak was consistently observed in the reductive unfolding at the retention time observed for intermediate IIa. Isolation of this peak from RP-HPLC and mass spectrometry confirmed that the mass was consistent with intermediate IIa.
Structural Characteristics of the Major Oxidative Folding
Intermediate of Kalata B1--
To further characterize the
intermediate IIa the peak was isolated from RP-HPLC and examined using
NMR spectroscopy. A TOCSY spectrum was recorded immediately after
dissolution in 10% 2H2O/90% H2O
and revealed a very well dispersed spectrum consistent with a single
solution conformation. A NOESY spectrum recorded later had lower signal
intensity than that expected based on the signal intensity of the TOCSY
spectrum. This appears to be a result of the sample aggregating over
time and was confirmed by re-recording additional one-dimensional
spectra. A one-dimensional spectrum recorded immediately after
dissolution of the sample and one recorded 24 h later highlights
the changes that occur (Fig.
3a).
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Despite the instability of the sample there was still sufficient
information gained from the TOCSY/NOESY spectra to assign the peaks in
IIa (Fig. 3b). A comparison of the H chemical shifts of
the intermediate with the native peptide is shown in Fig.
4a and reveals that IIa has a
native-like structure. The only significant differences occur near
residue Cys1, suggesting that the disulfide bond involving
this residue is perturbed (absent) in the intermediate.
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An analysis of the H chemical shift differences between the native
kalata B1 and IIa further confirmed the identity of the reduced
cysteine residues. The separation of the
-proton chemical shifts
(
) for four of the six cysteine residues is very similar in
the native peptide and in IIa (Fig. 4b). However,
Cys1 and Cys15 are both affected significantly.
In the native peptide the
values for Cys1 and
Cys15 are 0.35 and 1.2 ppm, respectively, but in IIa they
fall to 0.0 and 0.3 ppm, which suggests an altered conformation for
these two residues. Furthermore, the direction of the change,
i.e. toward a decreased chemical shift separation suggests a
less structured local conformation. Thus, it appears that IIa contains
a native-like structure with the two native disulfide bonds
Cys5-Cys17 and
Cys10-Cys22 intact, but with Cys1
and Cys15 in the reduced state. The location of the reduced
disulfide bond is highlighted in Fig. 4c.
Analysis of the NMR sample of IIa by RP-HPLC after 24 h in solution revealed a trace very similar to that seen in Fig. 2a at 10 min. This suggests that the intermediate does not directly convert to the native product with time but equilibrates via the earlier eluting forms. Refolding reactions on the isolated IIa were performed to further examine the folding properties of kalata B1. Dissolving the purified intermediate in the oxidation buffer used to fully refold kalata B1 (0.1 M ammonium bicarbonate, pH 8.5, 50% isopropyl alcohol (v/v) and 1 mM reduced glutathione) (6), resulted in a small percentage of the earlier eluting peaks. The intermediate was initially retained but a significant amount of the native peptide was formed over a 6-h period. However, when the buffer was changed to 0.5 M GnHCl in 0.05 M potassium phosphate, pH 7.8, the majority of the intermediate converted to the early eluting forms and over a 6-h period only a small percentage of native peptide was formed. Both of these reactions were performed in the presence of reduced glutathione. When the purified intermediate was placed in 0.1 M ammonium bicarbonate alone, similar profiles to the reaction containing denaturant were observed, where the majority of the intermediate converted to the early eluting forms and very little native peptide was formed over the time the reaction was monitored (6 h).
When IIa is incubated without isopropyl alcohol in the presence of reduced glutathione, once again the majority of the intermediate is converted into the early eluting forms but then native peptide is present within an hour. In contrast, when isopropyl alcohol is included with no reduced glutathione, the intermediate persists for longer and does not appear to convert to the native conformation, suggesting that disulfide reshuffling is required to attain the native conformation.
Three-dimensional Structure of [Ala1,15]Kalata
B1--
The instability of purified IIa over time prevented a complete
structural analysis. Therefore, to further structurally characterize the intermediate an analogue was synthesized with Cys1 and
Cys15 replaced with alanine residues. Assignments of
[Ala1,15]kalata B1 were made using established techniques
(39) and the 1H chemical shifts are supplied as
supplementary material. Chemical shifts in the amide region are well
dispersed and the large number of resolved cross peaks in the NOESY
spectrum allowed determination of a well defined structure. A
comparison of the secondary shifts of [Ala1,15]kalata B1
with IIa shown in Fig. 5a
highlights the similarities between the two molecules. The
shifts and retention times on RP-HPLC also show the similarities (Fig.
5, b and c). A slight change in
shifts
is observed for Cys5, suggesting minor differences for this
residue (Fig. 5b).
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The three-dimensional structure of [Ala1,15]kalata B1 was calculated with 321 distance restraints and 19 angle restraints using a simulated annealing protocol in CNS. The disulfide connectivities (Cys5-Cys17 and Cys10-Cys22) were also included as restraints in the structure calculations. The resulting family of structures had good structural and energetic statistics, as shown in Table I. A stereoview and ribbon representation of the secondary structure is shown in Fig. 6 along with a comparison with native kalata B1.
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Analysis of the structures with PROMOTIF (35) identified a type I
-turn between residues 5-8, a type II
-turn between residues
12-15, a type VIa1
-turn between residues 18-21, and a type I
-turn between residues 24-27. An anti-parallel
-sheet is
recognized between residues 16-18, 21-24, and 27-29, as shown in
Fig. 6b. Residues 16-18 and 21-24 constitute the
-hairpin that is often present in cystine knot proteins. The
disulfide bond between Cys10 and Cys22 is
characterized as a left-handed spiral, however the disulfide bond
between residues Cys5 to Cys17 did not fall
into one of the established classifications of disulfide bond
geometries (35).
Given the recent suggestion that kalata B1 may not contain
a cystine knot (16), but rather a Cys 1-22, 5-17, 10-15 disulfide connectivity it was of interest to examine the structures of the other
theoretically possible disulfide connectivities of
[Ala1,15]kalata B1 (i.e.
Cys5-Cys10,
Cys17-Cys22, and
Cys5-Cys22,
Cys10-Cys17). Structures were thus calculated
in which these two alternative disulfide connectivities were included
as restraints. The energies associated with the experimental
constraints, provided as supplementary material, are significantly
lower (more favorable) for the Cys5-Cys17 and
Cys10-Cys22 connectivity than the two
alternative connectivities. Thus a side benefit of the synthetic mutant
is that it was able to provide strong evidence in favor of the
originally proposed knotted topology of kalata B1. Since the mutant
contains only two disulfide bonds it must adopt one of only three
possible disulfide isomers (relative to the 15 isomers possible for a
three-disulfide species), and thus it provides a convenient model
system for confirming the native disulfide connectivity.
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DISCUSSION |
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The cyclotides have only recently been discovered but represent a structurally fascinating class of miniproteins with important biological functions including antimicrobial and insecticidal activity (40, 41). Little is known about the in vivo folding and biosynthesis of these molecules but the present study has provided an insight into the in vitro folding of kalata B1 and into the intricacy of the folding pathways of cystine knot proteins. We have shown that a native-like two-disulfide intermediate is present during oxidative refolding but does not accumulate to a significant extent in the reductive unfolding of kalata B1. Chemical shift analysis of the isolated intermediate, IIa, revealed a native-like three-dimensional fold and strongly suggested the presence of two-native disulfide connectivities (Cys5-Cys17 and Cys10-Cys22). This connectivity and the native-like structure of the intermediate were confirmed by a three-dimensional structural analysis of an analogue of the intermediate, [Ala1,15]kalata B1.
In addition to providing valuable new information on the folding pathway of kalata B1, [Ala1,15]kalata B1 provides strong support for the originally proposed disulfide connectivity of kalata B1. Skjeldal et al. (16) recently suggested that kalata B1 may have a disulfide connectivity of 1-22, 5-17, and 10-15, (based on the numbering in Fig. 1) rather than the originally proposed knotted connectivity (1-15, 5-17 and 10-22) (11). Clearly, the disulfide bonds 1-22 and 10-15 are not possible in [Ala1,15]kalata B1 and given the highly native-like conformation of this analogue it appears that the originally proposed connectivity is correct. Furthermore, the calculation of alternative structures of [Ala1,15]kalata B1 with the three possible two-disulfide connectivities strongly supports the knotted topology. Indeed the suggestion by Skjeldal et al. of a different disulfide connectivity for kalata B1 was somewhat surprising given a range of supporting evidence for the originally proposed connectivity for other members of the cyclotide family, including that from directed chemical synthesis of circulin, A and circulin B and cyclopsychotride A (7, 15) and mass spectral analysis of the circulins (42). A recent high resolution structural analysis of kalata B1 has further supported the original disulfide assignment (43).
Despite the native-like overall structure of IIa it appears that direct formation of the final disulfide bond does not occur directly from this intermediate and that a structural rearrangement may be required to form the native conformation. Refolding of the purified intermediate is greatly facilitated by reduced glutathione, suggesting that disulfide bond reshuffling is required. A predominant folding intermediate that does not readily form the native peptide has also been observed for human epidermal growth factor (EGF), a 53-residue protein containing three-disulfide bonds. In that case a stable intermediate (EGF-II) containing two of the three native disulfide bonds was isolated along the oxidative folding pathway and shown to be a major kinetic trap in the folding. Formation of the third disulfide bond did not occur directly and it appeared that the native structure was accessed instead via three-disulfide scrambled isomers (44). It appears that a similar situation applies for kalata B1, except that the native structure is accessed by an alternative two-disulfide intermediate.
Structural analysis of [Ala1,15]kalata B1 provides a
possible explanation for why IIa accumulates as a kinetic trap in the
oxidative refolding reactions and does not readily form the native
peptide. The three-dimensional structure of
[Ala1,15]kalata B1 is very similar to the native
peptide but a surface analysis of the structure reveals that the side
chain of Ala1 is solvent exposed (Table
II) and not in close proximity to Ala15 (Fig. 7). The most significant
differences between native kalata B1 and [Ala1,15]kalata
B1, in both chemical shifts and in three-dimensional structure, occur
near Cys1/Ala1. In particular, the chemical
shift of proline 28 H is shifted significantly upfield compared with
the native peptide. This shift is seen in both
[Ala1,15]kalata B1 and in the intermediate IIa,
suggesting that the differences observed in this region of
[Ala1,15]kalata B1 are also present in IIa. Consequently,
Cys1 in IIa may be distant from Cys15, thereby preventing direct
oxidation of the final disulfide bond. It would appear that to lead to
a productive intermediate this disulfide bond must be formed before the
other two are locked in place, to avoid its constituent Cys residues
being placed in an unfavorable geometric arrangement.
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The accumulation of intermediates in the reductive unfolding of kalata B1 is influenced by the pH of the reaction. When the reduction was performed at pH 8.5 with DTT there was no significant accumulation of intermediates (Fig. 2b). However at pH 4.5, using TCEP, intermediates were observed (Fig. 2c). These intermediates do not accumulate to a significant extent relative to the levels observed in the oxidative refolding (Fig. 2a). The two most significant peaks have retention times very close to the reduced species, suggesting a non-native three-dimensional structure. However, it can be assumed that the disulfide connectivities are native, based on the low level of disulfide reshuffling that occurs at low pH (45). These peaks were shown to correspond to a one-disulfide and two-disulfide species based on LCMS analysis (Fig. 2c). Trace amounts of IIa were also observed in the TCEP reduction. The observation of two intermediates containing two disulfide bonds (IIa and IIb) suggests that reduction of kalata B1 may occur via multiple pathways. Clearly, IIb represents a more populated pathway than that involving IIa, and we propose here that this reflects a kinetic preference for this intermediate. Parallel unfolding pathways have previously been observed for ribonuclease A, a protein containing four disulfide bonds. Two well-populated pathways were observed in the unfolding reaction in that case (46).
The accumulation of IIa during oxidative refolding is consistent with
it having both a favorable low energy conformation and a high energy
barrier between it and the native peptide as schematically represented
in Fig. 8. The conformational
rearrangement required to form the native peptide would account for the
high energy barrier for conversion to fully oxidized kalata B1. The low
level of IIa in the reductive unfolding is also consistent with a
high-energy barrier for the reverse process (i.e. reduction
of native kalata B1 to IIa). The latter may reflect steric hindrance to
access of reducing agents to the Cys1-Cys15
disulfide bond because of the cyclic backbone. The observation of IIb
in the reductive unfolding suggests that it is accessed via a lower
energy barrier, however the non-native structure of IIb, based on the
retention time being close to the reduced rather than native
conformation, suggests that it is of higher energy than IIa. At this
stage the direct precursor to kalata B1 is uncertain, however the
observation of IIb in the reductive unfolding implies that it is a
likely candidate. Further, it is likely that the Cys5-Cys17 bond is reduced in this
intermediate but it was not possible to isolate sufficient quantities
to definitively confirm this. However, a consideration of the degree of
surface exposure of the Cys residues in native kalata B1 strongly
supports this suggestion. The percentage surface exposure of the sulfur
atoms in native kalata B1 and [Ala1,15]kalata B1 is given
in Table II. Cys17 is the only cysteine residue to have a
significant degree of surface exposure, as is further highlighted in
Fig. 7. Thus, the disulfide bond involving Cys17
(i.e. CysII-CysV in the generic cystine knot numbering
scheme of Fig. 1), is likely to be the most susceptible to reduction and to be the bond broken in IIb.
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Comparison of the folding intermediates characterized for kalata B1 and EETI-II reveals that they are topologically equivalent as both lack the I-IV disulfide bond and contain II-V and III-VI disulfide bonds. On this basis it might be thought that the folding pathways are similar. However, when the rate of conversion to the native peptide and the reductive unfolding of kalata B1 and EETI-II are considered it is apparent that the pathways are clearly different. These pathways are schematically represented in Fig. 8b. The two-disulfide intermediate of kalata B1, IIa, does not appear to be the immediate precursor of the native peptide and is only weakly detected during reductive unfolding. In contrast, the predominant intermediate in the folding of EETI-II was proposed to be a direct precursor of the native form, based on the absence of any other intermediates observed in the NMR sample, which showed the presence of both intermediate and native forms after incubation for several weeks (22). Furthermore, the EETI-II intermediate was also present during reductive unfolding (22). Thus, despite the presence of topologically equivalent intermediates in the oxidative refolding of kalata B1 and EETI-II there appears to be alternative folding pathways for these cystine knot proteins.
The alternative folding pathways observed for kalata B1 and EETI-II are likely to be related to structural differences between the molecules. The most obvious differences are the cyclic backbone and the size of the ring comprising the cystine knot. Kalata B1 contains eight residues in the knot whereas EETI-II contains twelve. The restraints of the cyclic backbone and the smaller ring size may increase the stability of intermediate IIa and disfavor its conversion to the native conformation without rearrangement of the two already formed disulfide bonds. Similarly, the susceptibility of individual disulfide bonds to reduction may be affected by the added constraints of the cyclic backbone in the cyclotides. In particular the linker region that cyclizes kalata B1 is in close proximity to the Cys1-Cys15 disulfide bond (arrow A in Fig. 8b). By contrast, the corresponding bond is much more exposed in EETI-II (arrow B in Fig. 8b). In summary, the cyclic backbone and compact structure of kalata B1 appears to have a significant influence on how the disulfide bonds are stabilized.
Previous studies have highlighted the diversity of disulfide folding pathways of disulfide-rich proteins, but a general correlation between the reductive unfolding and oxidative refolding pathways of proteins has been suggested (47). Reduction of disulfide bonds in a simultaneous manner is often associated with a high degree of heterogeneity of folded intermediates, whereas sequential reduction of the disulfide bonds is associated with predominant intermediates with native-like structures. The results from the reductive unfolding of kalata B1 at high pH with DTT suggest that the disulfide bonds are reduced in a simultaneous manner under these conditions. However, the reduction at lower pH with TCEP suggests a sequential pathway with the accumulation of both a two-disulfide and one-disulfide intermediate. The sequential pathway is consistent with the general correlation mentioned above as kalata B1 has a predominant intermediate during oxidative refolding. However, the current study has emphasized the differences in folding pathways between linear and cyclic cystine knot peptides even when common intermediates are observed.
The folding pathway of the cystine knot-containing glycoprotein hormone
-subunit has recently been examined using transiently transfected
cells labeled with [35S]cysteine (48). Glycoprotein
hormone
-subunit is a member of the growth factor cystine knot
family that is topologically distinct from the cyclotides and EETI-II,
which belong to the inhibitor cystine knot family (49, 50). Although
the connectivities are identical, the penetrating disulfide bond is
I-IV in the growth factor cystine knots instead of III-VI in the
inhibitor cystine knots (50). The study by Darling et al.
(48) indicated that folding proceeds through only one detectable
intermediate that was determined to be a one-disulfide species
containing the CysII to CysV disulfide bond.
Through a series of experiments involving analogues containing Ala
residues in place of selected cysteine residues it was established that
the order of disulfide bond formation was
CysII-CysV,
CysI-CysIV, followed by
CysIII-CysVI. The presence of only one
detectable disulfide intermediate containing one disulfide bond is in
contrast to kalata B1 and EETI-II and suggests that parallels cannot be
drawn between the folding of the two different families of cystine knots.
In conclusion, a native-like intermediate accumulates in the oxidative
refolding of kalata B1 but is only a trace component in the reductive
unfolding. This intermediate appears to be a kinetic trap and not the
immediate precursor to the native structure. Despite the topological
and structural similarities in the intermediates characterized for
kalata B1 and the related cystine knot peptide EETI-II there appears to
be alternative pathways in the folding of these peptides. The cyclic
backbone of kalata B1 has a significant influence on the folding and in
particular on the unfolding pathway. Furthermore, besides differences
in the folding of cyclic and linear cystine knot peptides, it appears
that inhibitor and growth factor cystine knots follow different folding pathways.
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ACKNOWLEDGEMENT |
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We thank Ulf Goransson for helpful comments.
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FOOTNOTES |
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* This work was supported in part by a grant from the Australian Research Council (to D. J. C.).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
The on-line version of this article (available at
http://www.jbc.org) contains supplementary materials.
The atomic coordinates and the structure factors (code 1N1U) have been deposited in the Protein Data Bank, Research Collaboratory for Structural Bioinformatics, Rutgers University, New Brunswick, NJ (http://www.rcsb.org/).
An Australian Research Council Senior Fellow. To whom
correspondence should be addressed. Tel.: 61-7-3365-4945; Fax:
61-7-3365-2487; E-mail: d.craik@imb.uq.edu.au.
Published, JBC Papers in Press, December 12, 2002, DOI 10.1074/jbc.M210492200
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ABBREVIATIONS |
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The abbreviations used are: CCK, cyclic cystine knot; DTT, dithiothreitol; TCEP, Tris(2-carboxyethyl)phosphine; RP-HPLC, reversed-phase high performance liquid chromatography; LCMS, liquid chromatography mass spectrometry; TOCSY, two-dimensional total correlation spectroscopy; NOE, nuclear Overhauser effect; NOESY, two-dimensional NOE spectroscopy; DQF-COSY, double quantum filtered correlation spectroscopy; ECOSY, exclusive correlation spectroscopy; WATERGATE, water suppression by gradient-tailored excitation; RMSD, root mean square deviation.
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